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Benzene is the smallest of the organic aromatic hydrocarbons. It contains sigma bonds (represented by lines) and regions of high-pi electron density, formed by the overlapping of p orbitals (represented by the dark yellow shaded area) of adjacent carbon atoms, which give benzene its characteristic planar structure. Benzene (C 6 H 6 ) , simplest organic, aromatic hydrocarbon and parent compound of numerous important aromatic compounds . Benzene is a colourless liquid with a characteristic odour and is primarily used in the production of polystyrene . It is highly toxic and is a known carcinogen ; exposure to it may cause leukemia . As a result, there are strict controls on benzene emissions. The structure of benzene has been of interest since its discovery. German chemists Joseph Loschmidt (in 1861) and August Kekule von Stradonitz (in 1866) independently proposed a cyclic arrangement of six carbons with alternating single and double bonds. Kekule subsequently modified his structural formula to one in which oscillation of the double bonds gave two equivalent structures in rapid equilibrium . In 1931 American chemist Linus Pauling suggested that benzene had a single structure, which was a resonance hybrid of the two Kekule structures. Characteristics of benzene Modern bonding models (valence-bond and molecular orbital theories) explain the structure and stability of benzene in terms of delocalization of six of its electrons, where delocalization in this case refers to the attraction of an electron by all six carbons of the ring instead of just one or two of them. This delocalization causes the electrons to be more strongly held, making benzene more stable and less reactive than expected for an unsaturated hydrocarbon. As a result, the hydrogenation of benzene occurs somewhat more slowly than the hydrogenation of alkenes (other organic compounds that contain carbon-carbon double bonds), and benzene is much more difficult to oxidize than alkenes. Most of the reactions of benzene belong to a class called electrophilic aromatic substitution that leave the ring itself intact but replace one of the attached hydrogens. These reactions are versatile and widely used to prepare derivatives of benzene. Get exclusive access to content from our 1768 First Edition with your subscription. Subscribe today Experimental studies, especially those employing X-ray diffraction, show benzene to have a planar structure with each carbon-carbon bond distance equal to 1.40 angstroms (Å). This value is exactly halfway between the C=C distance (1.34 Å) and C—C distance (1.46 Å) of a C=C—C=C unit, suggesting a bond type midway between a double bond and a single bond (all bond angles are 120°). Benzene has a boiling point of 80.1 °C (176.2 °F) and a melting point of 5.5 °C (41.9 °F), and it is freely soluble in organic solvents, but only slightly soluble in water.
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Have you ever taken a bite from an apple and felt your mouth get itchy? Did a tasty banana cause your tongue to swell? If so, chances are you have oral allergy syndrome, or pollen-food allergy syndrome as it’s also known. It happens because your immune system can’t tell the difference between proteins in these foods and pollen. The symptoms are usually itching, tingling, and swelling, mostly to the mouth, lips, and throat. You Can Have It and Not Know It Oral allergy syndrome is common, says Robert Eitches, MD, attending physician at Cedars-Sinai Medical Center. He says he has about 500 patients who have it. But many who have it don’t know they do. A lot of people with pollen allergies know they can’t tolerate these foods, but they don’t make the connection between them and their allergies, he says. People find out when their allergy testing is negative for foods but positive for something like birch pollen, grass pollen, or ragweed pollen, Eitches says. "We’re just learning about the syndrome over the last 5 or 10 years," Eitches says. "I think it’s been around longer than we realized. It’s become more obvious in the last 2 or 3 years." Who Gets It? Oral allergy syndrome mostly affects teens and adults, though younger children sometimes get it, too. In most cases the reactions are mild and don’t last long. Symptoms usually show up right after you eat. But it could take up to an hour. What If My Reactions Are Severe? Treat it like a pollen allergy. Antihistamines, epinephrine (for severe reactions) and immunotherapy are three courses of action. But there isn’t a specific medication to treat oral allergy syndrome. In rare cases, it can cause a life-threatening reaction known as anaphylaxis. Symptoms may include: Shortness of breath Tightness in your throat Hives Vomiting Nausea Diarrhea Dizziness Call 911 if you have any of these signs. Your doctor can tell you if you’re at risk for anaphylaxis. He may prescribe an epinephrine auto-injector.
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We’ve all seen cell phone towers. At about 200 feet tall, they let us upload things and talk to people from a distance. Now, Notre Dame and the city of South Bend are collaborating to help you do this with cutting-edge technology. Studies show people ages 18 to 33 use their cell phones about 85 times every day. That’s about five hours! The city of South Bend and researchers at Notre Dame recognize the importance of cell phone usage, so they're teaming up for an opportunity to make it even better. “We think that we can be competitive and bring the "testbed" here, and what that means to the everyday person is that some really exciting things are going to be happening in the wireless space around them,” said J. Nicholas Laneman, Co-Director of the Wireless Institute and Professor of Electrical Engineering at the University of Notre Dame. “So this is a prototype base station, or access point, for Wi-Fi. The technology that we’re developing in collaboration with our industry partners allows Wi-Fi devices to talk to the access point simultaneously,” said Laneman. This just means their technology would make it so you won't have to try again and again uploading posts or sending messages in crowded areas like football games or concerts. “This testbed will put both Notre Dame and South Bend on the map,” said Laneman. Doctor Laneman also says it’s a chance to show what both parties can bring to the table. “Companies and also researchers can take their technologies out of the lab and test it at city scale,” said Laneman.
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Q: Using increment in ternary operator in C For the example, after I use int a = 5, b = 6; x = (a < b) ? a++ : b++; x gets the value of a, which is 5, and a increments to 6, which is expected. When I use a = (a < b) ? a++ : b++; After this line, a still remains 5. But a = (a++ < b++) ? a : b; a is now 6. Why is this happening and why isn't increment operator executed in the first case? EDIT: Just to clarify, I'm asking why this happens when I'm using these lines separately, one by one, not all three in the same time. A: a = (a < b) ? a++ : b++; here, we stored a in a, and then incremented it. But it is like a = a++; // as a<b which shows undefined behaviour. a = (a++ < b++) ? a : b; here, a is being incremented at the time of comparison, so now a is 6, which is stored in a. A: Both cases involve undefined behaviour of some sort because you are incrementing a, returning a and assigning to a on the left side within 2 sequence points. 3 would be required for a clearly defined result. In this case : a = (a < b) ? a++ : b++; if a is smaller than b a is returned (value = 5) as the result of the ternary operator a is incremented (value = 6). the result of the ternary operator (5) is assigned to the left hand side variable a (over-writing 6) The order of steps 3 and 4 is not defined. It is equivalent to a = a++; In this case : a = (a++ < b++) ? a : b; If a is smaller that b a and b are incremented (regardless which is smaller) a is returned as the result of the ternary operator it is assigned to the left hand side variable a The order of steps 2 and 3 is not clearly defined. It's important to keep track of sequence points in such cases. Relevant rules : The 1st expression of ternary operator on the left of ? is sequenced before the 2nd or 3rd expressions. And either of them is sequenced before assignment. The comparison is sequenced before the ? In expressions like a++ the value is returned before incrementing Undefined behaviour: In expressions like a = a++; there is no sequence point between (post)incrementing a and assigning to a on the left side. Both happen after the original value of a is returned In expressions like a++ ? a : b there is no sequence point between (post)incrementing a and returning a from the ternary operator. Both happen after the ?
3.5625
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Black pepper is produced from the unripe berries of the pepper plant while they are still green. The berries are cooked briefly in hot water, both to clean them and to prepare them for drying. The heat ruptures cell walls in the fruit, speeding the work of browning enzymes during drying. The berries are dried in the sun or by machine for several days, during which the fruit around the seed shrinks and darkens into a thin, wrinkled black layer, the result of a fungal reaction. Once dried, the fruits are called black peppercorns. Black pepper has a fine pungent, fruity fragrance with warm woody notes. The taste is hot and clean with a strong aftertaste. White pepper consists of the seed only, with the fruit removed. This is usually accomplished by allowing fully ripe berries to soak in water for about a week, during which the flesh of the fruit softens and decomposes. Rubbing then removes what remains of the fruit, and the naked seed is dried. Alternative processes are used for removing the outer fruit from the seed, including removal of the outer layer from black pepper produced from unripe berries. White pepper can be slightly musty and is what is normally sold as finely ground pepper. Green pepper, like black, is made from the unripe berries. Dried green peppercorns are treated in a manner that retains the green colour, such as treatment with sulphur dioxide or freeze drying. Pickled peppercorns, also green, are unripe berries preserved in brine or vinegar. Fresh, unpreserved green pepper berries, largely unknown in the West, are used in some Asian cuisines, particularly Thai cuisine. Their flavour has been described as piquant and fresh, with a bright aroma. They decay quickly if not dried or preserved. Green peppers have a light aroma and a fresh taste. They go well with fish. Chef's tip This was drummed into me on my various Indian cookery classes, back in the day: If any recipe calls for black pepper and some form of frying / sautéing / cooking in oil or butter, whatever the recipe says, add your black pepper to the oil. It will flavour the oil, which then does a far better job of flavouring the food than adding it at the end.
3.140625
3
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Q: Find the Min Even Integer and Max Even Integer in an Array int i,max,min; int A[11]; min = A[1]; max = A[1]; for(i=1;i<=10;i++) { if(min > A[i] && A[i]%2 ==0 ) min = A[i]; if(max < A[i] && A[i]%2 ==0 ) max = A[i]; } printf("Minimum Even : %d\n",min); printf("Maximum Even : %d\n",max); getch(); } When I fill my array with 1, 2, 3, 4, 5, 6, 7, 8, 9, 10 Why is the minimum even number equal to 1? A: This test case exposes one of the dark sides of your code where you have initialized your min and max to A[1] regardless of whether A[1] is odd or even. Problem: There may be cases where the array does not contain any even number. In such cases, you may wish to print so instead of printing -1 or INT_MIN or INT_MAX. If you are new to INT_MIN and INT_MAX, this will serve as a starter before proceeding to the solution. Solution: This solution modifies your code in such a way that it handles all the cases given that you provide the inputs without any error. Have a flag to know whether you found your min and max: int foundAnswer = 0; Add the header file limits.h and initialize your min and max as follows: min = INT_MAX; max = INT_MIN; Modify your loop such that the flag serves a purpose: Note: Don't waste the zeroth index of your array without any reason. Modify your array declaration and input loop accordingly before changing this one. for (i = 0; i < ARRAY_SIZE; ++i) { if (A[i] % 2 == 0) { foundAnswer = 1; if (A[i] < min) min = A[i]; if (A[i] > max) max = A[i]; } } Modify your printing code slightly so that all the cases are covered. if (foundAnswer) { // Print min // Print max } else { // Print "min and max not found" } Bonus: You can learn from the following links in order to optimize your code: How do I check if an integer is even or odd using bitwise operators The algorithms discussed here will provide you with a better time complexity to achieve the same.
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The 6502 and the Propeller are connected via a few glue-logic chips. The Propeller has 32 digital I/O pins and they are all in use; many of them are used in more ways than one. The Propeller controls the 6502, and enables the SRAM memory chip. The Propeller generates the clock pulses for the 6502, at a maximum rate of 1MHz. During the first half of each clock pulse, the 6502 doesn't use the data bus, so the Propeller can use this time to enable two 74HC244 octal buffers to connect to the address bus. It can use the address to make decisions about what to do during the second half of the clock pulse, for example if the 6502 is in the process of writing a byte into the screen buffer, the Propeller can catch this write and put the byte in its own memory to show a character on the screen. Signals such as interrupts and Reset can be generated by the Propeller by using a 74HC574 octal D flipflop. During the first half of the clock pulse, the Propeller puts the signals on the pins that are connected to the '574 and clocks the flipflops so that the updated signals will be sent to the 6502 continuously even though the Propeller only updates them once per clock pulse. The RAM chips is connected to the data bus and address bus of the 6502 and its Chip Select line is permanently active; however the two pins that control whether the RAM reads or writes a byte from or to the data bus are under direct control of the Propeller. When the 6502 accesses a memory area that's mapped into the Propeller (such as a video buffer), the Propeller just needs to make sure that the RAM chip doesn't get activated at the same time. The 6502 has to boot from a memory area that's initialized with data before the 6502 starts. This can be done in two ways: The first way is to simply map the ROM area into the Propeller. The second way is for the Propeller to write the ROM image to the SRAM chip before starting the 6502. However, the Propeller doesn't have direct control over the address bus and the 6502 can't start until there's something in memory. This problem is solved by a clever algorithm that generates a Reset or NMI on the 6502. The 6502 retrieves a pointer to a location to start executing a Reset or NMI handler, and the Propeller intercepts the retrieval of that pointer to send the 6502 to a location where the code needs to be stored. During the first half of each clock pulse (when the 6502 isn't using the data bus but an address is already available), the Propeller puts the byte to store onto the data bus, and enables the Write line on the RAM chip to store the data. Then during the second half of the clock pulse, it disables the RAM chip and generates dummy instructions for the 6502. So the 6502 thinks that it's busy doing nothing to handle the Reset or NMI, but the Propeller is storing data into memory behind the back of the 6502. At the time of this writing, the download algorithm hasn't been totally debugged yet, but I've been successful in setting up an emulator for the Apple 1 and mapping Ken Wessen's Krusader ROM into 6502 memory which makes it possible to write programs in Assembly language or Basic. See http://youtu.be/8BCoQepmyYU for a demo. This is just the first emulator of an existing system. More emulators for other systems will follow, and of course it's possible to design a new system that's not based on any pre-existing hardware at all. Furthermore it's possible to use an expansion bus to connect hardware that might be too difficult to emulate with the Propeller.
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Digital video capabilities can be incorporated into a wide range of devices, including digital televisions, digital direct broadcast systems, wireless communication devices, personal digital assistants (PDAs), laptop computers, desktop computers, video game consoles, digital cameras, digital recording devices, cellular or satellite radio telephones, and the like. Digital video devices can provide significant improvements over conventional analog video systems in processing and transmitting video sequences. Different video encoding standards have been established for encoding digital video sequences. The Moving Picture Experts Group (MPEG), for example, has developed a number of standards including MPEG-1, MPEG-2 and MPEG-4. Other examples include the International Telecommunication Union (ITU)-T H.263 standard, and the ITU-T H.264 standard and its counterpart, ISO/IEC MPEG-4, Part 10, i.e., Advanced Video Coding (AVC). These video encoding standards support improved transmission efficiency of video sequences by encoding data in a compressed manner. Various video encoding standards support video encoding techniques that utilize similarities between successive video frames, referred to as temporal or Inter-frame correlation, to provide Inter-frame compression. The Inter-frame compression techniques exploit data redundancy across frames by converting pixel-based representations of video frames to motion representations. Frames encoded using Inter-frame techniques are referred to as P (“predictive”) frames or B (“bi-directional”) frames. Some frames, referred to as I (“intra”) frames, are encoded using spatial compression, which is non-predictive.
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Researchers at the Yale School of Public Health have discovered a mathematical relationship that sheds new light on the rate at which cancer cells mutate and why some survive and rapidly multiply, yet others do not. The discovery by members of the laboratory of Jeffrey Townsend, Ph.D., the Elihu Professor of Biostatistics and of Ecology and Evolutionary Biology, will allow essential calculations to be performed that determine the likely scope of cancerous cells as they develop. The finding has implications for decision-making for precision-medicine tumor boards, the selection and design of clinical trials, the development of pharmaceuticals and basic research prioritization. The study is published in the Journal of the National Cancer Institute. “For the past 10 years we’ve been able to calculate from tumor sequencing which mutated genes are winners and losers—which mutated genes help the cancer survive and reproduce, and which do nothing,” Townsend said. “But we haven’t been able to compute their cancer effect size—how important one mutation is compared to another. Now we can.” A major goal of cancer biology is to not just identify the important and unimportant genes to the development of cancer, but to determine the relative importance of each cellular mutation to the survival and spread of cancer cells and, ultimately, what it means for the patient, Townsend explained. In the study, the researchers estimated the effect sizes of all recurrent single nucleotide variants in 22 major types of cancer, and quantified the relative importance of each. Tumor sequencing studies have typically reported how frequent mutations are seen and a statistical measure (a P value) indicating whether the gene is overburdened with mutations beyond expectation, both important measures. However, neither measure is an effect size for cancer. Neither measure communicates how important the gene is to tumorigenesis and cancer disease. To quantify cancer effect size, Townsend and colleagues broke down the frequency that a mutation is observed in tumors into two contributing factors: the baseline mutation rate, and the degree of selection for the mutation in the cancer lineage. Both mutation and selection contribute to the frequency of variants among cells. Townsend and colleagues were able to use diverse genome-scale data to calculate the mutation rate. By essentially dividing out the contribution of mutation from the frequency that mutations were observed in tumors, they showed how to calculate the cancer effect size Townsend credits the breakthrough to insights that come from having a background in evolutionary biology. “Whereas in the cancer world the focus has always been on mutation rates, the focus in evolutionary biology has been on the process of natural selection on those mutations. The quantification of cancer effect sizes is a great example of how interdisciplinary research is not only helpful, but essential to scientific progress,” he said. Why is the cancer effect size important? Townsend uses an example of a tumor, from which a DNA sequence shows that two genes known to be related to cancer have mutated. There are two highly effective drugs targeting these exact mutations but no clinical trial has been conducted to compare them. “By looking at cancer through the lens of evolution we can harness the wealth of molecular data made available through tumor DNA sequencing to both better understand what is driving cancer and to also expand and refine evolutionary theory,” said Vincent Cannataro, Ph.D., a postdoctoral associate and the study’s first author. The study was co-authored by Stephen Gaffney, Ph.D., an associate research scientist at the Yale School of Public Health. The research was funded by a grant from Gilead Sciences, Inc. Publication: Vincent L Cannataro, et al., “Effect Sizes of Somatic Mutations in Cancer,” Journal of the National Cancer Institute, 2018; doi:10.1093/jnci/djy168
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Visualizing Decision Trees with Python (Scikit-learn, Graphviz, Matplotlib) Learn about how to visualize decision trees using matplotlib and Graphviz Image from my Understanding Decision Trees for Classification (Python) Tutorial. Decision trees are a popular supervised learning method for a variety of reasons. Benefits of decision trees include that they can be used for both regression and classification, they don’t require feature scaling, and they are relatively easy to interpret as you can visualize decision trees. This is not only a powerful way to understand your model, but also to communicate how your model works. Consequently, it would help to know how to make a visualization based on your model. This tutorial covers: How to Fit a Decision Tree Model using Scikit-Learn How to Visualize Decision Trees using Matplotlib How to Visualize Decision Trees using Graphviz (what is Graphviz, how to install it on Mac and Windows, and how to use it to visualize decision trees) How to Visualize Individual Decision Trees from Bagged Trees or Random Forests As always, the code used in this tutorial is available on my GitHub. With that, let’s get started! How to Fit a Decision Tree Model using Scikit-Learn In order to visualize decision trees, we need first need to fit a decision tree model using scikit-learn. If this section is not clear, I encourage you to read my Understanding Decision Trees for Classification (Python) tutorial as I go into a lot of detail on how decision trees work and how to use them. Import Libraries The following import statements are what we will use for this section of the tutorial. import matplotlib.pyplot as plt from sklearn.datasets import load_iris from sklearn.datasets import load_breast_cancer from sklearn.tree import DecisionTreeClassifier from sklearn.ensemble import RandomForestClassifier from sklearn.model_selection import train_test_split import pandas as pd import numpy as np from sklearn import tree Load the Dataset The Iris dataset is one of datasets scikit-learn comes with that do not require the downloading of any file from some external website. The code below loads the iris dataset. import pandas as pd from sklearn.datasets import load_irisdata = load_iris() df = pd.DataFrame(data.data, columns=data.feature_names) df['target'] = data.target Original Pandas df (features + target) Splitting Data into Training and Test Sets The code below puts 75% of the data into a training set and 25% of the data into a test set. X_train, X_test, Y_train, Y_test = train_test_split(df[data.feature_names], df['target'], random_state=0) The colors in the image indicate which variable (X_train, X_test, Y_train, Y_test) the data from the dataframe df went to for a particular train test split. Image by Michael Galarnyk. Scikit-learn 4-Step Modeling Pattern # Step 1: Import the model you want to use # This was already imported earlier in the notebook so commenting out #from sklearn.tree import DecisionTreeClassifier # Step 2: Make an instance of the Model clf = DecisionTreeClassifier(max_depth = 2, random_state = 0) # Step 3: Train the model on the data clf.fit(X_train, Y_train) # Step 4: Predict labels of unseen (test) data # Not doing this step in the tutorial # clf.predict(X_test) How to Visualize Decision Trees using Matplotlib As of scikit-learn version 21.0 (roughly May 2019), Decision Trees can now be plotted with matplotlib using scikit-learn’s tree.plot_tree without relying on the dot library which is a hard-to-install dependency which we will cover later on in the blog post. The code below plots a decision tree using scikit-learn. tree.plot_tree(clf); This is not the most interpretable tree yet. In addition to adding the code to allow you to save your image, the code below tries to make the decision tree more interpretable by adding in feature and class names (as well as setting filled = True ). fn=['sepal length (cm)','sepal width (cm)','petal length (cm)','petal width (cm)'] cn=['setosa', 'versicolor', 'virginica'] fig, axes = plt.subplots(nrows = 1,ncols = 1,figsize = (4,4), dpi=300) tree.plot_tree(clf, feature_names = fn, class_names=cn, filled = True); fig.savefig('imagename.png') How to Visualize Decision Trees using Graphviz Decision Tree produced through Graphviz. Note that I edited the file to have text colors correspond to whether they are leaf/terminal nodes or decision nodes using a text editor. Graphviz is open source graph visualization software. Graph visualization is a way of representing structural information as diagrams of abstract graphs and networks. In data science, one use of Graphviz is to visualize decision trees. I should note that the reason why I am going over Graphviz after covering Matplotlib is that getting this to work can be difficult. The first part of this process involves creating a dot file. A dot file is a Graphviz representation of a decision tree. The problem is that using Graphviz to convert the dot file into an image file (png, jpg, etc) can be difficult. There are a couple ways to do this including: installing python-graphviz though Anaconda, installing Graphviz through Homebrew (Mac), installing Graphviz executables from the official site (Windows), and using an online converter on the contents of your dot file to convert it into an image. Creating the dot file is usually not a problem. Converting the dot file to a png file can be difficult. Export your model to a dot file The code below code will work on any operating system as python generates the dot file and exports it as a file named tree.dot . tree.export_graphviz(clf, out_file="tree.dot", feature_names = fn, class_names=cn, filled = True) Installing and Using Graphviz Converting the dot file into an image file (png, jpg, etc) typically requires the installation of Graphviz which depends on your operating system and a host of other things. The goal of this section is to help people try and solve the common issue of getting the following error. dot: command not found . dot: command not found How to Install and Use on Mac through Anaconda To be able to install Graphviz on your Mac through this method, you first need to have Anaconda installed (If you don’t have Anaconda installed, you can learn how to install it here). Open a terminal. You can do this by clicking on the Spotlight magnifying glass at the top right of the screen, type terminal and then click on the Terminal icon. Type the command below to install Graphviz. conda install python-graphviz After that, you should be able to use the dot command below to convert the dot file into a png file. dot -Tpng tree.dot -o tree.png How to Install and Use on Mac through Homebrew If you don’t have Anaconda or just want another way of installing Graphviz on your Mac, you can use Homebrew. I previously wrote an article on how to install Homebrew and use it to convert a dot file into an image file here (see the Homebrew to Help Visualize Decision Trees section of the tutorial). How to Install and Use on Windows through Anaconda This is the method I prefer on Windows. To be able to install Graphviz on your Windows through this method, you first need to have Anaconda installed (If you don’t have Anaconda installed, you can learn how to install it here). Open a terminal/command prompt and enter the command below to install Graphviz. conda install python-graphviz After that, you should be able to use the dot command below to convert the dot file into a png file. dot -Tpng tree.dot -o tree.png Windows installing of Graphviz through conda. This should fix the ‘dot’ is not recognized as an internal or external command, operable program or batch file issue. How to Install and Use on Windows through Graphviz Executable If you don’t have Anaconda or just want another way of installing Graphviz on your Windows, you can use the following link to download and install it. If you aren’t familiar with altering the PATH variable and want to use dot on the command line, I encourage other approaches. There are many Stackoverflow questions based on this particular issue. How to Use an Online Converter to Visualize your Decision Trees If all else fails or you simply don’t want to install anything, you can use an online converter. In the image below, I opened the file with Sublime Text (though there are many different programs that can open/read a dot file) and copied the content of the file. Copying the contents of a dot file In the image below, I pasted the content from the dot file onto the left side of the online converter. You can then choose what format you want and then save the image on the right side of the screen. Save visualization to computer Keep in mind that there are other online converters that can help accomplish the same task. How to Visualize Individual Decision Trees from Bagged Trees or Random Forests A weakness of decision trees is that they don’t tend to have the best predictive accuracy. This is partially because of high variance, meaning that different splits in the training data can lead to very different trees. The image above could be a diagram for Bagged Trees or Random Forests models which are ensemble methods. This means using multiple learning algorithms to obtain a better predictive performance than could be obtained from any of the constituent learning algorithms alone. In this case, many trees protect each other from their individual errors. How exactly Bagged Trees and Random Forests models work is a subject for another blog, but what is important to note is that for each both models we grow N trees where N is the number of decision trees a user specifies. Consequently after you fit a model, it would be nice to look at the individual decision trees that make up your model. Fit a Random Forest Model using Scikit-Learn In order to visualize individual decision trees, we need first need to fit a Bagged Trees or Random Forest model using scikit-learn (the code below fits a Random Forest model). # Load the Breast Cancer (Diagnostic) Dataset data = load_breast_cancer() df = pd.DataFrame(data.data, columns=data.feature_names) df['target'] = data.target # Arrange Data into Features Matrix and Target Vector X = df.loc[:, df.columns != 'target'] y = df.loc[:, 'target'].values # Split the data into training and testing sets X_train, X_test, Y_train, Y_test = train_test_split(X, y, random_state=0) # Random Forests in `scikit-learn` (with N = 100) rf = RandomForestClassifier(n_estimators=100, random_state=0) rf.fit(X_train, Y_train) Visualizing your Estimators You can now view all the individual trees from the fitted model. In this section, I will visualize all the decision trees using matplotlib. rf.estimators_ In this example, notice how we have 100 estimators. You can now visualize individual trees. The code below visualizes the first decision tree. fn=data.feature_names cn=data.target_names fig, axes = plt.subplots(nrows = 1,ncols = 1,figsize = (4,4), dpi=800) tree.plot_tree(rf.estimators_[0], feature_names = fn, class_names=cn, filled = True); fig.savefig('rf_individualtree.png') Note that individual trees in Random Forest and Bagged trees are grow deep You can try to use matplotlib subplots to visualize as many of the trees as you like. The code below visualizes the first 5 decision trees. I personally don’t prefer this method as it is even harder to read. # This may not the best way to view each estimator as it is small fn=data.feature_names cn=data.target_names fig, axes = plt.subplots(nrows = 1,ncols = 5,figsize = (10,2), dpi=3000) for index in range(0, 5): tree.plot_tree(rf.estimators_[index], feature_names = fn, class_names=cn, filled = True, ax = axes[index]); axes[index].set_title('Estimator: ' + str(index), fontsize = 11) fig.savefig('rf_5trees.png') Create Images for each of the Decision Trees (estimators) Keep in mind that if for some reason you want images for all your estimators (decision trees), you can do so using the code on my GitHub. If you just want to see each of the 100 estimators for the Random Forest model fit in this tutorial without running the code, you can look at the video below. Concluding Remarks This tutorial covered how to visualize decision trees using Graphviz and Matplotlib. Note that the way to visualize decision trees using Matplotlib is a newer method so it might change or be improved upon in the future. Graphviz is currently more flexible as you can always modify your dot files to make them more visually appealing like I did using the dot language or even just alter the orientation of your decision tree. One thing we didn’t cover was how to use dtreeviz which is another library that can visualize decision trees. There is an excellent post on it here. Image from produced by dtreeviz library. If you have any questions or thoughts on the tutorial, feel free to reach out in the comments below or through Twitter. If you want to learn more about how to utilize Pandas, Matplotlib, or Seaborn libraries, please consider taking my Python for Data Visualization LinkedIn Learning course.
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Q: に vs で again: 前に vs 後で Following the current trend of pitting the particles に and で against each other, here is another question that does the same but from another type of usage and perspective. When we want to say "do X before Y", we use "Y 前に X": 食べる前に「いただきます」と言う。 On the other hand, when we want to say "do X after Y", we use "Y 後で X": 食べた後で「ごちそうさまでした」と言う。 What is the simplest explanation to explain the differences between 前 and 後 that make 前 goes with に while 後 goes with で in the two situations above? A: で derives from に+て, and て roughly corresponds to the present/past participles (-ing, -en) in Western languages. Kuno (1973) notices that て implies temporal order. So when you have 走ってころんだ '(By) running, I fell', running has to precede falling; it cannot be the other way around. This much is the general consensus. Notice that the usage of で in the question involves temporal notions rather than locations. Now, I found an interesting explanation here: Q14 that connects the facts mentioned above. According to this, when you have an expression A [temporal noun] で B, the て that is included in で obeys the temporal restriction mentioned above; that is, what is expressed by A [temporal noun] has to precede B. Going in the other temporal order is not allowed. Therefore, expressions like 食べた後で「いただきます」と言う。 [Temporal order: 食べた => 言う] are grammatical but × 食べる前で「いただきます」と言う。 [Temporal order: 食べる <= 言う] × 食べるよりも先で「いただきます」と言う。 [Temporal order: 食べる <= 言う] are not. に can be used by all the examples above: 食べた後に「いただきます」と言う。 食べる前に「いただきます」と言う。 食べるよりも先に「いただきます」と言う。 If there is preference of 食べた後で「いただきます」と言う over 食べた後に「いただきます」と言う, then some kind of slight difference in meaning like what phirru mentions in the comment may be playing a role here. A: In 後でする the focus is that you will do whatever you were doing, just later; whereas in 後にする the focus is that you will postpone whatever you are supposed to do until later. Treating で as the "instrumental" particle, this way, "後でする" would mean "to do (whatever), by using the time after now" And "後にする" would mean "to do (whatever), at a point of time after now" So "前に" would be "at a time before now", and "前で" would be impossible since you cannot use a time before now. Alternatively, treating で as the verb-conjunctive form of the copula だ, ”後でする” would mean "It is afterwards, and do it" This also shows the impossibility of 前で which would translate strangely into "It is now before and..." which is temporally impossible for the past to exist in the present. A: If you want a very simple answer, then you can look at the meaning of ni and de, again: ni means things are separate and interacting. de means that things are contiguous and acting in a similar manner (i.e., to the same ends). I think I answered a question you asked about them earlier to tell you that に and で could be compared to an English analogue of 'each other' and 'themselves'. Anyway... 後で is used because after the past happens, it is included as a part of a continuing timeline 'themselves'. 前に is used because the prior event interacts with the future event through time or the doer or whatever 'each other'. So, 'ホニャホニャの後でいく' = 'With/'contingent on' whatever's happening, I will do it.' 'ホニャホニャ前にいく' means, 'Whatever happened, and my going before that is related somehow'. And to reiterate one more time: '後で' means: 'the future comes only with complete a specific past' and '前に' means: 'the future seems to interacts with a past'.
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Q: Assign domain to IP address How do i go about making my Java app run an HTTP server on some socket (e.g 172.16.1.10:8080) and make it so that when another computer on the network connects to a domain (e.g http://myjavadomain.com) it gets redirected to the socket? A: If you want to run a fully fledged HTTP server then you will probably want to use some external library. For instance, Tomcat is written in Java, but there is also SUN's httpserver package. If it's just a simple socket server you're after, you can use the built-in classes from the java.net package: ServerSocket server = new ServerSocket(8080); while (running) { Socket socket = server.accept(); handleConnection(socket); } This will listen for incoming socket connections on port 8080 and create a new Socket whenever a client connects. You can then communicate with the client through the Socket's InputStream and OuputStream, which you would probably do in a separate Thread, so that your ServerSocket can continue listening for incoming connections from other clients. As for the second part of your question: by default, a web browser will connect to port 80, and there are several ways you could do port forwarding. One possible solution using iptables is given on this website: iptables -t nat -I PREROUTING --src 0/0 --dst 172.16.1.10 -p tcp --dport 80 -j REDIRECT --to-ports 8080 But the easiest solution would be to just specify the port number directly when connecting to your machine, e.g. http://myjavadomain.com:8080 This is assuming that your DNS is configured so that it resolves myjavadomain.com to 172.16.1.10 already.
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Introduction ============ Microalgae are promising source of biomass due to their advantageous features such as their phototropic nature, high growth rate, lack of competition with food crops for arable land, and abundant nutritious components, such as protein, pigments, and trace elements ([@ref-14]; [@ref-37]). Therefore, it has been used as feedstock, such as in food, feed, functional foods, biofuels, or chemicals integrated in novel biorefinery concepts ([@ref-43]; [@ref-36]). Unlike terrestrial plants, the biologically active compounds extracted from microalgae have shown unique properties, such as antibacterial, antiviral, antifungal, antioxidative, anti-inflammatory, and anti-tumor properties ([@ref-7]; [@ref-13]; [@ref-15]; [@ref-16]; [@ref-6]; [@ref-8]). From economical point of view, polysaccharides from algae are promising products due to their abundance in algae ([@ref-22]). Polysaccharides can be extracted from algae by several "green" extraction techniques, such as microwave-assisted extraction ([@ref-30]) and enzyme-assisted extraction methods ([@ref-21]). The characteristics of different polysaccharides from microalgae, including their composition and structure, were discussed ([@ref-7]). It was reported that *G. impudicum* and *C. vulgaris* contained homo galactose ([@ref-40]) and glucose ([@ref-27]), respectively. However, the other polysaccharides from microalgae are heteropolymers of galactose, xylose, glucose, rhamnose, fucose, and fructose ([@ref-24]; [@ref-34]; [@ref-28]). [@ref-11] found that the structure of the polysaccharides from *Phaeodactylum tricornutum* was a ramified sulfated flucoronomannan, with a backbone composed of β-(1,3)-linked mannose. Many studies have shown that the polysaccharides from microalgae are characterized by antibacterial, antitumor, and antiviral properties ([@ref-26]). As a kind of diatom, PTP has been found in great abundance in coastal and oceanic waters ([@ref-4]). It contains approximately 36.4% crude protein, 26.1% carbohydrate, 18.0% lipid, 15.9% ash, and 0.25% neutral detergent fiber on a dry weight (dw) basis ([@ref-29]). In addition, it can accumulate valuable pigments such as fucoxanthin, triacylglycerols, and omega-3 long-chain polyunsaturated fatty acids, such as eicosapentaenoic acid (EPA; C20:5) ([@ref-18]; [@ref-31]; [@ref-41]; [@ref-25]). Currently, it is commercialized for its lipids, especially EPA, and several studies have sought to increase the production yield of EPA and biomass ([@ref-12]; [@ref-2]; [@ref-25]). In recent years, due to its many therapeutic activities, fucoxanthin has been commercialized from PTP. However, there is little research about the polysaccharides extracted from PTP. Therefore, to make full use of the alga, in this paper, we extracted polysaccharides from PTP, characterized its chemical structure, and studied the anticancer activity of the polysaccharides. Materials and methods ===================== *Phaeodactylum tricornutum* samples and reagents ------------------------------------------------ Dried PTP powder was supplied by the Institute of Oceanology, Chinese Academy of Sciences. All the reagents used were of analytical grade and commercially available unless otherwise stated. Extraction of polysaccharides from *Phaeodactylum tricornutum* (PTP) -------------------------------------------------------------------- The extraction diagram was as [Fig. 1](#fig-1){ref-type="fig"}. ![Extraction process.\ The extraction diagram of PTP.](peerj-07-6409-g001){#fig-1} The dried PTP powder was extracted by the Soxhlet method with ethanol to remove pigments and lipids. The residue was then dried in an oven at 50 °C, and polysaccharides were extracted by hot distilled water with the assistance of ultrasonic methods. The optimal temperature, times of ultrasonic treatment, and extraction time were determined (shown in [Supplemental Information](#supplemental-information){ref-type="supplementary-material"}). According to the optimal conditions, the residue algal powder was treated by the ultrasonic method for 20 times, 10 s working, 10 s rest, and 380 W power. Then, it was extracted at 80 °C for 2 h with stirring. The solution produced by filtration was condensed by rotary evaporator and dialyzed for salt removal. The obtained solution was condensed again, and the final solution was freeze-dried to get the purified sulfated polysaccharides, called PTP. Chemical characterization ------------------------- The Mw of PTP was measured by HPLC with a TSK gel G4000PWxl column using 0.05 mol/L Na~2~SO~4~ as the mobile phase on an Agilent 1260 HPLC system equipped with a refractive index detector. The column temperature was 35 °C, and the flow rate of the mobile phase was 0.5 mL/min. Dextran standards with a Mw of 1, 5, 12, 50, 80, 270, and 670 KDa (Sigma, Mendota Heights, MN, USA) were used to calibrate the column. Total sugars were analyzed by the phenol-sulfuric acid method ([@ref-10]) using galactose as the standard. sulfated content was determined by the barium chloride gelatin method ([@ref-17]). The molar ratios of the monosaccharide composition were determined according to [@ref-33]. 1-phenyl-3-methyl-5-pyrazolone pre-column derivation HPLC was used to determine the molar ratio of the monosaccharide composition. Briefly, 10 mg polysaccharide sample was dissolved into one mL distilled water. The mixture was hydrolyzed in 4 mol/L trifluoroacetic acid, followed by neutralization with sodium hydroxide. Then, HPLC was used to determine every monosaccharide composition on a YMC Pack ODS AQ column (4.6 mm × 250 mm). Mannose, rhamnose, fucose, galactose, xylose, glucose, and glucuronic acid from Sigma-Aldrich were used as standards. FT-IR spectra of PTP were determined on a Nicolet-360 FT-IR spectrometer between 400 and 4,000 cm^−1^. Evaluation of inhibiting HepG2 growth activity in vitro ------------------------------------------------------- ### Cell culture HepG2 cells purchased from Kunming Cell Bank, Chinese Academy of Sciences, were cultured in DMEM supplemented with 10% fetal bovine serum solution, 100 U/mL penicillin and 100 mg/mL streptomycin at 37 °C in a humidified atmosphere containing 5% CO~2~. ### Evaluation of inhibiting HepG2 growth activity in vitro The cell growth inhibitory activity of PTP with different concentrations (50, 100, 150, 200, and 250 ug/mL) was assessed by MTT assay. The cells were seeded in a 96-well plate at a concentration of 1 × 10^4^ cells/mL and incubated with various concentrations PTP for 48 h. Then, 200 ul 0.5 mg/mL MTT solution was added to each well. After 4 h incubation, the plates were centrifuged for 10 min at 8,000 rpm. MTT solution was removed. And 200 uL DMSO was added into each well. The absorbance at 570 nm was determined. ### Apoptosis assessment The apoptosis states of HepG2 cells were determined by an Annexin V-FITC/PI apoptosis kit. Cells were collected and washed with ice-cold PBS twice. Then, the cells were resuspended and diluted to 1 × 10^6^ cell/mL with binding buffer. The suspended cells were dyed by 10 μL of Annexin V-FITC for 30 min at room temperature and then stained with five μL of propidium iodide (PI) for 5 min. After incubation, the apoptosis of cells was determined by flow cytometry with Guava® easyCyte 6-2L (Millipore, Billerica, MA, USA). ### Analysis of the cell cycle A cell cycle analysis kit (Beyotime, Haimen, Jiangsu, China) was used to analyze the cell cycle according to the manufacturer\'s instructions. Briefly, cells were plated in DMEM with different concentrations of sample for 24 h. Then, both the suspension and the adherent cells were collected and placed into the flow cytometry tube and centrifuged at 1,500 rpm for 5 min to obtain cell pellets. After that, the cell pellets were washed with precooling PBS and fixed in ice-cold 70% ethanol overnight at 4 °C. Fixed cells were rewashed with PBS and incubated with PI staining solution (0.5 mL of staining buffer, 25 μL of PI staining solution, and 10 μL of RNAase A) for 30 min at 37 °C in the dark. Cell cycle analysis was carried out with Guava® easyCyte 6-2L (Millipore, Billerica, MA, USA) using 10,000 counts per sample. The percentage of cells distributed in the different phases of G0/G1, S, and G2/M were recorded and analyzed. Statistical analysis -------------------- All data are shown as means ± SD (standard deviation) of three independent experiments to ensure the reproducibility of the results. Statistical analysis was performed using SPSS. The difference among groups was analyzed by one-way ANOVA. Results ======= Chemical characterization ------------------------- *Phaeodactylum tricornutum* was extracted and purified from , with a yield of 1.5%(% dw). It was further characterized regarding Mw, total sugars, sulfate content, and monosaccharide composition ([Table 1](#table-1){ref-type="table"}). 10.7717/peerj.6409/table-1 ###### Chemical composition. ![](peerj-07-6409-g006) Sample Total sugar/% Sulfate/% Mw/kDa Monosaccharides composition (Molar ratio) -------- --------------- ----------- -------- ------------------------------------------- ------ ------ ------ ------ ------ ------ PTP 29.94 20.36 4810 0.00 0.25 0.68 0.53 0.56 1.00 0.75 **Notes:** Chemical composition of PTP (%w/w dry weight). Man, mannose; Rha, rhamnose; Glc A, glucuronic acid; Gal, galactose; Glc, glucose; Xyl, xylose; Fuc, fucose. According to [Table 1](#table-1){ref-type="table"}, the total sugar and sulfate contents were 29.94% and 20.36%, respectively, which indicated that PTP was a type of sulfated polysaccharide. The Mw of PTP was higher (4,810 kDa). The results of the monosaccharide composition showed that the most common monosaccharide of PTP was xylose, followed by fucose, glucose, and galactose, with a small amount of rhamnose. The glucuronic acid content of PTP (0.68) was higher. These results indicated that PTP was a hybrid and acidic polysaccharide. To further characterize the chemical structure of PTP, the corresponding FT-IR spectrum was examined ([Fig. 2](#fig-2){ref-type="fig"}). The O--H stretching vibration appeared at 3,272 cm^−1^, and the C--H stretching vibration appeared at 2,926 cm^−1^. The adsorption at 1,632 and 1,408 cm^−1^ represented the asymmetric and symmetric stretching vibration of C=O, respectively. The adsorption at 1,226 and 1,038 cm^−1^ corresponded to the S=O stretching vibration and C--O--H deformation vibration, respectively. These results further indicated that PTP was an acidic and sulfated polysaccharide, which chelated with other positive ions. ![FTIR.\ FT-IR spectra of PTP.](peerj-07-6409-g002){#fig-2} Evaluation of inhibiting HepG2 growth activity in vitro ------------------------------------------------------- [Figure 3](#fig-3){ref-type="fig"} shows the inhibitory effect of different concentrations of PTP on HepG2 tumor cells. The results indicated that PTP had an antiproliferative effect on HepG2 cells in a dose-dependent manner. With concentration increasing, PTP had higher inhibitory activity, and the inhibition rate was up to 60.37% when the concentration was 250 ug/mL. However, the manner of PTP inhibiting HepG2 growth was not clear. To analyze the main cause, we determined the cell apoptosis and cell cycle by flow cytometry. ![Inhibition rate of HepG2 by MTT assay.\ The effect of different concentration PTP on the inhibition rate of HepG2 by MTT assay for 48h.](peerj-07-6409-g003){#fig-3} Induction of apoptosis according to cell cycle analysis ------------------------------------------------------- [Figure 4](#fig-4){ref-type="fig"} shows the results of flow cytometry, when the HepG2 cells were treated with different concentrations of PTP. From the results, we deduced the apoptosis rate under different concentrations of PTP (shown in [Fig. 4](#fig-4){ref-type="fig"}). From [Fig. 4](#fig-4){ref-type="fig"}, when HepG2 cells were treated with PTP, the apoptosis rate increased in a dose-dependent manner, although it decreased slightly under 200 ug/mL PTP. When the concentration of PTP was 250 ug/mL, 30% apoptosis of cells was induced. Double negative PI-Annexin V cells accounted for about 63%. The above results were consistent with those of the MTT assay. They indicated that PTP could significantly induce cell apoptosis. Then, we determined the HepG2 cell cycle rate under three different concentrations (50, 150, and 250 ug/mL) of PTP, as shown in [Fig. 5](#fig-5){ref-type="fig"}. From [Fig. 5](#fig-5){ref-type="fig"}, the treatment of different concentrations of PTP did not influence the HepG2 cell cycle rate, which might indicate that PTP's anticancer effect occurred mainly through induction of apoptosis without affecting the mitosis of HepG2 cells. ![Cell apoptosis rate.\ The cell apoptosis rate under different concentration of PTP.](peerj-07-6409-g004){#fig-4} ![Cell cycle.\ The cell cycle rate under different concentration of PTP.](peerj-07-6409-g005){#fig-5} Discussion ========== Cancer is the leading threat to the world population, and it is the first-leading cause of death worldwide. The current cancer treatments often cause side effects ([@ref-32]; [@ref-5]). Recently, due to their favorable properties, polysaccharides from microalgae have been given increased attention. Polysaccharides from *Spirulina platensis* have been shown to have antitumor functions on human HT-29 cells ([@ref-38]), MB-231 cells ([@ref-39]), HeLa cells ([@ref-42]) and HepG2 cells ([@ref-9]). Polysaccharides from *Platymonas subcondigoramis* inhibited melanoma ([@ref-23]). [@ref-35] showed that polysaccharides from the dinoflagellate *Gymnodinium* sp. exhibited significant cytotoxicity against a variety of cancer cells, which meant that the polysaccharides might be a potential anticancer chemotherapeutic agent. For PTP, some references reported antioxidant ([@ref-1]), anti-obesity ([@ref-19]), anti-inflammatory, and immunomodulatory activities ([@ref-20]; [@ref-13]). A novel fatty alcohol ester isolated from PTP showed apoptotic anticancer activity ([@ref-32]). Few studies have addressed polysaccharides isolated from PTP. [@ref-1] extracted endo-exopolysaccharide and determined its antioxidant activity on DPPH. The composition of the polysaccharides included xylose, glucose, and galactose. Similarly, the monosaccharide composition of PTP mainly included xylose, fucose, glucose and galactose. Fucose was not reported by [@ref-1], which may be due to the different origins of the algae. In this paper, we determined not only the monosaccharide composition but also the total sugar, sulfate contents and Mw (29.94%, 20.36%, and 4,810 kDa, respectively) and found that PTP is a complicated sulfated polysaccharide. A type of lipopolysaccharide extracted from Phaeodactylum tricornutum exhibited anti-inflammatory activity by blocking the activation of nuclear factor-κB and phosphorylation of p38 mitogen-activated protein kinases, extracellular signal-regulated kinases 1 and 2 and c-Jun N-terminal kinase ([@ref-20]). However, there was no related information about the lipopolysaccharide. To our knowledge, no anticancer activity has been reported for PTP. In this paper, we determined the anticancer activity of PTP on HepG2 cells. Significant anticancer activity (up to 60.37% under 250 ug/mL) by MTT assays, which was much better than for polysaccharides isolated from *Spirulina platensis* ([@ref-38], [@ref-39]). In addition, several studies reported that polysaccharides isolated from *Spirulina platensis* exhibited anticancer activity by blocking G0/G1 phase of cancer cells, which induced the mitosis of cancer cells and led to apoptosis of the cells ([@ref-38], [@ref-39]; [@ref-42]; [@ref-9]). However, in this paper, although the apoptosis rate of HepG2 cells increased, cell cycle analysis indicated that PTP's anticancer effect occurred mainly through induction of apoptosis without affecting the cell cycle and mitosis of HepG2 cells. This result might differ according to the chemical components and structure. It needs further investigation. In addition, some references reported that microalgae polysaccharides have the capacity to modulate the immune system so that they display anticancer activity in vivo ([@ref-3]). For this study, only in vitro cell experiments were carried out, and it is necessary to explore the anticancer activity in vivo. Further research will address this issue. Conclusion ========== In this paper, a sulfated polysaccharide (PTP) was extracted from PTP with a high Mw (4,810 kDa). The monosaccharide composition of PTP was mainly xylose, fucose, glucose, and galactose. MTT assays showed that PTP has significant anticancer activity (up to 60.37% under 250 ug/mL). Furthermore, the anticancer effect occurred mainly through induction of apoptosis without affecting the cell cycle and mitosis of HepG2 cells. Thus, PTP may be a potential drug for anticancer treatment. Supplemental Information ======================== 10.7717/peerj.6409/supp-1 ###### Anticancer activity of PTP. ###### Click here for additional data file. 10.7717/peerj.6409/supp-2 ###### Apoptosis and cycle analysis of PTP. ###### Click here for additional data file. 10.7717/peerj.6409/supp-3 ###### Extraction. Selecting the optimal extraction conditions ###### Click here for additional data file. Additional Information and Declarations ======================================= The authors declare that they have no competing interests. [Shengfeng Yang](#author-1){ref-type="contrib"} conceived and designed the experiments, performed the experiments, prepared figures and/or tables, authored or reviewed drafts of the paper, approved the final draft. [Haitao Wan](#author-2){ref-type="contrib"} performed the experiments. [Rui Wang](#author-3){ref-type="contrib"} analyzed the data. [Daijun Hao](#author-4){ref-type="contrib"} analyzed the data, contributed reagents/materials/analysis tools. The following information was supplied regarding data availability: The raw measurements are available in the [Supplementary Files](#supplemental-information){ref-type="supplementary-material"}.
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Introduction ============ Having excellent knowledge of the referent values of red blood cells (RBCs) variables with children and adolescents is profoundly important for proper interpretation of the results of complete blood count. Reference values for RBCs variables are lower with children in comparison with the adults ([@B1]). Several studies which investigated hematologic parameters have been done in different populations, racial, ethnic and gender subgroups, even in different seasons ([@B2]--[@B5]). In most of these studies, age, ethnic and sex differences were significant and therefore it was stressed the need for establishing normal reference values for different populations. RBC variables are fairly stable through adult life, but significant differences exist in the pediatric population. The newborn infant, older child, and adult show profound differences ([@B6]). Because hemoglobin level and red cell indices vary with age, it is crucial to take as reference standards that change in each period of life, from fetal life to adolescence. Adult value will be reached gradually during the second part of childhood, around 15 yr of age ([@B7]). To ensure that interpretation of hematology results in children are appropriate, the laboratory has to have established age-specific reference ranges ([@B8]). The sex differences in hemoglobin level in adults are well documented, and the underlying mechanisms are probably a direct effect of sex hormones, both estrogen and androgens on erythropoiesis ([@B9]). "In pre-pubertal humans no major differences can be found between the sexes in red blood cell count or hemoglobin and serum ferritin concentrations" ([@B10]). "The difference in hematological variables between sexes emerges after onset of menstruations and persistent until 10 yr after the menopause" ([@B9], [@B10]). Menstruation and nutritional intake are principal reasons for lower values of hemoglobin and iron of women regarding men ([@B11]). The total amount of hemoglobin increases more in boys than in the girls in the period of puberty ([@B12]). Among children 6--14 yr old the values increased from about 12 to about 14 gr per 100 ml of blood. In girls between 14 and 20 yr of age, the hemoglobin values decreased slightly, reaching 13gr/100ml. In boys of corresponding ages, there was an increase to about 15gr/100ml. In both sexes, these values were attained at about 20 yr of age and remained characteristic of the third decade of life ([@B13]). A few comparative studies have been conducted on children in pre-adolescent and adolescent years and the lack of studies and information on hematological parameters for this population is obvious. Assessment of RBC variables in young population and determination of normal values is necessary for identification of anemia. The aim of this paper was to determine the values of RBC variables with young population from both sexes, within age span 8 to 18 years. Possible differences in the group(s) have to be determined regarding the age difference and between the groups regarding the sex. Methods ======= Subjects -------- Study participants consisted of 300 healthy young individuals (age span 8 to 18 yr) which participated continuously in different kinds of sports activities and were involved in regular medical pre-participation check-ups in 2016. A group with male subjects was composed of 240 participants and female group was composed of 80 participants. Both groups were divided into subgroups regarding the two-year interval: under 10 (U10); under 12 (U12); under 14 (U14); under 16 (U16); under 18 (U18). Blood collection ---------------- The hematological testing was part of complete medical checkup for sports pre-participation screening, during morning hours (from 8:00 to 12:00 am) in a controlled laboratory with constant temperature (between 20 °C and 24 °C) and humidity. To determine the blood count blood samples were collected from capillary vessel using sterile plastic containers with anticoagulant (EDTA K3) incorporated in its walls. An experienced evaluator was in charge of the collection procedures. Analysis was determined by automated hematology analyzer ABX Micros 60-OT (ABX hematology, Montpelier, France). The technical error intra rater measurement showed values lower than 1%. Reagents, calibrators, and controls were obtained from the instrument manufacturer. Analysis of samples was performed immediately after blood drawing. The testing was conducted at The Institute of Physiology, Medical Faculty Skopje, Republic of Macedonia. Definitions of analyzed hematological parameters ([@B14], [@B15]) ----------------------------------------------------------------- The erythrocyte or red blood counts also referred to as "RBCs", involve counting the number of RBCs per unit volume of whole blood. Male 4.7 -- 6.1 × 10^6^ cells/mm^3^; female 4.2--5.4 × 10^6^ cells/mm^3^. Hematocrit (Hct) is the percentage of blood that is represented by the red blood cells. Normal ranges for hematocrit are strongly dependent on the age, and well described from newborns to adult age. Optimal values for adult males are between 42% and 54% and for female 38% to 46%.Hemoglobin level (Hb) is expressed as the amount of hemoglobin in grams per deciliter of whole blood. Adult males should have between 14 to 18 g/dl, adult woman 12 to 16 g/dl.Mean corpuscular volume (MCV) is the mean volume of all the red blood cells in the sample or the average size of the red blood cell. It can be calculated by dividing the hematocrit (volume of all RBC) by RBC number. The value is expressed in volume units, femtolitres (fL=10^−15^ L). The normal range is 80-94fL.Mean corpuscular hemoglobin (MCH) represents the mean mass of hemoglobin in the one red blood cell and is expressed in the mass unit, picograms (pg= 10^−12^ gr). It is calculated by dividing the total mass of hemoglobin by the number of red blood cells. The normal range is 27--31 pg.Mean corpuscular hemoglobin concentration (MCHC) is the mean concentration of hemoglobin in the red cell or average concentration of hemoglobin in one liter of red blood cells. It is calculated by dividing the hemoglobin by the hematocrit. MCHC fulfill the meaning of MCH considering the size of the cell. The normal range is 31.5--35 g/dl.RDW or red cell distribution width is parameter that measures variation in red blood size or red blood cell volume. The reference ranges for RDW for adult is 11.6%--14.6%. Ethics ------ Institutional ethical approval was received from the Ethics Committee of the Medical Faculty, Ss Cyril and Methodius University, Skopje, Republic Macedonia (No=03-1197/5). Informed consents were obtained from the parents. Statistical Analysis -------------------- Statistical analysis as performed using the computer software SPSS for Windows version 14.0 (SPSS Inc., Chicago, USA). Analysis of variance factorial analysis and post hoc multiple comparisons were used to evaluate the significance of the differences. Differences in proportions were analyzed using the Chi-square test or Fisher's exact test when appropriate. All data were presented as mean (±SD). Results were considered to be statistically significant when *P*-value was less than 0.05 (*P*\<0.05). Results ======= Hematologic parameters in males ------------------------------- The mean value and standard deviations for general features (age, height and weight) and hematologic parameters (RBCs-red blood cells; Hb-hemoglobin, Hct -- hematocrit; and hematological indices: MCV, MCH, MCHC and RDW) for group of male participants (N=240) are presented in [Table 1](#T1){ref-type="table"}. All parameters are shown for five age different subgroups. High statistically significant difference is found for all general features of participants: age, height, and weight. ###### General characteristics and hematologic parameters of the male participants (8--18 yr, N=240) for age different subgroups ***MALE*** ***U10*** ***U12*** ***U14*** ***U16*** ***U18*** ***P-value*** ----------------- --------------- --------------- -------------- --------------- --------------- --------------- Age(yr) 9.24 (0.32) 11.08 (0.58) 13.28 (0.28) 14.93 (0.54) 16.78 (0.35) 0.001 Height (cm) 131,78 (22.9) 148,69 (22.9) 168,08 (8.6) 177,06 (6.87) 182,29 (6.88) 0.001 Weight (kg) 33,00 (6.9) 41,93 (6.99) 58,65 (12.3) 65,68 (17.02) 76,13 (9.45) 0.001 RBC (10^9/^/dl) 4,79 (0.38) 4,84 (0.39) 5,08 (0.37) 5,27 (0.36) 5,22 (0.35) 0.001 Hb (gr/dl) 12,95 (0.89) 13,31 (0.9) 14,35 (1.15) 14,96 (0.9) 15,25 (0.98) 0.001 HCT (%) 40,48 (2.67) 40,87 (2.69) 44,02 (3.5) 46,25 (2.83) 46,79 (2.81) 0.001 MCV (μm^3^) 84,00 (3.2) 84,45 (3.2) 86,75 (3.4) 87,88 (3.5) 89,7 (2.37) 0.001 MCH (pg) 27,07 (1.36) 27,62 (28.3) 28,28 (1.5) 28,46 (1.89) 29,24 (1.45) 0.001 MCHC (g/dl) 32,21 (0.95) 32,65 (9.5) 32,61 (1.5) 32,39 (1.37) 32,62 (1.37) 0.423 RDW (%) 9,9 (0.56) 9.67 (0.6) 9,76 (0.48) 9,78 (0.45) 9,63 (0.39) 0.174 Values are mean (SD): RBC-red blood cell count, Hct,- packed cell volume, Hb - hemoglobin concentration, MCV- mean corpuscular volume, MCH- mean corpuscular hemoglobin, MCHC - mean corpuscular hemoglobin concentration, RDW- red cell distribution width ANOVA test and multivariate tests (Pillal's trace, Wilks Lambda, Hotelling's trace, and Roy's largest root) showed high statistical level of significance between age different groups (*P*=0.001) for all studied parameters except MCHC (*P*=0.423) and RDW (*P*=0.174). Post hoc multiple comparisons tests for hematologic parameters between age different groups showed that subjects from U10 and U12 groups have similar values between themselves and significantly lower values from all other groups for all parameters except for MCHC and RDW. The similar situation is within U16 and U18 group. They have insignificantly different results between themselves (for RBC, Hb, Hct, MCV, MCH) and significantly higher mean values for these parameters from the younger groups. The subjects from U14 group showed statistically higher means for hematological parameters than U10 and U12 group, but statistically lower means than U16 and U18 group. Values are mean (SD): RBC- red blood cell count, Hct,- packed cell volume, Hb - hemoglobin concentration, MCV- mean corpuscular volume, MCH- mean corpuscular hemoglobin, MCHC - mean corpuscular hemoglobin concentration, RDW- red cell distribution width Hematologic parameters in girls ------------------------------- The mean values and standard deviations for general features and hematologic parameters for group of female participants are presented in [Table 2](#T2){ref-type="table"}. All parameters are shown for five age different subgroups. ANOVA test and multivariate tests showed that there is no significantly difference for all hematological parameters between age different groups (*P*\>0.05). Multiple comparisons test for hematologic parameters between age different groups showed that only subjects from U10 and U18 groups significantly differ for only two parameters, RBC (*P*=0.05) and MCH (*P*=0.28). The youngest group show significantly higher mean RBC than the oldest group. ###### General characteristics and hematologic parameters in female participants (8--18 yr, N=80) for age different subgroups ***Variable*** ***U10*** ***U12*** ***U14*** ***U16*** ***U18*** ***ANOVA, P*** ----------------- -------------- --------------- -------------- -------------- -------------- ---------------- Age(yr) 9.11 (0.42) 10.98 (0.56) 13.12 (0.25) 14.73 (0.51) 16.81 (0.45) 0.001 Height (cm) 133,87 (9.5) 149,34 (10.8) 162,46 (6.3) 164,71 (4.3) 170,25 (7.1) 0.001 Weight (kg) 32,0 (8.29) 44,78 (10.3) 51,85 (7.86) 58,18 (9.3) 62,94 (13.4) 0.001 RBC (10^9/^/dl) 4,99 (0.39) 4,71 (0.22) 4,71 (0.46) 4,68 (0.55) 4,59 (0.26) 0.349 Hb (gr/dl) 12,98 (1.26) 13,33 (1.0) 13,08 (1.38) 12,92 (1.1) 13,49 (1.5) 0.800 Hct (%) 40,61 (3.53) 40,50 (3.2) 40,72 (3.75) 40,6 (3.4) 41,27 (3.33) 0.990 MCV (μm^3^) 81,75 (6.86) 86,25 (34.3) 82,43 (17.5) 87,0 (7.0) 89,75 (3.85) 0.362 MCH (pg) 26,15 (2.74) 27,98 (2.1) 28,25 (3.43) 27,62 (3.16) 29,32 (2.08) 0.253 MCHC (g/dl) 31,94 (0.97) 32,69 (1.3) 30,59 (6.2) 30,18 (6.38) 32,61 (1.12) 0.490 RDW (%) 9,94 (0.58) 9,89 (0.65) 9,82 (0.88) 10,15 (0.78) 10,16 (0.61) 0.712 Comparison of red blood cell parameters by sex ---------------------------------------------- The comparison of the hematologic parameters for total male and female group is presented in [Table 3](#T3){ref-type="table"}. All studied parameters, except MCV and MCH, showed sex-related differences. Analysis of variance factorial analysis applied to the whole male and female groups showed that male participants have significantly higher red blood count (*P*\<0.001), Hemoglobin content (*P*\<0.001) and hematocrit *(P*\<0.001). No differences were found for mean corpuscular volume (MCV) and mean concentration of hemoglobin in one red blood cell (MCH), (*P*=0.292; *P*=0.563). MCHC, mean corpuscular concentration of hemoglobin in 1 L of RBC was significantly higher in boys (*P*=0.002) and RDW, the range of red blood cells width distribution were significantly wider in girls (*P*=0.004). ###### Comparison of hematologic parameters of physically active boys (N=240) and girls (N=80) ***Variable*** ***groups*** ***mean*** ***SD*** ***SE*** ***95% Confidence Interval for Mean*** ----------------- -------------- ------------ ---------- ---------- ---------------------------------------- ------- -------- ------- RBC (10^12^/dl) boys 5.02 0.42 0.274 4.97 5.08 24.450 0.001 girls 4.72 0.41 0.526 4.62 4.83 Hb (gr/dl) boys 14.08 1.29 0.084 13.92 14.25 25.617 0.001 girls 13.15 1.19 0.155 12.84 13.46 Hct (%) boys 43.37 3.85 0.249 42.88 43.86 23.622 0.001 girls 40.69 3.33 0.437 39.82 41.57 MCV (μm^3^) boys 86.27 4.03 0.261 85.75 86.78 1.115 0.292 girls 85.40 9.87 1.274 82.85 87.95 MCH (pg) boys 28.07 1.83 0.118 27.84 28.31 0.335 0.563 girls 27.90 2.84 0.374 27.15 28.65 MCHC (g/dl) boys 32.53 1.23 0.079 32.38 32.69 9.978 0.002 girls 31.51 4.37 0.574 30.36 32.66 RDW (%) boys 9.75 0.49 0.319 9.68 9.81 8.496 0.004 girls 9.98 0.72 0.943 9.79 10.17 Values are mean, SD-standard deviation, SE-standard error. The frequency of hemoglobin concentration is fewer than the lower boundary in nominal values, 12g/dl. With the boys, 4.6% showed subnormal values, i.e. the rest 95.4% used to have normal values. Frequency of suboptimal values of Hb with girls (13.3%) was significantly higher than with the boys (*P*=0.013) ([Table 4](#T4){ref-type="table"}). ###### Frequency of normal and low hemoglobin concentration in boys and girls ***Variable*** ***Hb lower than 12g/dl*** ***Hb normal values*** ***Total*** ***Chi-square test (Pearson)*** ---------------- ---------------------------- ------------------------ ------------- --------------------------------- ------- Male Count % 11 229 240 0.013 4.6% 95.4% 100% Female Count % 8 52 60 13.3% 86.7% 100% Total Count % 19 281 300 6.4% 93.6% 100% Discussion ========== In the Republic of Macedonia, there are no elaborate studies used as local reference ranges for basic RBC parameters and hematological indices for young population. The goal of this study was to help the physicians in comparing the laboratory test results with locally generated RBC variables values. The results of the present study support findings reported by number of authors that the red blood cell variables undergo age different changes in adolescents, and sex-related difference between boys and girls. Dependence of the hematologic parameters of age ----------------------------------------------- Children's reference ranges for routine hematological testing are usually stratified as reference values for newborn at birth, at 2 wk, 4 wk, 2--6 months, 6 months to year, 1 to 6 yr and 6--12 yr, for both sexes. Reference values for children older than 12 yr are different for male and female subjects ([@B16]). Some authors suggest different reference values for hematologic parameters for girls and boys after 13 yr of age ([@B17]). In this paper we decided to divide the examinees from 8 to 18 yr of age, into age different groups from 2-year intervals, groups. The mean values for RBC, Hct, Hb, MCV and MCH in male group showed tendency of increasing with the growth of the age. These parameters in groups U10 and U12 show significantly lower values than other (older) groups, and U16 and U18 show higher values for these parameters from other (younger group). Therefore, the U14 group has significantly higher values for most of the hematologic indices than U10 and U12, and significantly lower values than two older groups U16 and U18. These data indicate that boys older than 12 but younger than 14 year of age, are in the intermediate period regarding the hematological parameters. As far as the hematological indices with the male participants are concerned, the average size of erythrocyte (MCV) grows with the age. Average content, mass of hemoglobin in one erythrocyte (MCH), also grows gradually, with significantly highest values with U18, but with boys younger than 12 (U10 and U12) and boys older than 12 (U14, U16 and U18) there is a significant difference. The average concentration of hemoglobin in one erythrocyte (MCHC) does not show intergroup difference because the size of the cell is taken into consideration. The explanation is simple, with the age of the young examinees, the size of the cell grows and the average content of hemoglobin in it. But their ratio, i.e. concentration of hemoglobin in the cell remains approximately the same. Another parameter, RW, which describes the span of the size of different erythrocytes shown in percentages, does not show mutual difference which leads to equality of the size of erythrocytes in all different groups. The analysis of the hematological parameters with the girls showed that there was not statistically significant difference among the examined hematological parameters. Even though there was a significant difference in age, weight and height, there was not any significant difference found among the hematological parameters, except for the RBC and MCH between the youngest and the oldest group. When age different groups were compared, the only significant difference was found in the number of the erythrocytes (RBC) between the youngest (U10) and the oldest (U18) groups and it was in favor of the younger examinees. The amount of hemoglobin is similar in all groups (it increased insignificantly with the age), but the number of erythrocytes decreases insignificantly with the age and it is much bigger with U10 then with U18. The lack of this examination is that a fairly small number of girls were included, because of the low presence of girls as patients in our laboratory. A similar cross-sectional study of hematologic parameters was conducted in Spain where adolescents with age ranging from 13 to 18.5 yr old. Younger male subjects presented lower RBC, Hb, Hct and MCV mean values than their older counterparts. Same as in our study, these differences were not found in female subjects. As expected and as we found in this study, RBC, Hb, and Hct mean values were found significantly higher in males than in the females ([@B18]). Evaluation of hematologic indices in healthy Ugandan population (aged 1 to 94 yr) showed that erythrocytes, hemoglobin, hematocrit levels and mean corpuscular volume all significantly increased with age (*P*\<0.001) and were independent of age until the age of 13 yr (*P*\<0.001) ([@B19]). The hematologic parameters in youth national soccer teams were investigated and found no difference between U14, U15, and U16 groups, except for the RBC variable ([@B20]). Hemoglobin contents and the RBCs gradually rise to adult levels by the age of puberty ([@B21]). Investigation of hematological parameters in population 1 to 14 yr of age in Bangladesh showed difference between age groups and no difference was found between two sex groups ([@B22]). Dependence of hematologic parameters of sex ------------------------------------------- Men and women have different mean hemoglobin levels in health in venous blood --- women have mean levels approximately 12% lower than men. Since no difference is noticed in the level of erythropoietin with different sexes, the difference in the intensity of erythropoiesis comes from the physiological changes in the kidneys not in bone marrow ([@B9]). There is no evidence showing reduced cellular mechanisms for hem synthesis in women, and there is no difference in the iron absorption between women and men ([@B23]). The established reference ranges for woman are under the influence of large proportion of those with iron deficiency. ([@B11]). The difference in hemoglobin concentration regarding sex has not been found in infants and preschool children ([@B24]), but it has been shown in teenagers and adolescents ([@B25]). In our research, we compare the hematological parameters with male and female examinees, as well as whole groups regardless of their age. The male examinees showed significantly higher values of RBC (5.02 \*10^12^/l vs 4.72 \*10^12^/l; *P*\<0.001); higher values of Hb (14.08 g/dl vs 13.15 g/dl; *P*\<0.001); Hematocrit (43.37% vs 40.69%; *P*\<0.001). The average size of red blood cells (MCV) and medium content of Hb in them (MCH) insignificantly higher with the boys. Due to the similar size of the cells and higher total amount of hemoglobin with the males, MCHC, concentration of Hb in erythrocyte, is higher with the boys (*P*=0.002). The size span of erythrocytes is wider with the girls which lead to bigger variability of the erythrocytes size. For the clinical reference values of RBC, Hb, and Hct no sex differences were observed bellow the age of 12. The values for males were significantly higher than in females in the age range 13--79 ([@B26]). Unusual results are reported regarding the hematologic indices in male and female children younger than 12 yr. Mean Hb, Hct, MCV, and MCH of school-aged boys were significantly lower than girls ([@B27]). In the survey on haemoglobin level in the different age groups in man and woman in Indian population in the group aged 12 to 19 yr, males showed Hb mean concentration of 11.76 g/dl and female showed higher mean value, 12.31 g/dl ([@B28]). The research on hematological indices in in Kuwaiti children aged 7--12 yr, were RBC=4.78±0.42; Hb=127.3±9.4 /dl for boys and RBC=4.7±0.4; Hb=126.9±9.8 /dl for girls. Same parameters for older children, 13--17 yr, were RBC=5.18±0.48; Hb=145±14.4 /dl for boys and RBC=4.68±0.43; Hb=129.6±9.8 /dl for girls ([@B29]). As we can see these results are concordant with ours, regarding the sex differences (in favor of boys), and regarding the existing substantial age difference in male group and no age difference in female group. Normal hemoglobin levels according to WHO for children aged 5--12 yr above 11.5 gr/dl and teenagers aged 12--15 yr equal or above 12g/dl. Above 15 yr the adolescent are referred to as adults, and normal Hb level for adult male is 13.8--17.2 g/dl, and for adult female 12.1--15.1 g/dl ([@B30]). The primary aim of analyzing red blood cells variables is to discover and diagnose type of anemia in case it is present. Anemia was defined as hemoglobin concentration \<11g/dL for children aged between 6 and 59 months, while 11.5 g/dl for children aged 5 and 11 yr and \< 12 g/dl for children older than 12 yr according to WHO ([@B30]). As a lower boundary of nominal values for hemoglobin concentration in our laboratory is considered the value of 12 g/dl. In our laboratory that value is the same for both children and adults. Only 4.6% of our male examiners had low values of hemoglobin, and much more in the female group 13.3%. Conclusion ========== The young male examinees there exists a significant difference among different age groups, with special emphasis that hematological variables in boys aged 12 to 14 yr have the intermediate values between those with pre-puberty (\<12 yr) towards those adolescent boys (\>14 yr). RBC variables with girls from different age subgroups did not show significant differences. Significant difference is found only in red blood cell counts between the oldest (U18 group) and youngest (U12 group) in favor of the younger girls. RBC variables, regardless of the age, differ very much between male and female examiners, in favor of the male examinees. Hematological indices were insignificantly higher in males. Ethical considerations ====================== Ethical issues (Including plagiarism, informed consent, misconduct, data fabrication and/or falsification, double publication and/or submission, redundancy, etc.) have been completely observed by the authors. The researchers want to thank the Institute of Physiology, Medical Faculty, UKIM, Skopje, and all the people who had been involved in this study. **Conflict of interest** The authors declare that there is no conflict of interests.
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Q: Why isn't the acceleration at the top point of a ball’s journey zero? When I shoot a ball vertically upward, its velocity is decreasing since there is a downward acceleration of about $9.8\,\mathrm{ms}^{-2}$. I have read that at the top most point, when $v = 0$, the acceleration is still $9.8\,\mathrm{ms}^{-2}$ in the downward direction where $v=0$. That is, the acceleration is still the same. But at the highest point, the ball is stationary, so it is not even moving. How can it accelerate? A: You throw the ball upwards with velocity $v$ and it returns to your hand with velocity $-v$. Let's draw a graph showing the velocity as a function of time: Acceleration is defined as: $$ a = \frac{dv}{dt} $$ so it is the gradient of the line in this graph. The velocity-time line is straight so the gradient is constant which means the acceleration is constant. The gradient is just the gravitational acceleration $9.81$ m/s$^2$. The point is that the gradient, and hence the acceleration, does not depend on $v$ at all. So it is the same value of $9.81$ m/s$^2$ when $v = 0$ just as it is at all other values of $v$.
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AVR programming with Arduino Written by Victor van Poppelen The Arduino Nano The Nano is a very simple board, essentially just an AVR MCU with an FTDI chip for communicating over USB. On the top left of the schematic is the pinout of the board, and in the centre is the pinout of the AVR chip (an ATmega328 or ATmega328p). You can follow the pins to various components, and/or directly to the pins of the board itself. For example, the D0/TX and D1/RX pins on the board are connected to the PD0 and PD1 pins of the AVR, which are the UART TX and RX pins. The schematic is confusing at first but gets simpler once you see that every label is unique, and anywhere a label appears multiple times means they are connected at those points within the board. So, in the case of the D0 and D1 pins, they are connected to the AVR directly before the 1k resistors RP1B and RP1C , which are in turn connected to the TXD and RXD pins of the FT232RL (via the RX and TX labels, respectively). The FT232RL chip is a USB slave to UART converter that connects to the mini-USB connector (labelled USB-MINI-B%C ). The on-board voltage regulator UA78M05 accepts 7–25 V as input via VIN , and outputs a regulated 5 V up to 500 mA. Alternatively, USB can power the board directly. The components thus use a 5 V logic level to communicate binary signals. A binary signal is a form of modulation (the concept of encoding data within a signal, in this case electrical) using voltage level to determine a high value or a low value. The ‘‘logic level’’ determines the actual voltages used, in our case 5 V for high and 0 V for low. Whether high is considered a logical 1 (active-high) or a logical 0 (active-low) is dependent on the pin configuration. When a pin is configured to be active-low, it is usually labelled with a bar over it (as in RESET ) or appended with a # , but other conventions are also used. What you can tell from the schematic is that the UART pins of the AVR are directly connected to the pins of the board, but also connected to the FT232R. You can also tell that the FT232R is only connected to the AVR using these 2 pins, beyond a few power and reset pins. So if the computer (via USB) is only able to communicate with the FT232R, then clearly your only method of communicating with the AVR is via the UART. We will look at how to use the UART in a later section. Using the GNU toolchain We can use gcc and GNU binutils to program the AVR. For most systems, you will need to install a separate instance of gcc and binutils built to target AVR. The toolchain modules are invoked using the prefix avr- ; all the same flags and features are available. After cross-compiling a program for AVR, the resulting binary needs to be written to the flash and/or eeprom using a ‘‘programmer’’. The programmer requires a physical connection to the AVR, and uses an algorithm specified in the datasheet (chapter 28) to write the passed program to the chip. The usual tool for interfacing with the programmer is avrdude. We will be using a programmer called arduino, which is really just the Arduino bootloader pre-loaded in the AVR’s memory. The bootloader reads the binary via the UART and writes to the application memory space. The linker produces ELF-formatted binaries by default, but this programmer doesn’t accept those. Instead, we use Intel hex format binaries: avr-gcc -mmcu = atmega328p -Wl ,--oformat = ihex -o program.hex program.c Then we tell avrdude to upload the binary: avrdude -p atmega328p -c arduino -P /dev/ttyUSB0 -b 57600 -D -U flash:w:program.hex:i How do we know the baud rate should be 57600? Well, avrdude is communicating directly with the bootloader, so all we have to do is look at the bootloader code. The Microcontroller So far this doesn’t look too foreign. The differences show up when we try to actually write a program for the AVR. An MCU does not have the same features as a microprocessor. There is no kernel/user mode distinction, so the usual abstracted functions to access operating system services do not exist, as there is no operating system to speak of. There is only one process, delineated by the main() function, as process preemption requires a multitasking operating system (generally facilitated by virtual memory, which MCUs do not have). As such, your program must do all hardware initialization explicitly. Fortunately, MCUs are simple enough that this is a reasonable task. We can use avr-libc to provide basic macros and functions. The project attempts to mimic the C standard library, with the limitation that there is no operating system for hardware abstraction. The header file <avr/io.h> supplies macros for the registers of most available chips, and <avr/interrupt.h> supplies macros for interrupt vectors and initialization routines. Here is the AVR pinout from the datasheet, which you can cross-reference with the Arduino schematic: The chip is configured as having 3 ‘‘ports’’: Port B (corresponding to PBn pins), Port C ( PCn ), and Port D ( PDn ). The idea is that each port has 8 pins (except Port C, read Pin Descriptions in section 1.1) for parallel communication of bytes when configured for regular digital I/O (the default). Within each port, each pin also has alternatively configurable functions, which correspond to the parenthesized labels. So the UART pins, RXD and TXD , are alternative functions of the Port D pins 0 and 1. Other alternative functions include clock inputs ( XTALn , timers/counters and PWM s ( OCnx ), external interrupts ( PCINTn ), serial protocols like SPI ( SCK , MISO , MOSI , SS ) and I2C, ADC s ( ADCn ), and more. When the MCU begins program execution, no alternative pin functions are initialized. The only exception is PC6 , which is programmed with a fuse bit to configure reset functionality. All other port pins are set as tri-stated inputs (high-impedance, i.e. won’t source or sink current), and interrupts are disabled. The program must then configure how each pin should be used. A simple program could be to set Port B as an output, and increment the value input on Port D: #include <avr/io.h> int main ( void ) { DDRB = 0xff ; while ( 1 ) PORTB = 1 + PIND ; return 0 ; } The DDRx registers determine whether each pin of the corresponding port is an output or an input. Setting the register to 0xff configures all Port B pins as outputs. To specify only certain pins, we use the macro _BV , which is equivalent to (1 << Pxn) : DDRB |= _BV ( PB0 ); // To set PB0 as an output DDRB &= ~ _BV ( PB0 ); // To set PB0 as an input The PORTx registers are writeable I/O memory addresses to toggle outputs on the respective port. The PINx registers are readable addresses for capturing inputs. avr-libc hides the specific addresses within these macro definitions for each chip by including chip-specific header files in the <avr/io.h> header, switched by the -mmcu compiler flag. We use an infinite loop so that we are continuously sampling the input at Port D. Alternatively, we could set PORTB once, and then put the MCU to sleep to latch the value determined at program start. The UART A UART is a simple device for serial communication. Serial means data is sent in sequence over the same wire, as opposed to having, say, 8 wires transmit a byte all at once (called parallel communication). When two UARTs are connected for communication, the transmit pin TX of one is wired to the receive pin RX of the other, and vice versa. Both the AVR and the FT232R are full-duplex, meaning they can transmit and receive simultaneously, without having to take turns (half-duplex). On the host (computer) side, the FT232R driver exposes the communication as a TTY interface, which acts like a pipe to the FT232R. So if you write a character to the TTY (generally will be /dev/ttyUSB0), a data frame containing that character will pop out at the TXD pin of the FT232R, which is then connected to the RXD pin of the AVR. Conversely, if you program the AVR to transmit a character, it will send a data frame from its TXD pin, which is received by the RXD pin of the FT232R, which the Linux driver than decodes and writes to the TTY. If you then read from the TTY (e.g. cat /dev/ttyUSB0 ), you will retrieve the sent character. Because UARTs are asynchronous, and do not have a clock line for synchronization, they must synchronize over the same lines used for data transmission. This is only possible if the baud rate (same as the bit rate when using binary modulation) and frame format are agreed upon prior to communication. UARTs use a prescaler to divide the provided clock to a desired baud rate. With a given clock frequency, only a set number of baud rates can be configured. Section 20.10 of the AVR datasheet has a table of baud rate calculations for commonly-used clock frequencies. Not all standard baud rates are available for every frequency—due to the discrete number of prescaler values available—so the error to the nearest standard baud rate is listed. The range of acceptable errors is tabulated in section 20.8.3. To configure the baud rate, avr-libc provides macros in <util/setbaud.h>. To configure framing, we set the USART Control and Data Registers as outlined in section 20.4. The default is 8 data bits, no parity, and 1 stop bit—commonly used for serial communication with PCs. For the FT232R, you can set the baud rate via the Linux TTY driver. stty is a program used to alter TTY settings, including baud rate and frame format. You can also affect the TTY programmatically, via the termios structure in libc. The datasheet specifies prescaler options in section 4.2: [ … ] baud rates are calculated as follows - Where can be any integer between 2 and 16,384 ( = 214 ) and can be a sub-integer of the value 0, 0.125, 0.25, 0.375, 0.5, 0.625, 0.75, or 0.875. When , i.e. baud rate divisors with values between 1 and 2 are not possible. As an example, we could write a simple program that accepts characters from the host, and sends each character back incremented by one: #include <avr/io.h> #define F_CPU 16000000 #define BAUD 38400 #include <util/setbaud.h> int main ( void ) { UBRR0H = UBRRH_VALUE ; // UBRR is a 12-bit prescaler register UBRR0L = UBRRL_VALUE ; // The value is determined by util/setbaud.h UCSR0B = _BV ( TXEN0 ) | _BV ( RXEN0 ); // This enables the UART pins char c ; while ( 1 ) { loop_until_bit_is_set ( UCSR0A , RXC0 ); // Wait for a character c = UDR0 ; loop_until_bit_is_set ( UCSR0A , UDRE0 ); // Ensure the transmit buffer is empty UDR0 = c + 1 ; } return 0 ; } We set our clock rate F_CPU to match the frequency of the external crystal seen in the schematic. Then we select a baud rate that has a suitable error for both the AVR and the FTDI. Finally, we block on the values of RXC0 and UDRE0 to know when the receive and transmit buffers are ready for reading and writing, respectively. Simulating and debugging We can use simavr to simulate many AVR chips locally, including the ATmega328. simavr has GDB and VCD support, which is especially helpful to those who don’t have access to an oscilloscope, or don’t have an AVR at all. Datasheets and Documentation
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Machine learning defines models that can be used to predict occurrence of an event, for example, from sensor data or signal data, or recognize/classify an object, for example, in an image, in text, in a web page, in voice data, in sensor data, etc. Machine learning algorithms can be classified into three categories: unsupervised learning, supervised learning, and semi-supervised learning. Unsupervised learning does not require that a target (dependent) variable y be labeled in training data to indicate occurrence or non-occurrence of the event or to recognize/classify the object. An unsupervised learning system predicts the label, target variable y, in training data by defining a model that describes the hidden structure in the training data. Supervised learning requires that the target (dependent) variable y be labeled in training data so that a model can be built to predict the label of new unlabeled data. A supervised learning system discards observations in the training data that are not labeled. While supervised learning algorithms are typically better predictors/classifiers, labeling training data often requires a physical experiment or a statistical trial, and human labor is usually required. As a result, it may be very complex and expensive to fully label an entire training dataset. A semi-supervised learning system only requires that the target (dependent) variable y be labeled in a small portion of the training data and uses the unlabeled training data in the training dataset to define the prediction/classification (data labeling) model.
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Variation in nitrogen use efficiencies on Dutch dairy farms. On dairy farms, the input of nutrients including nitrogen is higher than the output in products such as milk and meat. This causes losses of nitrogen to the environment. One of the indicators for the losses of nitrogen is the nitrogen use efficiency. In the Dutch Minerals Policy Monitoring Program (LMM), many data on nutrients of a few hundred farms are collected which can be processed by the instrument Annual Nutrient Cycle Assessment (ANCA, in Dutch: Kringloopwijzer) in order to provide nitrogen use efficiencies. After dividing the dairy farms (available in the LMM program) according to soil type and in different classes for milk production ha(-1) , it is shown that considerable differences in nitrogen use efficiency exist between farms on the same soil type and with the same level of milk production ha(-1) . This offers opportunities for improvement of the nitrogen use efficiency on many dairy farms. Benchmarking will be a useful first step in this process.
3.40625
3
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According to an old tradition, the monastery was built where Mary, Joseph and the infant Jesus took shelter in a cave while fleeing from Herod the Great. This event is commemorated in the ground-floor crypt beneath the monastery church. An icon illustrates the Flight of the Holy Family into Egypt and a large painting depicts a contented Jesus being nursed at the breast by his mother Mary. Fresco of St Gerasimus with his lion (Bukvoed) The upper-floor church contains many holy icons and frescoes, including paintings of Gerasimus and his lion. Cabinets in the crypt store the bones of monks killed during the Persian invasion of 614. Hospitable place for pilgrims A place of hospitality and refreshment for pilgrims, with fruit trees, flowers and birdsong, the gold-domed monastery offers a contrast to the hot and barren environment of the Judaean wilderness. Founded in the fifth century, it was originally dedicated to Our Lady of Kalamon (Greek for reeds), but was later renamed in honour of Gerasimus, who founded a nearby monastery that had been abandoned. It was destroyed in 614, rebuilt by the Crusaders, abandoned after the Crusader period, restored in the 12th century, rebuilt in 1588, destroyed around 1734 and re-established in 1885. In Arabic it is known as Deir Hajla, meaning the monastery of the partridge, a bird common to the area. The monastery functioned in the form of a laura — with a cluster of hermits’ caves located around a community and worship centre. The hermits spent weekdays alone in their caves, occupied in prayer and making ropes and baskets. They went to the centre for Saturdays and Sundays, taking their handiwork and partaking in Divine Liturgy and communal activities. The monastic rule was strict. During the week the hermit monks survived on dry bread, dates and water. At the weekends they ate cooked food and drank wine. Their only personal belongings were a rush mat and a drinking bowl. Hermits’ caves can still be seen in the steep cliffs a kilometre east of the monastery and in the adjacent mountains. Gerasimus redeveloped monastic life Like many who founded Judaean monasteries, Gerasimus (also spelt Gerassimos or Gerasimos) came from outside the Holy Land — from a wealthy family in Lycia, in present-day Turkey. Already a monk when he came to Palestine, he followed the monastic leader Euthymius into the desert and became renowned for his piety and asceticism. Because of the similarity of names, Gerasimus is sometimes confused with St Jerome, the Bible translator who lived in Bethlehem. Gerasimus is credited with a new development in monastic life. Previously desert monks lived either in caves or in monasteries. He was the first to combine the solitude of a wilderness hermit with the communal aspect of a monastery by bringing hermits together on Saturdays and Sundays for worship and fellowship. He is believed to have attended the crucial Council of Chalcedon in 451, which caused a major rift in the Eastern Orthodox world. Called to settle differences of opinion on the nature of Christ, the council declared that he has two natures in one Person as truly God and truly man. Gerasimus briefly opposed this declaration, then accepted it. The lion depicted in icons of Gerasimus comes from a story that he found the animal wandering in the desert, suffering from a thorn embedded in a paw. The saint gently removed the thorn and tended to the wound. The lion thereafter devoted himself to Gerasimus, serving him and the monastery and retrieving the monastery’s donkey when it was stolen by thieves. The story has it that when Gerasimus died in 475 the lion lay on his grave and died of grief.
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Supraoptic nucleus The supraoptic nucleus (SON) is a nucleus of magnocellular neurosecretory cells in the hypothalamus of the mammalian brain. The nucleus is situated at the base of the brain, adjacent to the optic chiasm. In humans, the SON contains about 3,000 neurons. Function The cell bodies produce the peptide hormone vasopressin, which is also known as anti-diuretic hormone (ADH). This chemical messenger travels via the bloodstream to its target cells in the papillary ducts in the kidneys, enhancing water reabsorption. In the cell bodies, the hormones are packaged in large, membrane-bound vesicles that are transported down the axons to the nerve endings. The secretory granules are also stored in packets along the axon called Herring bodies. Similar magnocellular neurons are also found in the paraventricular nucleus. Signaling Each neuron in the nucleus has one long axon that projects to the posterior pituitary gland, where it gives rise to about 10,000 neurosecretory nerve terminals. The magnocellular neurons are electrically excitable: In response to afferent stimuli from other neurons, they generate action potentials, which propagate down the axons. When an action potential invades a neurosecretory terminal, the terminal is depolarised, and calcium enters the terminal through voltage-gated channels. The calcium entry triggers the secretion of some of the vesicles by a process known as exocytosis. The vesicle contents are released into the extracellular space, from where they diffuse into the bloodstream. Regulation of supraoptic neurons Vasopressin (antidiuretic hormone, ADH) is released in response to solute concentration in the blood, decreased blood volume, or blood pressure. Some other inputs come from the brainstem, including from some of the noradrenergic neurons of the nucleus of the solitary tract and the ventrolateral medulla. However, many of the direct inputs to the supraoptic nucleus come from neurons just outside the nucleus (the "perinuclear zone"). Of the afferent inputs to the supraoptic nucleus, most contain either the inhibitory neurotransmitter GABA or the excitatory neurotransmitter glutamate, but these transmitters often co-exist with various peptides. Other afferent neurotransmitters include noradrenaline (from the brainstem), dopamine, serotonin, and acetylcholine. The supraoptic nucleus as a "model system" The supraoptic nucleus is an important "model system" in neuroscience. There are many reasons for this: Some technical advantages of working on the supraoptic nucleus are that the cell bodies are relatively large, the cells make exceptionally large amounts of their secretory products, and the nucleus is relatively homogeneous and easy to separate from other brain regions. The gene expression and electrical activity of supraoptic neurons has been studied extensively, in many physiological and experimental conditions. These studies have led to many insights of general importance, as in the examples below. Morphological plasticity in the supraoptic nucleus Anatomical studies using electron microscopy have shown that the morphology of the supraoptic nucleus is remarkably adaptable. For example, during lactation there are large changes in the size and shape of the oxytocin neurons, in the numbers and types of synapses that these neurons receive, and in the structural relationships between neurons and glial cells in the nucleus. These changes arise during parturition, and are thought to be important adaptations that prepare the oxytocin neurons for a sustained high demand for oxytocin. Oxytocin is essential for milk let-down in response to suckling. These studies showed that the brain is much more "plastic" in its anatomy than previously recognized, and led to great interest in the interactions between glial cells and neurons in general. Stimulus-secretion coupling In response to, for instance, a rise in the plasma sodium concentration, vasopressin neurons also discharge action potentials in bursts, but these bursts are much longer and are less intense than the bursts displayed by oxytocin neurons, and the bursts in vasopressin cells are not synchronised. It seemed strange that the vasopressin cells should fire in bursts. As the activity of the vasopressin cells is not synchronised, the overall level of vasopressin secretion into the blood is continuous, not pulsatile. Richard Dyball and his co-workers speculated that this pattern of activity, called "phasic firing", might be particularly effective for causing vasopressin secretion. They showed this to be the case by studying vasopressin secretion from the isolated posterior pituitary gland in vitro. They found that vasopressin secretion could be evoked by electrical stimulus pulses applied to the gland, and that much more hormone was released by a phasic pattern of stimulation than by a continuous pattern of stimulation. These experiments led to interest in "stimulus-secretion coupling" - the relationship between electrical activity and secretion. Supraoptic neurons are unusual because of the large amounts of peptide that they secrete, and because they secrete the peptides into the blood. However, many neurons in the brain, and especially in the hypothalamus, synthesize peptides. It is now thought that bursts of electrical activity might be generally important for releasing large amounts of peptide from peptide-secreting neurons. Dendritic secretion Supraoptic neurons have typically 1-3 large dendrites, most of which projecting ventrally to form a mat of process at the base of the nucleus, called the ventral glial lamina. The dendrites receive most of the synaptic terminals from afferent neurons that regulate the supraoptic neurons, but neuronal dendrites are often actively involved in information processing, rather than being simply passive receivers of information. The dendrites of supraoptic neurons contain large numbers of neurosecretory vesicles that contain oxytocin and vasopressin, and they can be released from the dendrites by exocytosis. The oxytocin and vasopressin that is released at the posterior pituitary gland enters the blood, and cannot re-enter the brain because the blood–brain barrier does not allow oxytocin and vasopressin through, but the oxytocin and vasopressin that is released from dendrites acts within the brain. Oxytocin neurons themselves express oxytocin receptors, and vasopressin neurons express vasopressin receptors, so dendritically-released peptides "autoregulate" the supraoptic neurons. Francoise Moos and Phillipe Richard first showed that the autoregulatory action of oxytocin is important for the milk-ejection reflex. These peptides have relatively long half-lives in the brain (about 20 minutes in the CSF), and they are released in large amounts in the supraoptic nucleus, and so they are available to diffuse through the extracellular spaces of the brain to act at distant targets. Oxytocin and vasopressin receptors are present in many other brain regions, including the amygdala, brainstem, and septum, as well as most nuclei in the hypothalamus. Because so much vasopressin and oxytocin are released at this site, studies of the supraoptic nucleus have made an important contribution to understanding how release from dendrites is regulated, and in understanding its physiological significance. Studies have demonstrated that secretin helps to facilitate dendritic oxytocin release in the SON, and that secretin administration into the SON enhances social recognition in rodents. This enhanced social capability appears to be working through secretin's effects on oxytocin neurons in the SON, as blocking oxytocin receptors in this region blocks social recognition. Co-existing peptides Vasopressin neurons and oxytocin neurons make many other neuroactive substances in addition to vasopressin and oxytocin, though most are present only in small quantities. However, some of these other substances are known to be important. Dynorphin produced by vasopressin neurons is involved in regulating the phasic discharge patterning of vasopressin neurons, and nitric oxide produced by both neuronal types is a negative-feedback regulator of cell activity. Oxytocin neurons also make dynorphin; in these neurons, dynorphin acts at the nerve terminals in the posterior pituitary as a negative feedback inhibitor of oxytocin secretion. Oxytocin neurons also make large amounts of cholecystokinin as well as the cocaine and amphetamine regulatory transcript (CART). See also Paraventricular nucleus References External links Category:Neuroendocrinology Category:Hypothalamus
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Q: Please help me understand this. $\frac{dx}{dt} = S x (a-x)$. What does it mean for some constant $S$? How to find $x$ for fastest/slowest growth? I am having some trouble understanding this problem. There is this function that calculates reaction rate of a substance for some constant positive $S$. $a$ = original amount of the first substance $x$ = some amount of substance First question, what does $\frac{dx}{dt} = S x (a-x)$ mean? Does this mean that the rate of change of $x$ in the equation $(S x (a-x))$ is affected by the change in time? So if there was no '$x$' in the equation, than change in time would not affect the equation right? *This is the first time I am encountering '$dt$' in my derivative assignments. When finding derivatives for simple equations, its mostly been of d/dx notation. When I graphed $S x (a-x)$, I substituted random numbers for $S$ and $a$. Does this tell me anything about the function for rate of increase and decrease? Should I have solved for $a$? I notice the function increases and then decreases as $x$ moves away from $0$. I also know that when the derivative crosses the $x$ axis, the original function (which I don't know) will start to decrease. What do I need to do to determine the fastest/slowest growth rate using the derivative? Thanks A: It means that the amount $x(t)$ is a function of time (makes sense) and tells you that the rate of change of $x$ is a function of $x$ itself. If the right hand side were a constant, then the rate of change would be constant: every second the amount $x$ would increase by $S$. I'm sure in Calculus you've already seen examples of functions where the right-hand side depended on $t$. If that were the case, then you could calculate $x(t)$, given the formula for $dx/dt$, by integrating both sides, e.g. finding the area under the curve of $dx/dt$. Here the situation is a bit different, since the derivative depends on $x$ itself, and not $t$. It takes some getting used to but conceptually, the formula tells you the slope of $x(t)$, given the current value of $x(t)$. In this particular case, if there is no material ($x=0$) or there is exactly $a$ amount of material, then $dx/dt=0$ and the system is in equilibrium: the slope is 0 and $x$ does not change over time. If $x$ is between 0 and $a$, then $dx/dt$ is positive and $x$ will increase over time. As $x$ increases and approaches $a$, the rate of increase decreases. If $x$ is over $a$, then $dx/dt$ is negative and $x$ decreases over time towards $a$. The maximum increase will occur when $Sx(a-x)$ is most positive; you can find the value of $x$ as usual, by taking the derivative of $Sx(a-x)$ with respect to $x$ and setting it equal to zero. The equation $dx/dt = Sx(t)[a-x(t)]$ is called an ordinary differential equation and given the initial value of $x$ at time 0, $x(0)$, you can solve it for the function $x(t)$ which gives $x$ at all times, although you have probably not learned the techniques yet. Here are some plots of $x(t)$ for $S=1$, $a=1$, and several different values of $x(0)$: You can see the main characteristics of the system here, namely, that $x$ either decreases or increases towards $a$ depending on where it starts.
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Skeletal Dysplasias: An Overview. Constitutional disorders of bone, commonly termed skeletal dysplasias (SDs), are inherited disorders of cartilage and/or bone that affect their growth, morphometry and integrity. Associated skeletal abnormalities are usually but not invariably symmetrical. They may be classified as osteochondrodysplasias, which are conditions associated with abnormalities of the growth (dysplasias) or texture (osteodystrophy) of bone and/or cartilage, or dysostoses, which are conditions secondary to abnormal blastogenesis (occurring at or around the 6th week of in utero life). Skeletal involvement may also occur in other multisystem hereditary and acquired syndromes. The 2010 Nosology and Classification of Genetic Skeletal Disorders listed 456 conditions, of which approximately 50 are perinatally lethal, and 316 are associated with one or more of 226 genes. When an SD is suspected, a standard series of radiographs, collectively known as a skeletal survey, should be performed. The diagnosis of individual conditions is highly dependent on radiographic pattern recognition, which is achieved through a systematic review of the images and enhanced by discussion with colleagues and through the use of available tools, such as atlases and digital databases. This article summarises a systematic approach to the diagnosis of SDs, demonstrated using examples of some of the more common lethal and non-lethal conditions.
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WASH interventions were typically community-based. WASH interventions were delivered to households and communities through community mobilization, mass media, home visits, and infrastructural development (126, 130, 136–138). There were some examples of facility-based delivery of WASH interventions, such as in health clinics and schools (139, 140); however, this was not representative of the majority of delivery platform coverage. Health clinic delivery platforms had limited reach, often targeting pregnant women and women with young children. In an evaluation of WASH interventions delivered in India (141), more demanding behavioral practices, such as handwashing and consistent use of latrines, required more intense contact (e.g., multiple home visits) than less intense interventions, such as sweeping of courtyards, that could be effectively delivered in small group meetings such as those in health clinics and community centers. More research is needed to evaluate the benefits and barriers of different delivery platforms for women across the life course. UN Women believe that violence against women "is rooted in gender-based discrimination and social norms and gender stereotypes that perpetuate such violence", and advocate moving from supporting victims to prevention, through addressing root and structural causes. They recommend programmes that start early in life and are directed towards both genders to promote respect and equality, an area often overlooked in public policy. This strategy, which involves broad educational and cultural change, also involves implementing the recommendations of the 57th session of the UN Commission on the Status of Women[146] (2013).[147][148][149] To that end the 2014 UN International Day of the Girl Child was dedicated to ending the cycle of violence.[112] In 2016, the World Health Assembly also adopted a plan of action to combat violence against women, globally.[150] A BMI of 25 to 29.9 is considered overweight and one 30 or above is considered obese. For an idea of what this means, a 5-foot 5-inch woman who weighs 150 pounds is overweight with a BMI of 25. At 180 pounds, she would be considered obese, with a BMI of 30. Keep in mind that the tables aren't always accurate, especially if you have a high muscle mass; are pregnant, nursing, frail or elderly; or if you are a teenager (i.e., still growing). Child marriage (including union or cohabitation)[91] is defined as marriage under the age of eighteen and is an ancient custom. In 2010 it was estimated that 67 million women, then, in their twenties had been married before they turned eighteen, and that 150 million would be in the next decade, equivalent to 15 million per year. This number had increased to 70 million by 2012. In developing countries one third of girls are married under age, and 1:9 before 15.[92] The practice is commonest in South Asia (48% of women), Africa (42%) and Latin America and the Caribbean (29%). The highest prevalence is in Western and Sub-Saharan Africa. The percentage of girls married before the age of eighteen is as high as 75% in countries such as Niger (Nour, Table I).[11][92] Most child marriage involves girls. For instance in Mali the ratio of girls to boys is 72:1, while in countries such as the United States the ratio is 8:1. Marriage may occur as early as birth, with the girl being sent to her husbands home as early as age seven.[11] Popular belief says if you really want to make a big change, focus on one new healthy habit at a time. But Stanford University School of Medicine researchers say working on your diet and fitness simultaneously may put the odds of reaching both goals more in your favor. They followed four groups of people: The first zoned in on their diets before adding exercise months later, the second did the opposite, the third focused on both at once, and the last made no changes. Those who doubled up were most likely to work out 150 minutes a week and get up to nine servings of fruits and veggies daily while keeping their calories from saturated fat at 10 percent or less of their total intake.
3.28125
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Phyisicists created atom-thin sheets of silicon - and named the new material Silicene. The idea to create such sheets from Silicon emerged in 2007 - even though silicon doesn't naturally form the required atomic bonds. Silicene has a similar pattern to Graphene and possibly has the same electronic properties and might have advantages of Graphene because silicon is more integrateable into today's electronic devices. The Silicene was created by growing a thin layer of silicon on top of a ceramic material called zirconium diboride. X-rays shined on this thin layer of silicon revealed a honeycomb of hexagons similar to the structure of graphene.
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Sunflowers is a genus of plants comprising about 70 species in the family Asteraceae. Except for three species in South America, all Helianthus species are native to North America. The common name, “sunflower,” also applies to the popular annual species Helianthus annuus, the common sunflower. This and other species, notably Jerusalem artichoke (H. tuberosus), are cultivated in temperate regions as food crops and ornamental plants. The genus is one of many in the Asteraceae that are known as sunflowers. It is distinguished technically by the fact that the ray flowers, when present, are sterile, and by the presence on the disk flowers of a pappus that is of two awn-like scales that are caducous (that is, easily detached and falling at maturity). Some species also have additional shorter scales in the pappus, and there is one species that lacks a pappus entirely. Another technical feature that distinguishes the genus more reliably, but requires a microscope to see, is the presence of a prominent, multicellular appendage at the apex of the style. Sunflowers are especially well known for their symmetry based on Fibonacci numbers and the Golden angle. There is quite a bit of variability among the perennial species that make up the bulk of the species in the genus. Some have most or all of the large leaves in a rosette at the base of the plant and produce a flowering stem that has leaves that are reduced in size. Most of the perennials have disk flowers that are entirely yellow, but a few have disk flowers with reddish lobes. One species, H. radula, lacks ray flowers altogether.
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Metal-insulator-metal (MIM) capacitors and metal-oxide-metal (MOM) capacitors are among the most widely used capacitors in integrated circuits. FIG. 1 illustrates a typical MIM capacitor, which includes bottom plate 2, top plate 6, and insulation layer 4 therebetween. The bottom plate 2 and top plate 6 are formed of conductive materials. As is known in the art, the capacitance of a capacitor is proportional to its area and the dielectric constant (k) of the insulation layer, and is inversely proportional to the thickness of the insulation layer. Therefore, to increase the capacitance, it is preferable to increase the area and the k value and to reduce the thickness of the insulation layer. However, the thickness and the k value are often limited by the technology used for forming the capacitor. For example, the thickness cannot be less than what the existing technology allows. On the other hand, since the capacitors are often formed in low-k dielectric layers, the ability to increase the k value is also limited. Methods for increasing the area of the capacitor have been explored. A problem associated with increasing area is that greater chip area is required. This dilemma is solved by the introduction of vertical (multi-layer) capacitors. A typical vertical MOM capacitor 10 is shown in FIGS. 2, 3, and 4. FIG. 2 illustrates a perspective view of MOM capacitor 10, which includes metal electrodes 12 and 14 separated by dielectric materials. Each of the metal electrodes 12 and 14 forms a three-dimensional structure. For clarity, metal electrode 12 is not shaded, while metal electrode 14 is shaded with dots. Each of the metal electrodes 12 and 14 includes more than one layer interconnected by vias. FIG. 3 illustrates a top view of a first metal layer (please refer to the middle layer in FIG. 2). Metal electrode 12 includes fingers 122, and bus 121 for interconnecting fingers 122. Metal electrode 14 includes fingers 142, and bus 141 for interconnecting fingers 142. Fingers 122 and 142 are placed in an alternating pattern with a very small space between the neighboring fingers. Therefore, each finger 122/142 forms a sub capacitor(s) with its neighboring fingers 142/122 or a bus 141/121. The total capacitance is equivalent to the sum of the sub capacitors. FIG. 4 illustrates a top view of the capacitor 10 in a second metallization layer (refer to the top or the bottom layer in FIG. 2), which overlies the bottom metallization layer. Typically, the direction of the fingers in the second metallization layer is orthogonal to the direction of the fingers in the bottom metallization layer. Similarly, electrodes 12 and 14 in the second metallization layer include buses 121 and 141 and a plurality of fingers 122 and 142, respectively. Typically, buses 121 in all the layers have similar shapes and sizes and are overlapped vertically. Buses 141 in all the layers also have similar shapes and sizes and are overlapped vertically. Vias 16 connect buses 121 in the first and the second metallization layers, thereby forming an integral electrode 12. Similarly, vias 18 connect buses 141 in neighboring layers, thereby forming an integral electrode 14. To further increase the capacitance of MOM capacitors, the regions underlying the bottom metallization layer were also used to form a layer of the MOM capacitors. The resulting structure is similar to the structure as shown in FIG. 2, except that layer 1 of the MOM capacitor 10 is now formed in an inter-layer dielectric layer. Referring back to FIG. 3, in this case, electrodes 12 and 14 are formed of doped polysilicon, and layers 1 and 2 are interconnected by contact plugs, instead of vias. The introduction of the polysilicon MOM layer results in the increase in capacitance of the MOM capacitors. However, the use of polysilicon causes the degradation of the high-frequency response of the MOM capacitors, particularly at frequencies of about 1 GHz or higher. For example, the Q-factors of the capacitors having polysilicon layers may be degraded by about 74% compared to the MOM capacitors that have all layers formed of metals. Accordingly, new structures and manufacturing methods are needed to take advantage of the increased capacitance by forming a capacitor layer underlying the bottom metallization layer, without sacrificing high-frequency response.
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One of the most dramatic aspects of virology is the emergence of new virus diseases, which often receives widespread attention from the scientific community and the lay public. Considering that the discipline of animal virology was established over 100 years ago, it may seem surprising that new virus diseases are still being discovered. How this happens is the subject of this chapter. 1. How Do New Viral Diseases Emerge? {#s0010} ==================================== There are many recent books and reviews (see [Further Reading](#fread0010){ref-type="sec"}) that list the plethora of determinants that can lead to the emergence of infectious diseases ([Table 1](#t0010){ref-type="table"} ). In this chapter, we concentrate on those determinants that relate to viral pathogenesis and deal only briefly with the many societal and environmental factors that can be instrumental in disease emergence.Table 1Some of the Factors that Lead to Emergence or Reemergence of Viral DiseasesFactors Leading to EmergenceDeterminantEconomic and social developmentPopulation growth, density, distributionEnvironmental changes such as deforestation, dam building, global warmingIncreased global travelIncreased international commerceAgribusiness, food processing, distributionPovertyInadequate public health systemsOpen defecationLack of safe waterSocietal breakdownCivil chaosWarHuman factorsSexual activitySubstance abuseBiological factorsNatural mutationAntimicrobial resistanceImmunosuppression 1.1. Discovery of the Etiology of an Existing Disease {#s0015} ----------------------------------------------------- In some instances, the "emergence" of a viral disease represents the first identification of the cause of a well-recognized disease. An example is La Crosse virus, a mosquito-transmitted bunyavirus that was first isolated from a fatal case of encephalitis in 1964. The isolation of the causal agent and the development of serological tests made it possible to distinguish La Crosse encephalitis from the rubric of "arbovirus encephalitis, etiology unknown." Since that time, about 100 cases have been reported annually, without any significant increase since the 1970s. It appears that the emergence of this "new" disease reflected only the newfound ability to identify this etiologic entity, rather than any true change in its occurrence. Hantavirus pulmonary syndrome is another example of the "emergence" of an existing but previously unrecognized disease. In 1993, in the four corners area of the southwestern United States, there occurred a small outbreak of cases of acute pulmonary illness with a high mortality. Epidemiologic and laboratory investigation rapidly identified the causal agent, a previously unknown hantavirus, now named Sin Nombre virus (SNV). SNV is an indigenous virus of deer mice (*Peromyscus maniculatus*) that are persistently infected and excrete the virus. Apparently deer mice produce virus-infected excreta and, when they infest human dwellings, aerosolized fomites can result in occasional human infections. The 1993 outbreak is thought to reflect a transient rise in deer mouse populations associated with an unusual crop of pine nuts, a major food source for these rodents. The recognition of SNV soon led to the discovery of other heretofore unrecognized hantaviruses in North, Central and South America, many of which also cause serious human disease. 1.2. Increase in Disease Caused by an Existing Virus {#s0020} ---------------------------------------------------- On occasion, a virus that is already widespread in a population can emerge as a cause of epidemic or endemic disease, due to an increase in the ratio of cases to infections. Such an increase can be caused by either an increase in host susceptibility or enhancement of the virulence of the virus. Although counterintuitive, there are some dramatic instances of such phenomena. **Increase in host susceptibility.** Poliomyelitis first appeared as a cause of summer outbreaks of acute infantile paralysis in Sweden and the United States late in the nineteenth century ([Figure 1](#f0010){ref-type="fig"} ). Isolated cases of infantile paralysis had been recorded in prior centuries, and an Eygptian tomb painting indicates that poliomyelitis probably occurred in early recorded history. Why then did poliomyelitis emerge abruptly as an epidemic disease? When personal hygiene and public health were primitive, poliovirus circulated as a readily transmitted enterovirus, and most infants were infected while they still carried maternal antibodies (up to 9--12 months of age). Under these circumstances, the virus produced immunizing infections of the enteric tract, but passively acquired circulating antibodies prevented invasion of the spinal cord. With the improvement of personal hygiene in the late-nineteenth century, infections were delayed until 1--3 years of age, after the waning of maternal antibodies. Infections now occurred in susceptible children, resulting in outbreaks of infantile paralysis. This reconstruction is supported by seroepidemiological studies conducted in North Africa in the 1950s, when epidemic poliomyelitis first emerged in this region.Figure 1The appearance of epidemic poliomyelitis in the United States, 1885--1916. The graph is based on reported cases (mainly paralytic) during an era when reporting was estimated at about 50%.Data from Lavinder CH, Freeman SW, Frost WH. Epidemiologic studies of poliomyelitis in New York City and the northeastern United States during the year 1916. Washington: United States Public Health Service (1918). **Increase in viral virulence.** Viruses may undergo sudden increases in virulence resulting in emergence of dramatic outbreaks. An outbreak of lethal avian influenza in Pennsylvania in 1983 is one documented example. In eastern Pennsylvania, avian influenza appeared in chicken farms early in 1983, but the virus was relatively innocuous and most infections were mild. However, in the fall of that year a fatal influenza pandemic spread rapidly through the same farms. When viruses from the spring and fall were compared, it appeared that both isolates had almost identical genomes. The fall virus had acquired a single point mutation in the viral hemagglutinin that facilitated the cleavage of the hemagglutinin. The virus could now replicate outside the respiratory tract, markedly increasing its virulence (discussed in Chapter 7, Patterns of infection). This point mutation led to the emergence of an overwhelming epizootic, which was only controlled by a widespread slaughter program involving millions of birds. Similar outbreaks of avian influenza have occurred subsequently in other countries. 1.3. Accumulation of Susceptible Hosts and Viral Reemergence {#s0025} ------------------------------------------------------------ A virus that is endemic in a population may "fade out" and disappear, because the number of susceptibles has fallen below the critical level required for perpetuation in that population. If the population is somewhat isolated, the virus may remain absent for many years. During this interval, there will be an accumulation of birth cohorts of children who are susceptible. If the virus is then reintroduced, it can "reemerge" as an acute outbreak. In the years 1900--1950, Iceland had a population of about 200,000, which was too small to maintain measles virus, and measles periodically disappeared. When travelers to Iceland reintroduced the virus, measles reemerged in epidemic proportions. 1.4. Virus New to a Specific Population {#s0030} --------------------------------------- On occasion, a virus can enter and spread in a region where it had never previously circulated, leading to the emergence of a disease new to that locale. A dramatic example is afforded by the emergence of West Nile virus (WNV) in the United States, beginning in 1999 ([Figure 2](#f0015){ref-type="fig"} ). WNV, like most arboviruses, is usually confined to a finite geographic area, based on the range of its vertebrate reservoir hosts and permissive vectors. In an unusual event, WNV was imported into New York City, probably by the introduction of infected vector mosquitoes that were inadvertent passengers on a flight from the Middle East, where the virus is enzootic. This hypothesis was supported by the finding that the genomic sequence of the New York isolates was closely related to the sequence of contemporary isolates from Israel. Some American mosquito species were competent vectors for WNV, and certain avian species such as American crows were highly susceptible. As a result, West Nile encephalitis emerged as a significant disease new to the United States. Over a period of several years WNV spread across the continent, finally reaching the west coast and many areas in Latin America.Figure 2The emergence of West Nile virus in the United States, 1999--2005. West Nile virus neuroinvasive disease incidence reported to CDC ArboNET, by state, United States, 1999, 2001, 2002, and 2005.Accessed via <http://www.cdc.gov/westnile/statsMaps/finalMapsData/index.html>, December 20, 2014. Chikungunya virus (CHIKV), another mosquito-borne arbovirus, has been endemic for many years in regions of Africa and Asia where it periodically caused outbreaks of a febrile illness associated with severe arthritis and arthralgia. In 2005--2006, CHIKV caused a large epidemic on the island of Reunion in the Indian Ocean, apparently associated with a mutation that allowed the virus to be more efficiently transmitted by vector mosquitoes. Chikungunya subsequently spread to India and elsewhere in Asia, followed by the Americas. As of November 2014, transmission of CHIKV had been documented in 40 countries or territories in the Caribbean, Central, South and North America, resulting in nearly one million suspected cases each year. It appears that CHIKV may become established in the New World, where virtually the entire human population currently lacks immunity. 2. Zoonotic Infections as a Source of Emerging Viral Diseases {#s0035} ============================================================= Zoonotic infections of animals that can be transmitted to humans are a major cause of emerging virus diseases of humans. These viruses are transmitted by direct contact, by virus-laden droplets or aerosols, or by insect vectors. All zoonotic viruses have one or more animal reservoir hosts, which play an important role in the epidemiological dynamics of human infections. Although many zoonotic viruses can be transmitted to humans on occasion, their relative ability to spread from human to human determines whether or not they emerge as significant new virus diseases of mankind ([Table 2](#t0015){ref-type="table"} ).Table 2Zoonotic Virus Infections of Humans and the Extent of Their Human-to-Human TransmissionExtent of Human-to-Human SpreadVirusMaintenance Cycle in NatureNot contagious from human-to-human (humans are dead-end hosts; representative examples); the most frequent patternWest Nile (flavivirus)Mosquitoes, birdsYellow fever (flavivirus)Mosquitoes, primatesLa Crosse encephalitis (bunyavirus)Mosquitoes, wild rodentsRabies (rhabdovirus)Raccoons, skunks, bats, dogsLimited (\<10) human-to-human transmissions; an uncommon patternCrimean Congo hemorrhagic fever (bunyavirus)\ 1--3 serial infectionsTicks, agricultural and wild animalsLassa, Machupo, Junin (arenavirus)\ 1--8 serial infectionsRodentsMonkeypox (poxvirus)\ \<6 serial infectionsRodentsEbola, Marburg (filovirus)\ 1--4 serial infections[∗](#tbl2fn1){ref-type="table-fn"}Bats?MERS (coronavirus)Bats? camels?Nipah (paramyxovirus)Bats, pigsUnlimited human-to-human transmission (a new human virus); a rare patternHIV (lentivirus)Monkeys, apesSARS (coronavirus)Bats, other animals?Influenza (type A influenza virus)Wild birds, domestic poultry, domestic pigsEbola, Marburg (filovirus)\ \>10 serial infectionsBats?[^1] 2.1. Dead-end Hosts {#s0040} ------------------- Most zoonotic viruses that are transmitted to humans cannot be spread directly from person to person, so humans are considered to be "dead-end hosts." One familiar example is rabies, which is enzootic in several animal hosts, such as dogs, skunks, foxes, raccoons, and bats. Humans are infected by bite of a rabid animal or by aerosol exposure (in caves with roosting bats). Several zoonotic arenaviruses, such as Lassa, Machupo (Bolivian hemorrhagic fever), and Junin (Argentine hemorrhagic fever) viruses, are likely transmitted from the reservoir host (wild rodents) by inhalation of contaminated aerosols. There are more than 500 viruses---belonging to several virus families---that are also classified as arboviruses (arthropod-borne viruses), based on a vertebrate--arthropod maintenance cycle in nature. Arboviruses replicate in both the vertebrate host and the arthropod vector (mosquitoes, ticks, sandflies, and others), and transmission occurs when the vector takes a blood meal. Typically, arboviruses have only a few vertebrate hosts and are transmitted by a narrow range of arthropods. Humans are not the reservoir vertebrate hosts of most arboviruses, but can be infected by many of these viruses, if they happen to be bitten by an infected vector. In most instances, arbovirus-infected humans are dead-end hosts for several reasons. Many arthropod vectors competent to transmit a zoonotic arbovirus prefer nonhuman hosts as a blood source, reducing the likelihood of transmission from human to vector. Also, infected humans are usually not sufficiently permissive to experience a high titer viremia, so they cannot serve as effective links in the transmission cycle. There are only a few exceptions: in urban settings, dengue, urban yellow fever, Oropouche, and Chikungunya viruses can be maintained by an arthropod vector--human cycle. 2.2. Limited Spread among Humans {#s0045} -------------------------------- As [Table 2](#t0015){ref-type="table"} shows, a few zoonotic viruses can be transmitted directly from human to human, at least for a few passages, and can emerge as the cause of outbreaks involving a few to several hundred cases. Since many viruses in this group cause a high mortality in humans, even a small outbreak constitutes a public health emergency. These viruses belong to many different virus families, and there is no obvious biological clue why they should be able to spread from human to human, in contrast to other closely related viruses. Typically, infections are mainly limited to caregivers or family members who have intimate contact with patients, often in a hospital setting. However, transmission is marginal, so that most outbreaks end after fewer than 5--10 serial transmissions, either spontaneously or due to infection-control practices. 2.3. Crossing the Species Barrier {#s0050} --------------------------------- In the history of modern virology (the last 50 years) there are very few documented instances where zoonotic viruses have established themselves in the human population and emerged as new viral diseases of mankind ([Table 2](#t0015){ref-type="table"}). Most viruses have evolved to optimize their ability to be perpetuated within one or a few host species, and this creates what is sometimes called the "species barrier." In most instances, a virus must undergo some adaptive mutations to become established in a new species. **SARS coronavirus.** In November, 2002, an outbreak of severe acute respiratory disease (SARS) began in Guangdong Province, in southeast China near the Hong Kong border. In retrospect, the first cases were concentrated in food handlers, who then spread the virus to the general population in that region. Although not recognized immediately as a new disease, the outbreak continued to spread both locally and in other parts of China. In February, 2003, a physician who had been treating likely SARS patients, traveled to Hong Kong, where he transmitted SARS to a large number of contacts in a hotel. These persons, in turn, spread the infection to Singapore, Taiwan, Vietnam, and Canada, initiating a global pandemic that eventually involved almost 30 countries. From patient samples, several research groups isolated a novel coronavirus, which has been named the SARS coronavirus (SARS CoV). Clearly, this virus is new to the human population, and there is circumstantial evidence that it was contracted from exotic food animals that are raised for sale in restaurants in Guangdong Province. Recent studies suggest that horseshoe bats (genus *Rhinolophus*) may be the reservoir hosts and palm civets, consumed as food in China, may be the intermediary hosts for SARS CoV. SARS CoV went through a large number of human passages (perhaps 25) before being contained by primary control measures, such as respiratory precautions, isolation, and quarantine. The virus has been eliminated from the human population, but the 2003 outbreak showed that it could be maintained by human-to-human transmission. From that perspective, it is potentially capable of becoming an indigenous virus of humans. Since many coronaviruses infect the respiratory system and are transmitted by the respiratory route, the SARS virus did not have to undergo any change in its pathogenesis. However, the virus did have to replicate efficiently in cells of the human respiratory tract and it is unknown whether this required some adaptive mutations from the virus that is enzootic in its reservoir hosts. **Middle Eastern respiratory syndrome.** MERS is an acute respiratory disease of humans that was first recognized in 2012, when a novel coronavirus (MERS-CoV) was isolated from two fatal human cases in Saudi Arabia and Qatar. Since that time, more than 1400 clinical cases of MERS have been recognized, the great majority in Saudi Arabia but also in most of the other countries in the Arabian Peninsula and beyond ([Figure 3](#f0020){ref-type="fig"} ). Hospitalized cases of MERS are characterized by an acute respiratory disease syndrome (ARDS) with a fatality rate over 25%. However, evolving evidence suggests that there may be many additional human infections with little or no associated illness.Figure 3Distribution of reported cases of MERS, December, 2014.Redrawn from Enserik, M. Mission to MERS. Science 2014, 346: 1218--1220. What is the origin of this new disease? Based on fragmentary data now available, it appears that MERS-CoV is likely to be an enzootic virus of one or more species of bats. Camels are probably an intermediary host, and humans in close contact with camels can acquire infection. Also, MERS-CoV can spread from human to human, particularly to caretakers or others in close contact with acutely ill patients. However, there are many unknowns in this speculative reconstruction: How do camels become infected? Are camels the main source of human infections? What has caused this disease to emerge in 2012, or had it preexisted but was just recognized at that time? Is this an evolving outbreak, and if so, what is driving it? Several relevant facts have been ascertained from basic studies. MERS-CoV replicates well in cell cultures obtained from many species, including bats and humans. The pantropic nature of this virus is explained in part by its cellular receptor, dipeptidyl peptidase 4 (DPPT4), a widely distributed cell surface molecule. This would facilitate the transmission of this zoonotic infection from bats to camels to humans. Of interest, MERS-CoV infects type II alveolar pneumocytes while SARS CoV uses a different cell receptor (angiotensin-converting enzyme 2, ACE2) and infects type I alveolar pneumocytes. However, both viruses appear to cause a similar ARDS. **Type A influenza virus.** Genetic evidence strongly implicates avian and porcine type A influenza viruses as the source of some past pandemics of human influenza. It appears that new epidemic strains are often derived as reassortants between the hemagglutinin (and the neuraminidase in some cases) of avian influenza viruses with other genes of existing human influenza viruses. The new surface proteins provide a novel antigenic signature to which many humans are immunologically naïve. The human influenza virus genes contribute to the ability of the reassortant virus to replicate efficiently in human cells. It is thought that reassortment may take place in pigs that are dually infected with avian and human viruses. Currently, there is concern that a new pandemic strain of Type A influenza could emerge as a derivative of highly virulent avian H5N1 or H7N9 influenza viruses now causing epidemics in domestic chickens in southeast Asia. There have been several hundred documented human infections with each of these avian viruses in recent years---mainly among poultry workers---with significant mortality. However, few if any of these infections have spread from human to human, perhaps because the infecting avian virus has not undergone reassortment with a human influenza virus. A critical determinant is that avian influenza viruses preferentially attach to α2-3 sialic acid receptors while human viruses attach to α2-6 sialic acid receptors. The 1918 pandemic of influenza is presumed to be an example of a zoonotic influenza virus that crossed the species barrier and became established in humans where it caused an excess mortality estimated at 20--40 million persons. Recent viral molecular archaeology has recovered the sequences of the 1918 H1N1 influenza virus from the tissues of patients who died during the epidemic. All of the genes of the reconstructed virus are avian in origin, but it is unknown whether the virus underwent mutations that enhanced its ability to be transmitted within the human population. The reconstructed hemagglutinin of the 1918 virus has been inserted into recombinant influenza viruses, and---in mice---markedly increases the virulence of primary human isolates of influenza virus ([Table 3](#t0020){ref-type="table"} ), but the full virulence phenotype appears to require many of the avian influenza genes. Several physiological factors play a role in disease enhancement, including increased replication in pulmonary tissues and an enhanced ability to stimulate macrophages to secrete pro-inflammatory cytokines which, in turn, cause severe pneumonitis.Table 3Genetic Determinants of the Virulence of the 1918 Type A Influenza Virus (Spanish Strain) Based on Intranasal Infection of Mice with Reassortant Viruses. The M88 Isolate is a Human Type A Influenza Virus Which is Relatively Avirulent in Mice, Typical of Human Isolates. The Hemagglutinin (H) of the 1918 "Spanish" Virus Confers Virulence Upon the M88 Isolate and the Neuraminidase (N) Does Not Appear to Enhance the Effect of the Hemagglutinin. MLD 50: Mouse 50% Lethal Dose Determined by Intranasal Infection with Serial Virus DilutionsVirus StrainOrigin of Viral GenesLog 10 MLD 50Log 10 Virus Titer in Lung (Day 3 after Infection)HNOthersM88M88M88M88\>6.22.9M88/H^sp^Sp (1918)M88M884.45.1M88/H^sp^/N^sp^Sp (1918)Sp (1918)M885.24.7[^2] **Human immunodeficiency virus.** HIV has emerged as the greatest pandemic in the recent history of medical science. Modern methods have made it possible to reconstruct its history in great detail (see Chapter 9, HIV/AIDS). A provisional reconstruction of the sequence of events is summarized in [Figure 4](#f0025){ref-type="fig"} . The emergence of HIV may be divided into two phases: What was the zoonotic source of HIV and when did it cross into humans? And when did HIV spread from the first human cases to become a global plague?Figure 4Speculative reconstruction of events following the transmission of SIVcpz to humans.This reconstruction is based on data in Sharp and Hahn (2011), Pepin (2011). There have been several transmissions of simian immunodeficiency virus (SIV) to humans (Sharp and Hahn, 2011), and this account will focus on HIV-1 which appears to have been transmitted to humans in at least four separate instances, identified by individual HIV-1 lineages called groups (M, N, O, P). Of these, the most important was the M group of HIV-1, which has been responsible for the vast majority of human infections. Furthermore, HIV-1 is most closely related to SIVcpz, the SIV strain infecting two subpopulations of chimpanzees. Different segments of the SIVcpz genome, in turn, are closely related to genome segments of two SIVs of African monkeys, red-capped monkeys and *Cercopithecus* monkeys. It is hypothesized that chimpanzees, which regularly kill and eat monkeys, were infected during consumption of their prey; and that a recombination event produced SIVcpz, which was derived from parts of the genomes of the two acquired monkey viruses. It is speculated that a further transmission from chimpanzees may have occurred during the butchering of nonhuman primates, which occurs in rural Africa ([Figure 5](#f0030){ref-type="fig"} ).Figure 5Bushmeat is part of the diet in rural Africa.Photograph courtesy of Billy Karesh (2015). Amazingly, genomic similarities tentatively map the substrain of SIVcpz that is the ancestor of the M group of HIV-1, to chimpanzees in the southeastern corner of Cameroon, a small country in West Africa. Using a sequence analysis to compare diversity within current isolates, the common parent of the M group can be reconstructed. A molecular clock, derived from dated isolates, indicates that this virus was transmitted to humans during the period 1910--1930. The period from 1930 to 1980 is a mystery (Pepin, 2011), but there are fragmentary data suggesting that the virus persisted as a rare and unrecognized infection in residents of jungle villages in West Africa during this time. It has also been proposed that the reuse of unsterilized needles---a frequent practice during the period of colonial rule---could have inadvertently helped to spread the virus. Starting about 1980, the virus began to spread more rapidly. It appears that accelerated spread began in the region centered on Kinshasa (previously Leopoldville) in the Democratic Republic of the Congo (previously the Belgian Congo, then Zaire) and Brazzaville, just across the Congo River in Congo. Transmission was exacerbated by the chaos in postcolonial Zaire. During the period 1985--2004, HIV infection spread widely in Africa as shown in [Figure 6](#f0035){ref-type="fig"} . In the countries worst affected, the prevalence of infection among adults aged 15--49 years reached levels higher than 30%. The rapid spread was driven by many factors among which were: (1) a high frequency of concurrent sexual contacts in some segments of the population and the hidden nature of sexual networks; (2) the long asymptomatic incubation period during which infected individuals able to transmit the virus were sexually active; (3) the spread along commercial routes of travel within Africa; (4) the failure of health systems to publicize the risks and the underutilization of condoms and other measures to reduce transmission; and (5) the slow introduction of antiviral treatment after it became available in the northern countries about 1996.Figure 6The spread of HIV in Africa, showing the prevalence of HIV in the adult population, 1988--2003. The map ends in 2003, but the prevalence has remained very similar during the period 2004--2015. (After UNAIDS 2004 report on global AIDS epidemic.) Concomitantly with the spread of HIV in Africa, the M group of HIV-1 evolved into nine different subtypes (A--D, F--H, J, K), based on sequence diversity. During the spread within Africa, there were population bottlenecks that resulted in the predominance of different M group subtypes in different regions. Subtype C is most frequent in southern Africa, and subtypes A and D are most frequent in eastern Africa. During the 1980s, HIV also spread globally, although prevalence rates did not reach the levels seen in some African countries. Subtype B is dominant in the western hemisphere and Europe, while subtype C is most frequent in India and some other Asian countries. This implies that each of these regional epidemics was initiated by a small number of founder strains of HIV-1, improbable though that may seem. Thirty years after its appearance as a global disease, almost 40 million persons have died, and there are more than 30 million people living with HIV/AIDS. Although the global incidence of HIV has fallen slightly since 2010, there are still more than two million new infections each year (2014). **Ebola hemorrhagic fever.** The Ebola pandemic of 2014--15 is the most recent emerging virus disease that has riveted the attention of the world. Where did it come from? Why did it cause a pandemic? Why did the international health community fail to control it? Where will it end? These questions are discussed below. Ebola is a filovirus indigenous to Africa that is maintained in one or more reservoir species of wild animals, among which bats are a likely host. The transmission cycle is not well documented but it is thought that humans get infected, either by direct contact with bats, or while slaughtering infected wild animals who may act as intermediate hosts. Human-to-human spread can then occur. The pathogenesis of Ebola virus infection may be briefly summarized. Presumably Ebola enters the human host via the mucous membranes or cuts in the skin. The virus infects mononuclear cells including macrophages and dendritic cells and traffics to lymph nodes, whence it spreads to target organs including the liver, spleen, and adrenal glands. It causes a high titer viremia and a dysregulation of the innate immune system. Clinically, Ebola patients undergo severe vomiting and diarrhea with massive fluid losses and become very dehydrated, with a mortality that varies from 25% to 75%. In fatal cases, the infection of the liver leads to disseminated intravascular coagulopathy, a shock syndrome, and multiorgan failure, although the sequential details are not well understood. Infection is transmitted between humans by contact with bodily fluids of patients, but not by aerosols. Therefore, the virus is spread most frequently to caregivers or others who are in intimate contact with patients and their fomites. Rituals associated with funerals and burial practices often serve to transmit the virus. Ebola virus was first isolated in 1976 in an outbreak near the Ebola River in the Democratic Republic of the Congo (then called Zaire) and almost concurrently in a second outbreak in southern Sudan. Viruses recovered from these two outbreaks were subsequently shown to be different and are now known as Ebola-Zaire and Ebola-Sudan. Since that time there have been more than 25 individual outbreaks of Ebola disease, mainly in central Africa. Past outbreaks have been controlled by use of protective garments by caregivers and quarantine of infected or potentially infected contacts. These controlled outbreaks have been limited to no more than ∼5 serial human-to-human transmissions, and mainly ranged from about 25 to 300 cases. In December, 2013, an Ebola-Zaire outbreak began in Guinea, West Africa. It appears that the initial case was in an infant who may have been infected by contact with bats. The outbreak then spread to two contiguous countries, Liberia and Sierra Leone. By the fall, 2014, the epidemic had become a catastrophe, and was raging out of control in several parts of these three countries. Although the data are incomplete, it is estimated that there have been at least 20,000 cases (with at least 50% mortality) through February, 2015 ([Figure 7](#f0040){ref-type="fig"} ). The infection has spread to Nigeria, Senegal, Mali, the United States, and a few European countries, but these invasions have so far been controlled, with limited secondary cases. A global effort to control this pandemic was initiated, with participation from Doctors without Borders, the Red Cross, other nongovernment organizations, the World Health Organization, and the U.S. Centers for Disease Control and Prevention. As of March, 2015, it appeared that the epidemic was coming under control. Aggressive border screening, both on exit from the affected countries and on arrival at destinations, has limited spread by air travelers, but the porous land borders remain areas of concern.Figure 7The journalistic face of the 2013--2015 Ebola epidemic.Photograph courtesy of Tom Ksiazek, 2014. From an epidemiological viewpoint, why did this outbreak of Ebola explode into a massive pandemic, in contrast to the many prior outbreaks that were limited to no more than a few hundred cases at most? The outbreak began in Guinea and was mainly confined to that country for about 6 months before it spread to neighboring Liberia and Sierra Leone ([Figure 8](#f0045){ref-type="fig"} ). During this first 6 months, incidence in Guinea varied from a few to about 50 cases a week, and cases were concentrated in rural areas. From a public health viewpoint, this represented a missed opportunity to contain the outbreak. Contributing to this omission were a combination of factors: a weak health system fragmented by social disruption, a failure of local health authorities to recognize or respond to the outbreak, the failure of international health organizations such as WHO to take aggressive action, and local societal norms that brought family and friends into close contact with Ebola victims, during their illness and at their funerals (Washington Post, October 5, 2014; Cohen, 2014). Once Ebola infections spread from rural villages to urban centers, the outbreak exploded.Figure 8Ebola pandemic, by country, through April, 2015. After WHO: Ebola situation report, 29 April, 2015. Beginning in the fall of 2014, it was recognized that the pandemic was a global threat. In response, a number of countries and international organizations provided resources to Africa, including building facilities, sending equipment, and recruiting personnel to work in the pandemic areas. A major effort was made to get the local population to temporarily change some of their normal social responses to illness and death, to reduce the spread within the population. Combined with the efforts of the affected countries, these initiatives started to take hold about January, 2015. However, as of March, 2015, the epidemic was not yet terminated. In retrospect, the international community has acknowledged that it lacks a contingency plan to respond to global outbreaks wherever they may occur. Futhermore, because Ebola was a "neglected" disease, the tools to combat it had not been developed. The Ebola pandemic has spurred crash programs to develop a rapid diagnostic test, drugs and antibodies for treatment, and a vaccine for prevention (Product, 2015; Mire et al., 2015). **Canine parvovirus.** CPV is another example of a disease that emerged due to the appearance of a virus new to its host species. In the late 1970s, a highly lethal pandemic disease appeared in the dog populations of the world. The etiologic agent was a parvovirus previously unknown in canines. The sequence of CPV is almost identical to that of feline panleukopenia virus (FPV), an established parvovirus of cats, which causes acutely fatal disease in kittens. CPV has a few point mutations that distinguish it from FPV, and these mutations permit CPV to bind to and infect canine cells, a property not possessed by FPV. It is presumed that these mutations permitted the emergence of a new virus disease of dogs. 2.4. The Species Barrier and Host Defenses {#s0055} ------------------------------------------ Many mammalian viruses have evolved with their hosts so that different members of a virus family are associated with each host species. Furthermore, under natural circumstances, each member of the virus family usually "respects" the species barrier and does not cross into other species, although it spreads readily between individual animals within its host species. Diverse mechanisms contribute to the species barrier, including host defenses and viral genes. For a zoonotic virus to establish itself in humans or another new species, it is probable that mutations are needed for full adaptation. This requirement is likely part of the explanation for the rarity of such events. One of the best-studied examples is the transmission of SIVcpz, a virus of chimpanzees, to HIV, a human virus. Several recent studies have shown that APOBEC3 and tetherin are two very important gate keepers for transmission of lentiviruses between different primate species (reviewed in Sharp and Hahn, 2011). APOBEC3 proteins represent a powerful first line of defense, believed to be responsible for preventing the transmission of SIVs from monkeys to chimpanzees and from monkeys to humans (Etienne et al., 2013). However, APOBEC3 proteins can be counteracted by the HIV/SIV viral infectivity factor (Vif), albeit generally in a species-specific fashion. Thus, mutations in Vif were required for monkey SIVs to be able to infect chimpanzees and then humans (Letko et al., 2013). Tetherin is a second line of defense, and only HIVs that have evolved an effective tetherin antagonism have spread widely in humans (Kluge et al., 2014). Different lentiviruses use different viral proteins to antagonize tetherin: HIV-1 group M uses the viral protein U (Vpu); HIV-2 group A uses the envelope glycoprotein (Env), and HIV-1 group O uses the negative regulatory factor (Nef). In contrast, HIV-1 groups N and P, whose spread in the human population has remained very limited, are unable to counteract tetherin efficiently. Turning to another virus, recent studies using a mouse-adapted strain of Ebola virus to infect a panel of inbred mice provided by the Collaborative Cross (see Chapter 10, Animal models) found striking variation in the response to Ebola virus infection, from complete resistance to severe hemorrhagic fever with 100% mortality. This underlines the role of host genetic background as a determinant of susceptibility. Consistent with this are comments of clinicians that there are unpredictable differences in the outcome of individual Ebola cases. These studies suggest a dynamic relationship between host and pathogen that may determine when a virus can cross the species barrier and create a new virus disease of humankind. 3. Why Viral Diseases Are Emerging at an Increasing Frequency {#s0060} ============================================================= Although difficult to document in a rigorous manner, it does appear that new virus diseases of humans (and perhaps of other species) are emerging at an increased tempo. There are a number of reasons for this trend ([Table 1](#t0010){ref-type="table"}). 3.1. Human Ecology {#s0065} ------------------ The human population is growing inexorably, and is becoming urbanized even faster. As a result, there are an increasing number of large-crowded cities, which provide an optimal setting for the rapid spread of any newly emergent infectious agent. In the nineteenth century, it was noteworthy that someone could circumnavigate the globe in 80 days, but now it can be done in less than 80 h. However, the incubation period of viral infections (several days to several months) has stayed constant. Someone can be infected in one location and---within a single incubation period---arrive at any other site on earth. This enhances the opportunity for a new human virus to spread as a global infection before it has even been recognized, markedly increasing the opportunity for the emergence of a new disease. The same dynamics also apply to viral diseases of animals and plants, which has important economic and social consequences for humankind. The SARS pandemic of 2002--2003, described above, is an example of how rapidly and widely a new virus disease can emerge and spread globally. In this instance, it is extraordinary that the disease was brought under control---and eradicated from the human population---by the simple methods of isolation, quarantine, and respiratory precautions. Although conceptually simple, a heroic effort was required for success. Another example is the 2009 emergence of a novel H1N1 strain of influenza A virus that spread rapidly around the world before a vaccine could be produced. Remote areas of the world are now being colonized at a high frequency, driven by population pressures and economic motives, such as the reclamation of land for agriculture or other uses, and the harvest of valuable trees and exotic animals. The construction of new dams, roads, and other alterations of the natural environment create new ecological niches. It is possible that this is the origin of urban yellow fever. Yellow fever virus is an arbovirus maintained in a monkey--mosquito cycle in the jungles of South America and Africa. Humans who entered jungle areas became infected. When they returned to villages or urban centers, an urban cycle was initiated, where *Aedes aegypti* mosquitoes---that are well adapted to the urban environment and preferentially feed on humans---maintained the virus. In the last 25 years, agriculture has undergone a dramatic evolution with the development of "agribusiness." Food and food animals are now raised on an unprecedented scale and under very artificial conditions, where the proximity of many members of a single plant or animal species permits an infection to spread like wildfire. Furthermore, increasing numbers of plants, animals, and food products are rapidly transported over large distances; we enjoy fresh fruits and vegetables at any time, regardless of the season. International shipment of plants and animals can import viruses into new settings where they may lead to the emergence of unforeseen diseases. One example is the 2003 outbreak of monkeypox that caused about 80 human cases in the United States. This was traced to the importation from Africa of Gambian giant rats as exotic pets; several rodent species in west Africa appear to be reservoir hosts of this poxvirus. Monkeypox spread from these animals to pet prairie dogs and from prairie dogs to their owners. Because monkeypox causes infections in humans that resemble mild cases of smallpox, this outbreak was a major cause of public health concern. 3.2. Deliberate Introduction of a Virus New to a Specific Population {#s0070} -------------------------------------------------------------------- On occasion, a virus has been deliberately introduced into a susceptible population where it caused the emergence of a disease epidemic. For sport, rabbits were imported from Europe into Australia in the mid-nineteenth century. Because of the absence of any natural predator the rabbits multiplied to biblical numbers, and threatened natural grasslands and agricultural crops over extensive areas of southern Australia. To control this problem, myxomatosis virus was deliberately introduced in 1950 (Fenner, 1983). This poxvirus is transmitted mechanically by the bite of insects and is indigenous to wild rabbits in South America, in which it causes nonlethal skin tumors. However, myxomatosis virus causes an acutely lethal infection in European rabbits, and its introduction in Australia resulted in a pandemic in the rabbit population. Following the introduction of myxomatosis virus in 1950, co-evolution of both virus and host were observed. The introduced strain was highly virulent and caused epizootics with very high mortality. However, with the passage of time field isolates exhibited reduced virulence, and there was a selection for rabbits that were genetically somewhat resistant to the virus. Strains of moderate virulence probably became dominant because strains of lowest virulence were less transmissible and strains of maximum virulence killed rabbits very quickly. Concern has also been raised about disease emergence due to the deliberate introduction of viruses into either human or animal populations, as acts of bioterrorism. 3.3. Xenotransplantation {#s0075} ------------------------ Because of the shortage of human organs for transplantation recipients, there is considerable research on the use of other species---particularly pigs---as organ donors. This has raised the question whether known or unknown latent or persistent viruses in donor organs might be transmitted to transplant recipients. Since transplant recipients are immunosuppressed to reduce graft rejection, they could be particularly susceptible to infection with viruses from the donor species. In the worst scenario, this could enable a foreign virus to cross the species barrier and become established as a new human virus that might spread from the graft recipient to other persons. 4.. How Are Emergent Viruses Identified? {#s0080} ======================================== The impetus to identify a new pathogenic virus usually arises under one of two circumstances. First, a disease outbreak that cannot be attributed to a known pathogen may set off a race to identify a potentially new infectious agent. Identification of the causal agent will aid in the control of the disease and in prevention or preparedness for potential future epidemics. SARS coronavirus, West Nile virus, and Sin Nombre Virus are examples of emergent viruses that were identified in the wake of outbreaks, using both classical and modern methods. Alternatively, an important new virus may be discovered as a serendipitous by-product of research directed to a different goal, as was the case with hepatitis B virus (HBV). In this instance, a search for alloantigens uncovered a new serum protein that turned out to be the surface antigen (HBsAg) of HBV, leading to the discovery of the virus. When a disease outbreak cannot be attributed to a known pathogen, and where classical virus isolation, propagation, and identification fail, molecular virology is required. Hepatitis C virus (HCV), Sin Nombre and other hantaviruses, certain rotaviruses, and Kaposi's sarcoma herpesvirus (HHV8), are examples of emergent viruses that were first discovered as a result of molecular technologies. Below, we briefly describe some methods of viral detection and identification. More detailed information and technical specifics can be found in several current texts. 4.1. Classic Methods of Virus Discovery {#s0085} --------------------------------------- The first question that confronts the investigator faced with a disease of unknown etiology is whether or not it has an infectious etiology? Evidence that suggests an infectious etiology is an acute onset and short duration, clinical similarity to known infectious diseases, a grouping of similar illnesses in time and place, and a history of transmission between individuals presenting with the same clinical picture. For chronic illnesses, the infectious etiology may be much less apparent and a subject for debate. Faced with a disease that appears to be infectious, the next question is whether it is caused by a virus. A classical example that predates modern virology is the etiology of yellow fever. In a set of experiments that would now be prohibited as unethical, the Yellow Fever Commission, working with the US soldiers and other volunteers in Cuba in 1900, found that the blood of a patient with acute disease could transmit the infection to another person by intravenous injection. Furthermore, it was shown that the infectious agent could pass through a bacteria-retaining filter and therefore could be considered a "filterable virus." **Virus isolation in cell culture and animals.** The first step in identification of a putative virus is to establish a system in which the agent can be propagated. Before the days of cell culture, experimental animals were used for this purpose. Many viruses could be isolated by intracerebral injection of suckling mice, and some viruses that did not infect mice could be transmitted to other experimental animals. Human polioviruses---because of their cellular receptor requirements---were restricted to old world monkeys and great apes; the virus was first isolated in 1908 by intracerebral injection of monkeys and was maintained by monkey-to-monkey passage until 1949 when it was shown to replicate in primary cultures of human fibroblasts. The modern era of virology (beginning about 1950) can be dated to the introduction of cultured cells as the standard method for the isolation, propagation, and quantification of viruses. There are now a vast range of cell culture lines that can be used for the isolation of viruses, and currently this is the first recourse in attempting to isolate a suspected novel virus. Some viruses will replicate in a wide variety of cells but others are more fastidious and it can be hard to predict which cells will support their replication. It is also important to recognize that some viruses will replicate in cell culture without exhibiting a cytopathic effect. An important example is the identification of simian virus 40 (SV40). Poliovirus was usually grown in primary cell cultures obtained from the kidneys of rhesus monkeys, but SV40 had escaped detection because it replicated without causing a cytopathic effect. When poliovirus harvests were tested in similar cultures prepared from African green monkeys, a cytopathic effect (vacuolation) was observed, leading to the discovery of SV40 virus in 1960. Because inactivated poliovirus vaccine produced from 1955 to 1960 had been prepared from virus grown in rhesus monkey cultures, many lots were contaminated with this previously unknown virus, which inadvertently had been administered to humans. Since that time, viral stocks and cell cultures have been screened to exclude SV40 and other potential virus contaminants. A number of methods are available to detect a noncytopathic virus that is growing in cell culture. These include visualization of the virus by electron microscopy, detection of viral antigens by immunological methods such as immunofluorescence or immunocytochemistry, the agglutination of erythrocytes of various animal species by virus bound on the cell surface (hemagglutination), the production of interferon or viral interference, and the detection of viral nucleic acids. **Detection of nonreplicating viruses.** During the period from 1950 to 1980, there was a concerted effort to identify the causes of acute infections of infants and children. In seeking the etiology of diarrheal diseases of infants, it was hypothesized that---in addition to bacteria, which accounted for less than half of the cases---one or more viruses might be responsible for some cases of infantile diarrhea. Numerous unsuccessful attempts were made to grow viruses from stools of patients with acute diarrhea. It was conjectured that it might be possible to visualize a putative fastidious virus by electron microscopy of concentrated fecal specimens. When patients' convalescent serum was added to filtered and concentrated stool specimens, aggregates of 70 nm virions were observed in stools from some infants with acute gastroenteritis. The ability of convalescent but not acute illness serum to mediate virion aggregation provided a temporal association of the immune response with an acute diarrheal illness. Within 5 years, rotavirus was recognized as the most common cause of diarrhea in infants and young children worldwide, accounting for approximately one-third of cases of severe diarrhea requiring hospitalization. Once an emergent virus has been identified, it is necessary to classify it, in order to determine whether it is a known virus, a new member of a recognized virus group, or represents a novel virus taxon. This information provides clues relevant to diagnosis, prognosis, therapy, and prevention. In 1967, an outbreak of acute hemorrhagic fever occurred in laboratory workers in Marburg, Germany, who were harvesting kidneys from African green monkeys (*Chlorocebus aethiops*, formerly *Cercopithecus aethiops*). In addition, the disease spread to hospital contacts of the index cases, with a total of over 30 cases and 25% mortality. Clinical and epidemiological observations immediately suggested a transmissible agent, but attempts to culture bacteria were unsuccessful. However, the agent was readily passed to guinea pigs which died with an acute illness that resembled hemorrhagic fever. After considerable effort, the agent was adapted to tissue culture and shown to be an RNA virus. When concentrated tissue culture harvests were examined by electron microscopy, it was immediately recognized that this agent differed from known families of RNA viruses, since the virions consisted of very long cylindrical filaments about 70 nm in diameter. This was the discovery of Marburg virus, the first recognized member of the filoviruses, which now include Marburg and Ebola viruses. 4.2. The Henle--Koch Postulates {#s0090} ------------------------------- Isolation of a virus from patients suffering from an emergent disease provides an association, but not proof of a causal relationship. Formal demonstration that an isolated virus is the causal agent involves several criteria formulated over the past 100 years. These are often called the Henle--Koch postulates, after two nineteenth-century scientists who first attempted to enunciate the rules of evidence. [Sidebar 1](#b0010){ref-type="boxed-text"} summarizes these postulates, which have been modernized in view of current knowledge and experimental methods.Sidebar 1The Henle--Koch postulates (requirements to identify the causal agent of a specific disease)The Henle--Koch postulates were formulated in 1840 by Henle, revised by Koch in 1890, and have undergone periodic updates to incorporate technical advances and the identification of fastidious agents with insidious disease pathogenesis.Many of the following criteria should be met to establish a causal relationship between an infectious agent and a disease syndrome.1.The putative causal agent should be isolated from patients with the disease; or the genome or other evidence of the causal agent should be found in patients' tissues or excreta; and less frequently from appropriate comparison subjects. Temporally, the disease should follow exposure to the putative agent; if incubation periods can be documented they may exhibit a log-normal distribution.2.If an immune response to the putative agent can be measured, this response should correlate in time with the occurrence of the disease. Subjects with evidence of immunity may be less susceptible than naïve individuals.3.Experimental reproduction of the disease should occur in higher incidence in animals or humans appropriately exposed to the putative cause than in those not so exposed. Alternatively, a similar infectious agent may cause an analogous disease in experimental animals.4.Elimination or modification of the putative cause should decrease the incidence of the disease. If immunization or therapy is available, they should decrease or eliminate the disease.5.The data should fit an internally consistent pattern that supports a causal association. The classic version of the Henle--Koch postulates required that the causal agent be grown in culture. However, as discussed below, a number of viruses that cannot be grown in culture have been convincingly associated with a specific disease. Usually, this requires that many of the following criteria can be met: (1) Viral sequences can be found in the diseased tissue in many patients, and are absent in appropriate control subjects; (2) Comparison of acute and convalescent sera document induction of an immune response specific for the putative causal virus; (3) The disease occurs in persons who lack a preexisting immune response to the putative virus, but not in those who are immune; (4) The implicated virus or a homologous virus causes a similar disease in experimental animals; and (5) Epidemiological patterns of disease and infection are consistent with a causal relationship. 4.3. Methods for Detection of Viruses that Are Difficult to Grow in Cell Culture {#s0095} -------------------------------------------------------------------------------- Some very important human diseases---such as hepatitis B and hepatitis C---are caused by viruses that cannot readily be grown in cell culture. Experiences with these viruses have given credibility to the view that an infectious etiology can be inferred by clinical and epidemiological observations in the absence of a method for growing the causal agent. Also, they have stimulated researchers to devise novel techniques that bypass the requirement for replication in cell culture. Furthermore, the application of molecular biology, beginning about 1970, has led to an array of new methods---such as the polymerase chain reaction (PCR), deep sequencing, and genomic databases---that can be applied to the search for unknown viruses. Several case histories illustrate the inferences that lead to the hypothesis of a viral etiology, the strategy used to identify the putative causal agent, and the methods exploited by ingenious and tenacious researchers. **Sin Nombre virus.** Hantavirus pulmonary syndrome was described above, as an example of an emerging virus disease. The disease was first reported in mid-May, 1993, and tissues and blood samples from these cases were tested extensively, but no virus was initially isolated in cell culture. However, when sera from recovered cases were tested, they were found to cross-react with a battery of antigens from known hantaviruses, providing the first lead (in June, 1993). DNA primers were then designed, based on conserved hantavirus sequences, and these were used in a PCR applied to DNA transcribed from RNA isolated from tissues of fatal cases. Sequence of the resulting amplicon suggested that it was a fragment of a putative new hantavirus (July, 1993), yielding a presumptive identification of the emerging virus within 2 months after the report of the outbreak. An intense effort by three research teams led to the successful isolation of several strains of SNV by November, 1993. SNV is a fastidious virus that replicates in Vero E6 cells but not in many other cell lines. **Kaposi's sarcoma herpesvirus (HHV8).** KS was described over 100 years ago as a relatively uncommon sarcoma of the skin in older men in eastern Europe and the Mediterranean region. In the 1980s, KS emerged at much higher frequency, as one of the diseases associated with AIDS. Furthermore, KS exhibited an enigmatic epidemiological pattern, since its incidence in gay men was more than 10-fold greater than in other AIDS patients, such as injecting drug users and blood recipients. These observations led to the hypothesis that KS was caused by a previously undetected infectious agent that was more prevalent among gay men than among other HIV risk groups. However, researchers were unable to isolate a virus from KS tissues. Searching for footprints of such a putative agent, Chang and colleagues used the method of representational difference analysis to identify DNA sequences specific for KS tumor tissue. Several DNA fragments were identified, and found to be homologous with sequences in known human and primate herpesviruses. In turn, these sequences were used to design primers to obtain the complete genome of a previously undescribed herpesvirus, since named HHV8, human herpesvirus 8. To this date, HHV8 defies cultivation in tissue culture. 4.4. Computer Modeling of Emerging Infections {#s0100} --------------------------------------------- Is computer modeling a useful adjunct to the analysis or control of emerging viral diseases? The 2014--15 Ebola pandemic in West Africa offers an interesting case study. As the epidemic unfolded, several groups attempted to project how it would evolve (Meltzer et al., 2014; Butler, 2014). These projections had very wide confidence limits, and several of them had upper limits in the range of 100,000 or more cases. What the modelers could not foretell was that the infection did not spread across sub-Saharan Africa, and that several introductions (into countries such as Nigeria and Mali) were controlled by case isolation, contact tracing, and quarantine. However, modeling did contribute useful insights. Dobson (2014) suggested that rapid quarantine (within 5--7 days) of contacts of Ebola patients could be critical in epidemic control. 5. Reprise {#s0105} ========== One of the most exciting current issues in virology is the emergence of new viral diseases of humans, animals, and plants. Even though the era of modern virology has been well established for more than 65 years, virus diseases continue to appear or reemerge. The Ebola pandemic of 2014--15 highlights the associated dangers and obstacles to control. There are several explanations for emergence: (1) discovery of the cause of a recognized disease; (2) increase in disease due to changes in host susceptibility or in virus virulence; (3) reintroduction of a virus that has disappeared from a specific population; (4) crossing the barrier into a new species previously uninfected. Many zoonotic viruses that are maintained in a nonhuman species can infect humans, but most cause dead-end infections that are not transmitted between humans. A few zoonotic viruses can be transmitted between humans but most fade out after a few person-to-person transmissions. Rarely, as in the case of HIV, SARS coronavirus, and Ebola filovirus, a zoonotic virus becomes established in humans, causing a disease that is truly new to the human species. There are many reasons for the apparent increase in the frequency of emergence of new virus diseases, most of which can be traced to human intervention in global ecosystems. Emergent viruses are identified using both classical methods of virology and newer genome-based technologies. Once a candidate virus has been identified, a causal relationship to a disease requires several lines of evidence that have been encoded in the Henle--Koch postulates, guidelines that are periodically updated as the science of virology evolves. Identifying, analyzing, and controlling emerging viruses involve many aspects of virological science. Virus--host interactions play a key role, to explain persistence in zoonotic reservoirs, transmission across the species barrier, and establishment in human hosts. Thus, the issues discussed in many other chapters contribute to our understanding of emerging viral diseases. [^1]: Ebola in West Africa involved unlimited human-to-human transmission for over one year (see following). [^2]: After Kobasa D, Takada A, Shinya K, et al. Enhanced Virulence of Influenza a Viruses with the Haemagglutinin of the 1918 Pandemic Virus. *Nature*, 2004, 431: 703--707, with Permission
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1. Field of Invention. This invention relates to anchors, and in particular, to those anchors provided with pivotally mounted flukes and with a release mechanism to facilitate its unmooring. 2. Description of the Prior Art. An anchor moors a vessel to the sea bed, generally by a combination of its own weight and by hooking itself into the bottom. See The Illustrated Science and Invention Encyclopedia, H. S. Stuttman Co., Inc., Publishers, N.Y., Vol. 1, page 110. An ideal anchor is designed so that a near horizontal pull causes it to dig itself in firmly, but an upward pull dislodges it easily. It is attached to the vessel by a cable--this is a heavy chain on large ships. Anchors in use today provide a more or less firm mooring but require winching in the cable and running the vessel over the anchor's position for its unmooring. When the cable is more or less vertical the anchor should dislodge. However, it does not always dislodge easily. Sometimes, an underwater utility cable or mangrove root gets caught between the flukes and pulling the anchor out is just an exercise in futility. One of the most popular anchors, the Danforth anchor, is particularly susceptible to this problem.
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Living with diabetes blog Diabetes: Balancing your insulin, medication and exercise Controlling diabetes is a balancing act. You must carefully balance food, activity (exercise), and medications and insulin. All three are equally important to your health, and each can increase or decrease your blood glucose levels. Many of our readers ask if they need to adjust their insulin or medication before exercise. Physical activity, or exercise, includes anything that gets you moving, such as walking, dancing or working in your garden. Staying active improves your overall health. Regular exercise helps you: Better control glucose levels Increase overall fitness Feel more energetic Improve flexibility Improve blood pressure Lower your risk of developing cardiovascular disease Improve your appearance, weight and overall sense of well-being Insulin and diabetes medications lower your blood glucose. The amount of medication you need is unique to you. The time of day you take your medication and how much you take are important factors in allowing your medication to work when your blood glucose rises. As you make exercise a part of your life, your diabetes health care provider may change or adjust your medications based on the results recorded in your diabetes record book. It's a balancing act — if you eat more than your meal plan allows, your blood glucose level may rise, or, if you exercise less than usual, your blood glucose level may rise. Several factors affect your blood glucose during activity or exercise: Your physical condition Length of activity or exercise Type of activity or exercise Blood glucose level prior to exercising When you're more active than usual, your blood glucose may drop too low, causing low blood glucose (hypoglycemia). It's important that you prepare ahead of time. If you're taking insulin and you know ahead of time when you will exercise, decrease your rapid or short insulin meal dose before the activity instead of taking extra food during the activity. Talk with your diabetes health care team for help making the decision about how much to decrease your insulin dose. Also, avoid injecting insulin into your arms and legs that you will use during your activity or exercise. An abdominal injection site may help lower the risk for hypoglycemia associated with exercise. Some additional tips: Test your blood glucose before, during and after the activity to monitor how it affects your blood glucose level. This is important when beginning or changing your exercise program. When your insulin is peaking, exercise isn't recommended, as it may lead to low blood glucose. Before you exercise, take less insulin or eat more food at mealtime or as a snack. If your blood glucose is less than 70 mg/dL (3.8 mmol/L), take 1 to 2 carbohydrate choices and make sure your blood glucose is in goal range before you begin the activity or exercise. If you were in goal range before the activity and the activity drops your blood glucose more than 30 to 50 mg/dL (1.6 to 2.7 mmol/L) or hypoglycemia occurs — blood glucose less than 70 mg/dL (3.8 mmol/L) — stop exercising and take 1 carbohydrate choice. Recheck your blood glucose after 15 minutes and repeat until your blood sugar returns to a safe range. Then, return to your exercise and take 1 carbohydrate every 30 to 60 minutes while you're active. Don't exercise if your blood glucose is greater than 300 mg/dL (16 mmol/L). Exercising with blood glucoses over 300 mg/dL (16 mmol/L) can raise your blood glucose even more, because exercise causes the body to release or produce extra glucose and there won't be enough insulin available to use it. With harder or more strenuous activity, even if you're within goal range or above goal, 2 carbohydrate choices may be necessary to prevent low blood glucose. Ask your health care provider if you have questions about this. For longer duration or very strenuous activities, such as downhill/cross country skiing or long bike rides, take 1 carbohydrate choice every 30 to 60 minutes during the activity. Check your blood glucose every 1 to 2 hours during the activity. It isn't recommended that you be active or exercise when you're sick. We generally don't recommend exercising before bed due to the risk of delayed post-exercise hypoglycemia. If evening exercise is necessary, consider eating an extra carbohydrate after exercise to reduce the risk of hypoglycemia while sleeping. Remember, it's essential to check with your health care provider if you've been sedentary and want to begin an exercise routine. Didn't answer my question. I am a thin individual with type 2 diabetes, caused by a whipple surgery. If my blood sugar is 94 before breakfast and I take the prescribed amount of insulin (4 units) and then exercise within I/2 hour after breakfast, my blood levels will drop drastically after the exercise. Should I eat more carbs and take less insulin, wait about an hour and then exercise? Mark Swartz November 9, 2016 1:42 p.m. This information was so helpful thank Esther November 8, 2016 5:27 p.m. Please talk about high blood sugars. I struggle with them daily even with an insulin pump. Victoria November 8, 2016 11:34 a.m. Great info. Stavros September 9, 2016 11:37 p.m. Thanks for the great content. you have helped me fill knowledge gaps. Thanks Melissa Tower March 11, 2016 12:51 p.m. Very helpful. I'm 69 years old and a type1 diabetic since age 19. We bike, kayak and/or walk everyday. What make it difficult to maintain proper levels, is not the activity, but what that activity may entail. For example, we went kayaking and needed to carry two kayaks 100 yards to reach the water and then back to the car after 2 hours in the water. That was too much and blood sugar level dropped dangerously low. Yes I had my moniter and plenty of snacks but not for that activity. Energy conservation is also very important. Get the details about any activity and skip those that may zap you before you begin. Conserve energy and use it to have fun!! Frank M March 18, 2015 5:03 a.m. good article. useful joseph kirema March 17, 2015 4:00 p.m. Thank you Peggy, I have been type 1 diabetic for47 years. I agree with what you have said. And you said it very well. I am passing this onto my husband to read, so he better understands. Ann Ann Pownall March 17, 2015 1:53 p.m. Exercise is like medication. This is where it gets complicated for people on insulin or on other medications that can produce hypoglycemia. While it is true that regular exercise helps you better control glucose levels, lows before the insulin doses are adjusted can assert themselves after just a few days of regular exercise. This is where you recommend that “your diabetes health care provider may change or adjust your medications based on the results recorded in your diabetes record book.” From experience, I can say that it is hard to anticipate which night this will happen--and it always seems to be at night when it happens--unless you anticipate needing less insulin before you actually experience a low. Recall also that most physicians are not available to review a record book at the drop of a hat. There has to be something that can tip a patient off before having to risk whether the low will wake them up. Any ideas? Barbara March 17, 2015 12:09 p.m. Is there a certain amount of glucose in the bloodstream that causes problems Linda bonebrake March 17, 2015 11:45 a.m. Balancing exercise with insulin injections is truly a challenge that can cause a great deal of anxiety. The fact is that it is not a normal way to live, but what choice does one have? One must stay active as possible and try to manage the ups and downs of blood sugar fluctuations. Perhaps one day, easier methods of blood sugar monitoring will be made possible and other methods of regulating glucose levels will help people with this condition live an easier life. Better yet, perhaps, one day, diabetes will be eradicated. George November 13, 2013 9:50 p.m. I think the hard part is getting to admit you have it and that as young as you are people of all ages and fitness levels get. Its a mental nightmare at first. Lean on friends and family.You are not alone! With care,diet,meds,exercise,and patience. LIFE WILL BE GOOD! Rocky September 29, 2013 8:34 a.m. You read a lot about exercise and insulin, but I often wonder what adjustments should a DM non-insulin dependent should make prior to exercising? Plus, what are good source of 1 or 2 carbohydrates intake? Minnie September 22, 2013 2:57 p.m. must disagree with your advice about not exercising before bed. in my opinion their should never be any type of discouragement to exercising. benefits from any exercise far outweighs possible side effects. of course you can find extreme situations where their are adverse affects but for the 99.9% who will benefit their should be overwhelming encouragement. i credit exercising (and diet) with going from a a1c of 12 to an a1c of 5.5 without any medication.i'm not any kind of fitness freak at still over 275 lbs. i have been able to swim(very slow pace) and walk. just an average american who let their weight get away but through peoples encouragement to exercise even a little when i could good things have been happening for over a year. Legal Conditions and Terms Reprint Permissions A single copy of these materials may be reprinted for noncommercial personal use only. "Mayo," "Mayo Clinic," "MayoClinic.org," "Mayo Clinic Healthy Living," and the triple-shield Mayo Clinic logo are trademarks of Mayo Foundation for Medical Education and Research.
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It is believed that examples of known fuel injection systems use an injector to dispense a quantity of fuel that is to be combusted in an internal combustion engine. It is also believed that the quantity of fuel that is dispensed is varied in accordance with a number of engine parameters such as engine speed, engine load, engine emissions, etc. It is believed that examples of known electronic fuel injection systems monitor at least one of the engine parameters and electrically operate the injector to dispense the fuel. It is believed that examples of known injectors use electromagnetic coils, piezoelectric elements, or magnetostrictive materials to actuate a valve. It is believed that examples of known valves for injectors include a closure member that is movable with respect to a seat. Fuel flow through the injector it believed to be prohibited when the closure member sealingly contacts the seat, and fuel flow through the injector is believed to be permitted when the closure member is separated from the seat. It is believed that examples of known injectors include a spring providing a force biasing the closure member toward the seat. It is also believed that this biasing force is adjustable in order to set the dynamic properties of the closure member movement with respect the seat. It is further believed that examples of known injectors include a filter for separating particles from the fuel flow, and include a seal at a connection of the injector to a fuel source. It is believed that such examples of the known injectors have a number of disadvantages. It is believed that examples of known injectors must be assembled entirely in an environment that is substantially free of contaminants. It is also believed that examples of known injectors can only be tested after final assembly has been completed.
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Until recently, empirical testing of the impact of development projects was extremely weak, and controversial. Most research on the impact of development projects suffered from severe methodological problems: almost none of the available empirical studies appropriately addressed problems related to self-selection bias and/or programme placement bias. Fortunately, in the last few years, we have seen several new empirical analyses using rigorous methodologies. These new analyses are often based on so-called randomized controlled trials. In a randomized controlled trial the impact of development projects is studied by randomly assigning different households to treatment and control groups. In this course we will discuss important aspects of experimental design in the context of development projects. Special attention will be given to microfinance projects. The aim is to provide a better understanding of the theory and practice of field experiments in developing countries. Students will learn how to design randomized experiments, quasi-experiments and so-called lab-in-the-field games. We will also explain how to analyse the data and interpret the findings.
3.453125
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Glaucoma Surgery What is Glaucoma? Glaucoma is a disease that damages the eye’s optic nerve. It can cause blindness if left untreated, though only about half of the estimated three million Americans who have glaucoma know they are affected. Glaucoma generally produces few early symptoms and the disease progresses slowly. Overview While glaucoma is often treated with medicated eye drops, sometimes surgery becomes necessary. We perform selective laser trabeculoplasty (SLT), a procedure that uses a low-level energy laser to target specific cells in the trabecular meshwork, the eye’s drainage channels. This stimulates the eye’s draining function, easing the buildup of pressure from fluid. What to Expect Glaucoma surgery is an outpatient procedure that generally requires one follow-up exam. The doctor will put eye drops in the eyes before or after the procedure to decrease fluid and prevent elevation in pressure. A special microscope and lens will guide the laser beam to the canals where fluid drains. The doctor will then make small burns in the trabecular meshwork. While discomfort is usually minimal, some people will feel a heat sensation in the eye. Complications are rare, but the most common one is an increase in eye pressure. The pressure may be normal after surgery, but it can rise sharply within one to four hours. This can be prevented by using apraclonidine or brimonidine before or after surgery, especially in people with high intraocular pressure. Other complications may include: Inflammation of the colored part of the eye Clouding of the cornea Blockage of the draining angle Pain Decreased vision How to Prepare No preparation is necessary, though mild discomfort may exist temporarily after the procedure.
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Beatrice Black BearThe World's Wettest Dam Photographer by John Grandits, illustrated by Brian Floca Image: There is a picture of a bear, with a camera, standing at the base of a large dam and gesturing towards the top. Bear says, “I'm taking pictures at Lake Powell in Arizona. That huge wall is a dam built across the Colorado River. It holds back the water to create the lake. “Dams do a lot of work. They help make electricity, and people use lake water for drinking and farming.” Image: There is a picture of a bear with swimming goggles, and overlays of a person sailboarding, and of three children playing in the water. Bear says, “But when the work is done, it's time for fun! The lake is great for sailboarding… or swimming with your friends.” Image: There is picture of a bear water skiing in a human pyramid. The women on the bear's shoulders have started to fall. Bear says, “Water skiing is the best, but it's not as easy as it looks!” Activity What did building a dam across the Colorado River do to the river?[anno: It held back part of the river and made a lake.] Why is there a dam across the Colorado River?[anno: The dam helps make electricity. The lake provides people with fresh water for drinking and farming.] What would it be like to visit a dam? Write a sentence or two to tell what it might be like to visit a dam. What would you see and hear? If you have visited a dam, write about what it was like.[anno: Answers will vary. Students may write about seeing a lot of water and hearing a rush of water when the dam is opened.]
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Fauna of Louisiana The fauna of the State of Louisiana is characterized by the region’s low swamplands, bayous, creeks, woodlands, coastal marshlands and beaches, and barrier islands covering an estimated 20,000 square miles (counting for 40 percent of Louisiana's total land area). Southern Louisiana contains up to fifty percent of the wetlands found in the Continental United States, and are made up of countless bayous and creeks. The Creole State has a humid subtropical climate, perhaps the best example of a humid subtropical climate of all the Southern United States with long, humid and hot summers and short, mild winters. The subtropical characteristics of the state are due in large part to the influence of the Gulf of Mexico, which at its farthest point is no more than 200 miles away. Louisiana's varied habitats — tidal marshes, bayous, swamps, woodlands, islands, forests, and prairies — offer a diversity of wildlife. Some of the most common animals found throughout all of the parishes include otter, deer, mink, muskrat, raccoons, opossums, rabbits, squirrels, nutria, turtles, alligators, woodcocks, skunks, foxes, beavers, civet cats, armadillos, coyotes and bobcats. Deer, squirrel, rabbit, and bear are hunted as game, while muskrat, snakes, nutria, mink, opossum, bobcat, and skunk are commercially significant for fur. Prized game birds include quail, turkey, woodcock, and various waterfowl, of which the mottled duck and wood duck are native. There are several endemic plants and animals in Louisiana that are found nowhere else on Earth; an example could be the Louisiana bluestar or the white leucistic alligator. The Pearl river map turtle and the Ringed map turtle are only found in Louisiana and neighboring State of Mississippi. Louisiana contains a number of areas which are, in varying degrees, protected from human intervention. In addition to National Park Service sites and areas and the Kisatchie National Forest, Louisiana operates a system of state parks, state historic sites, one state preservation area, one state forest, and many Wildlife Management Areas. The Nature Conservancy also owns and manages a set of natural areas. State ecology Much of the state's lands were formed from sediment washed down the Mississippi River, leaving enormous deltas and vast areas of coastal marsh and swamp. The northern parts of Louisiana mostly consist of woodlands which are home to deer, squirrels, rabbits, bears, muskrats, mink, opossums, bobcats, and skunks. Louisiana's forests offer a mix of oak, pine, beech, black walnut, and cypress trees. In the Piney Woods in the Ark-La-Tex-region, Mammals such as the North American cougar, gray fox, feral hogs (razorback), and snakes such as the western cottonmouth, the western worm snake, the Louisiana pine snake, as well as other animals are common. Louisiana’s largest forest, the Kisatchie National Forest in the forested hills of Central Louisiana, has 155 species of breeding birds, 48 mammal species, 56 reptile species and 30 amphibian species. It is some 600,000 acres in area, more than half of which is vital flatwoods vegetation, which supports many rare plant and animal species. These include for instance the Louisiana pine snake, the red-cockaded woodpecker, the Louisiana black bear and the Louisiana pearlshell. Alligators are common in Louisiana's extensive swamps, bogs, creeks, lakes, rivers, wetlands, and bayous. Other water-loving reptiles such as the alligator snapping turtle live in the Louisiana swamps. The alligator snapping turtle is characterized by a very large head and three rows of spiked scutes. These wetlands of Louisiana make ideal homes for several species of turtles, crawfish and catfish - all of which are popular Acadian foods. Jambalaya, a Louisiana Creole dish that originated among the Cajuns in Acadiana, is made entirely by all sorts of meat found in the swampland of southern Louisiana: crawfish, herons, shellfish, catfish, toads, frogs, shrimp, oysters, alligator, duck, turtle, boar, venison, and myriad other species. Among invasive species that thrive in the wetlands of Louisiana is the nutria, a South American rodent that was likely introduced when individual animals escaped from fur farms. Mammals Forty species of mammals reside in Louisiana, excluding marine mammals. Seventy mammal species have been recorded in Louisiana or its immediate adjacent waters. Louisiana has for instance two species of squirrels: gray squirrels and fox squirrels, according to the Louisiana Department of Wildlife and Fisheries. Louisiana has two species of rabbits: eastern cottontails and swamp rabbits. Although the cottontail is considered more of an upland species and the swamp rabbit a wetland species, both species occur throughout the state. Rabbits have high productive rates in Louisiana when habitat and weather conditions are good. Louisiana black bear The Louisiana black bear once ranged throughout the State of Louisiana and parts of adjacent neighboring Mississippi, Arkansas, and Texas. The black bear was common at the time of early colonization, serving as food for Native Americans for generations. An 1890 record shows 17 parishes containing bears, all of them by the Mississippi-border and the Atchafalaya region. It was reported that the most extensive areas of bottomland hardwoods in the state have “at least a few bears”, with the greatest number found in the denser woodlands along the Tensas, Red, Black, and Atchafalaya Rivers. In the late 1950s, bears occupied habitat in the Tensas-Madison area in northeast Louisiana and in the lower fringes of the Atchafalaya Basin. Today, black bears can be found in all of Louisiana, but according to the Louisiana Department of Wildlife and Fisheries, most black bears are observed in a confined region made up of the following parishes: West- and East Carroll, Richland, Franklin, Madison, Tensas, Catahoula, Concordia, Avoyelles, Pointe Coupee, St. Landry, Vermilion, Iberia, as well as both St. Martin and St. Mary. Black bear could be legally hunted in parts of Louisiana through the late 1980s. One of the last organized bear hunts in Louisiana occurred December 15, 1955. During this hunt, five bears were harvested in the Lake Providence area. It was recommended to the Wildlife Commission that the bear season be closed. Bear hunting was closed the following season and remained closed until 1961. The season was opened again from 1962-1965 with hunting permitted only in northeast Louisiana and in the coastal parishes. The hunting season was again closed from 1966 to 1974. It was reopened in 1975-1987 with hunting restricted to the Atchafalaya Basin. The Louisiana bear hunting season has remained closed since 1988. From 1964 through 1967, 161 black bears were live-trapped in Cook County, Minnesota and released in the Mississippi and Atchafalaya River bottoms of Louisiana in an effort to restock black bear to the state. By 1968 there was evidence that the translocated bears were reproducing. However, most of the relocated bears were killed on roads, as nuisance animals, or during recapture. As of 2016, Louisiana black bears are no longer endangered. Reptiles The American alligator is the official state reptile of Louisiana. Perhaps the most iconic of Louisiana wetlands' animals, the American alligator has bounced back from near extinction to being relatively commonplace. An abundance of snake species make their home in Louisiana, including the eastern diamondback rattlesnake, Texas coral snake, eastern yellowbelly racer, mud snake, western pigmy rattlesnake, northern scarlet snake, rainbow snake, buttermilk racer, tan racer, western cottonmouth, red cornsnake, pit vipers and kingsnake. America's largest freshwater turtle, the alligator snapping turtle, shares the habitat with its cousin, the common snapping turtle. The green American chameleon also lives in the wetlands, along with the lizard-like tiger salamander, which is an amphibian. Other examples of reptiles in Louisiana are the gopher tortoise, razor-backed musk turtle, broad-headed skink, coal skink and the slender glass lizard. According to the Louisiana Alligator Council, there are over one million alligators in the state in 2014 and the number is continuously increasing. Alligators like swamps, rivers, lakes or wherever they can have an adequate habitat. Louisiana has several varieties of venomous snakes. The eastern coral snake, Texas coral snake, copperhead, western cottonmouth, western pygmy rattlesnake, and the eastern diamondback rattlesnake and canebrake rattlesnake can all be found in Louisiana. The largest reported American alligator was a male killed in 1890 on Marsh Island in Louisiana, and reportedly measured at . Birds Approximately 160 species of birds are year-round residents or probable confirmed breeders in Louisiana and another 244 are known to regularly migrate through or winter in the state or its immediate adjacent waters. There are 69 species on the CWCS species of conservation concern list of which 42 species are considered critically threatened, imperiled or rare, according to the Louisiana Natural Heritage Program. Shorebirds and songbirds constitute the majority of species. In 1902, the eastern brown pelican was made a part of the Seal of Louisiana and, ten years later, in 1912, the pelican and her young adorned the flag of Louisiana as well. The official nickname of Louisiana is the Pelican State. In 1958, the pelican was made the official state bird of Louisiana. This act was amended on July 26, 1966 to specifically designate the brown pelican, the National Basketball Association's New Orleans Pelicans are named in honor of Louisiana's state bird. The eastern brown pelican is also the national bird of Barbados and the Turks and Caicos Islands, it is also one of the mascots of Tulane University and is on the seals of Tulane University, Louisiana State University and the University of Louisiana at Lafayette. Shore birds are abundant in Louisiana and the most common is the great white egret. This large, all-white heron has an impressive wingspan and stature. The egret occurs often in the wetlands of Louisiana and coastal areas that provides it with plenty of fish, amphibians and small mammals to feast on. This bird is also the official symbol of the National Audubon Society. The American bald eagle nests in southeastern coastal parishes and, occasionally on large lakes in northern and central parishes, but these nests are less successful. Some of America's tallest birds, such as the great blue heron and great egret, cannot resist the fishing opportunities that exist in the Louisiana swampland. Raptors such as the osprey, American black vulture and barred owl live in the marshes of southern Louisiana. Migratory waterfowl and songbirds often make stopovers or actually spend the winter in these wetlands. Amphibians The American green tree frog was designated the official state amphibian of Louisiana in 1993. Examples of other amphibians in Louisiana are salamanders such as the eastern tiger salamander, southern red-backed salamander, Gulf Coast waterdog, dwarf salamander and the three-toed amphiuma. There are also toads such as Hurter's spadefoot toad and southern toad, as well as frogs such as pig frog, striped chorus frog and the bronze frog. American bullfrogs are the largest frogs native to Louisiana. Fish The white perch, sometimes called sac au lait from Cajun French, was designated the official state fish of Louisiana in 1993. Coastal beaches are inhabited by sea turtles, and whales are often seen from offshore. Freshwater fish include bass, crappie, and bream. Red and white crawfishes are the leading commercial crustaceans. Many sharks have been observed in Louisiana waters; including, but not limited to lemon sharks, tiger sharks, bull sharks and blacktip sharks. The sharks, for instance the bull shark, have often been observed throughout the Atchafalaya Basin, 900 miles up the Mississippi River, and in inland bayous and wetlands. The alligator gar and the frecklebelly madtom, which is native to Pearl River in Southeastern Louisiana, are two additional species of fish in Louisiana. The bowfin, known by many other names such as the mudfish, dogfish, grinnel, grindel, jack, jackfish, cypress trout, cotton fish, and in South Louisiana; choupique (pronounced shoe-pick or shoe-peg), or chew-pic, is found in many areas of Louisiana. Endangered species Threatened animal species include five species of sea turtles: green, hawksbill, Kemp's ridley, leatherback, and loggerhead). Twenty-three Louisiana animal species were on the U.S. Fish and Wildlife Service's threatened and endangered species list for 2003. Among those listed are the Louisiana black bear, American bald eagle, Inflated heelsplitter, and red-cockaded woodpecker. The Louisiana WAP identifies 240 species of concern. The mountain lion population in Louisiana is small but growing in recent times. There is a relatively small and threatened population of Louisiana black bears. The historic range of the Florida panther extended from Florida to Louisiana throughout the Gulf Coast states and Arkansas. Today, the only place with wild Florida panthers is the southwestern tip of Florida. The Florida panther is considered of historical occurrence in Louisiana. The historic range included as far west as Western Louisiana and the East Lower Mississippi River Valley through the southeastern states. Even though numerous sighting reports continue to surface annually throughout its historic range, it is unlikely that viable populations of the Florida panther presently occur outside of the State of Florida. The Louisiana Black Bear has been taken off the endangered species list. Mississippi diamondback terrapin is recognized as a “species of concern” in Louisiana, but is found on the Mississippi-border. Invasive species Coypu Tabasco tycoon and naturalist Edward McIlhenny brought thirteen adult coypu from Argentina to his home in New Iberia, during the 1930s, for the fur farming industry. Two years later, one hundred and fifty got out of the pen, supposedly escaping during a storm. The nutria reproduced at a high rate, increasing by the thousands every year. By the 1960s the number ranged to as high as twenty million, and increasing. By the time the government instituted a control program, the coypu was destroying Louisiana marshes and wetlands, causing widespread erosion. In the 21st century, the coypu is one of the most common and despised pests in the Bayou State. The story of the nutria is not unique. Many species of birds, mammals, fish, and plants have been introduced into the Louisiana environment in the past two centuries. Exotic species, or species that have been introduced to areas outside their native range, take heavy tolls on the ecosystems they colonize. Some invaders, such as the leafy vine kudzu (Pueria lobelia), destroy the habitat for resident wildlife. Other species fiercely compete with native plants and animals for resources. By some estimates, exotic species pose the second most serious threat to endangered species after habitat loss. Nutria were introduced into coastal marshes from Latin America in the mid-1900s, and their population has since exploded into the millions. They cause serious damage to coastal marshes and may dig burrows in levees. Hence, Louisiana has had a bounty to try to reduce nutria numbers. Large alligators feed heavily on nutria, so alligators may not only control nutria populations in Louisiana, but also prevent them spreading east into Florida and possibly the Everglades. Since hunting and trapping preferentially take the large alligators that are the most important in eating nutria, some changes in harvesting may be needed to capitalize on their ability to control nutria. Monk parakeet An agricultural pest in its native South American range, the monk parakeet was first brought to the U.S. as a cage bird. They were so popular that over 60,000 were imported between 1969 and 1972. By the 1980s it had already been released in many parts of the country and had established small breeding colonies. Twenty years later, monk parakeet numbers have increased exponentially but their distribution remains spotty. Monk parakeets tend to be restricted to urban areas where they feed and nest in ornamental palm trees, occupying a niche that no indigenous bird holds. So far, their distribution in Louisiana has been limited almost exclusively to the City of New Orleans, where they have had no adverse effects on local wildlife. If their numbers increase, however, monk parakeets could pose a serious threat to agricultural areas, possibly becoming as much of a pest here as they already are in their native range. Red Fire Ant Because of its tropical climate and its proximity to Mexico and Central America, Louisiana is able to support many invasive species that cannot survive elsewhere in the U.S. One such example is the red fire ant. Native to South America, the red fire ant has flourished in many southern U.S. states since its introduction in the 1930s. Superficially similar to most other ants, the fire ant is a vicious predator, attacking birds, rodents, and larger mammals in swarms. One study of white-tailed deer found that death rates for young deer were twice as high in areas with fire ants as in uninfested areas. In Louisiana, the spread of fire ants has been linked to the decline of the loggerhead shrike and some species of warblers. The red fire ant has replaced nearly half the native insect species in some areas it has colonised. See also Fauna of the United States References F01 .L
3.5
4
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Red River system The Red River system is a network of rivers surrounding the main river - Red River in North Vietnam. These branches of the system contribute to or receive water from Red River. Red River system, joining with the Thái Bình river system in the northeast, creates the Red River Delta - the second largest delta in Vietnam. Because of the close relation between Red River system and Thái Bình river system, the two system are known as the common name Red and Thai Binh rivers system. Alluvium of the Red River system creates the central and south Red River Delta. Two banks of the rivers are protected by a great dyke system. Rivers of the system Main river: Red River Confluences: Da River Lô River Besides that, confluences of another river - River Đáy, a river starts from mountainous area of Hòa Bình and Ninh Bình provinces, including Bôi river, Hoàng Long river, Vạc river although not contribute water to Red River, but for several reasons, they are still considered as Red River confluences. Branches: River Đáy and its branches Nhuệ River Đuống River Phủ Lý River (or Châu Giang River) Luoc River linking Red River with Thái Bình River Trà Lý River, flowing eastward through Thái Bình Province Diêm Hộ River Ninh Cơ River flowing southward through Nam Định Province Nam Định River So River Lân River River mouth Ba Lat, main river mouth, located in the border between Thái Bình provinces and Nam Định provinces Diêm Hộ, Trà Lý, Lân (Thái Bình Province) So, Lach Giang (Nam Định Province) Đáy, located in the border between Ninh Bình and Nam Định provinces. Category:Geography of Vietnam
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Queletia Queletia is a genus of fungi in the family Agaricaceae. The genus was described by Elias Magnus Fries in 1872. Fruit bodies of Queletia species are roughly spherical with a stipe-like base. They have a thin outer skin (peridium) and a harder inner skin that breaks into small pieces with age. The genus is named after French mycologist Lucien Quélet. See also List of Agaricales genera List of Agaricaceae genera References Category:Agaricaceae Category:Agaricales genera
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There has been a great deal of interest in recent years in the use of bio-oxidation to recover metals from sulfide ores. In such ores, the sulfides trap, or occlude, the metal particles within sulfide minerals, such as iron pyrite for example. The bio-oxidation techniques use natural microorganisms to catalyze the oxidation of sulfides in the ore into soluble sulfates, in order to adequately expose the metal in the ore for subsequent extraction. Typical metals which may be recovered in this way include gold, silver, copper, zinc, nickel or cobalt. In recent years, the gold industry has shown a particular interest in the use of bio-oxidation techniques for the recovery of gold, in large part because of the high value of gold. The primary goal of the gold mining industry is cost-effective recovery of gold from ore, and the most commonly used techniques for gold recovery from ore are smelting and cyanidation. However, a great deal of ore is to be found in ore which is naturally resistant to conventional recovery techniques. Such ore is called “refractory,” and usually contains gold particles which are locked, or occluded, within sulfide minerals. To obtain adequate gold recovery from such refractory ore, the ore must first be subjected to a pre-treatment process in which the sulfide minerals are degraded by oxidation. The ore may then be treated by a traditional reagent such as cyanide to dissolve the gold, in order to recover the gold from the treated ore. Such bio-oxidation techniques are particularly useful for pre-treatment of mine tailings, which are the byproducts of mining operations. Not only does this allow gold extraction from highly refractory ores, but it provides the added benefit of removing a barrier to redevelopment and a potential environmental hazard. Bio-oxidation is particularly well suited to the pre-treatment of tailings, as the low gold concentrations found in such tailings are not a problem for the microorganisms involved. The microorganisms simply ignore the waste products in the ore, and proceed to oxidize the sulfides surrounding the gold, often resulting in ultimate extraction recoveries not achievable by other methods One method of bio-oxidation used to pre-treat sulfide-refractory gold ores is heap bio-oxidation, which is described in U.S. Pat. No. 5,246,486 to Brierley et al. In this method, coarsely ground (P80>¼″)1 refractory ores are first agglomerated while being inoculated with a microorganism slurry, then heaped onto a leach pad with aeration and drain lines. This is referred to as a “free-drained” system; i.e., one in which there is no water table within the bed, no part of the bed is flooded, and the water leaves the system drained by gravity. Initially the inoculum is grown in a tank, but after the heap oxidation process matures, the solution draining from the heap contains the organisms and is used as the inoculum. The bio-oxidation continues until the predetermined target level of sulfide oxidation has been achieved. The ongoing sulfide oxidation levels are determined by the analysis of sulfate concentration in the bioreactor effluent solution and the bioreactor effluent cumulative mass flow. Once the bio-oxidation is complete, the ore is removed from the pad and lime is added to neutralize the ore. This makes the microorganisms in the ore become dormant, and also conditions the bio-oxidized ore for cyanide leaching to extract the gold. 1“P80” is a commonly used abbreviation in the mining industry, and means that 80% of the ore particles are finer than the specified size—in this case, ¼ inch. Heap bio-oxidation can permit ultimate gold recoveries in the range of 60-70% from refractory ore. In addition, it uses inexpensive pond liners and allows air addition via high-volume blowers, which are relatively efficient and low-cost. However, heap bio-oxidation suffers from certain inefficiencies, primarily due to the large particle sizes, typically with a P80 of approximately ½ inch and no finer than a P80 of ¼ inch, with −150 [Tyler] mesh2 (106 microns) fines totaling less than 10% by weight of the total ore (expressed in the industry as P80=¼″, <10% −150 mesh). This large particle size causes “channeling,” in which water and solution seek large gaps between particles, and thus tend to flow by the ore without making substantial contact. To counter this channeling effect, a relatively high solution application rate is utilized in order to maintain contact with the ore. However, such high solution application rates result in a relatively thick layer of solution around each ore particle which impedes air flow through the heap, so that the oxidation rate is significantly slowed. 2A minus sign in front of a size designator, such as mesh or microns, followed by a percentage, is a standard abbreviation used in the mining industry to indicate that the specified percentage of the ore particles are finer than the specified size. In this case, the abbreviation is used to signify that less than 10% of the particles are smaller than 150 mesh (106 microns). Further, it has long been known that the more finely ground an ore, the more efficiently it may be oxidized and the higher the ultimate gold recoveries would be in the subsequent gold recovery process. This is because as a given quantity of ore is ground into smaller particles, the overall surface area of that quantity of ore is increased. Since an increased surface area increases the contact with the oxidizing solutions, the oxidation proceeds at a faster rate, and is also more complete. However, a great deal of experience with heap leach gold cyanidation led to the conclusion that particle sizes less than P80=¼ inch tended to migrate through the heap, until ultimately they bind together into a clay-like mass, thereby “plugging” the flow of both solution and air through the heap. Since such plugging would render the heap bio-oxidation extremely inefficient, no use of particle sizes smaller than P 80=¼ inch has traditionally been attempted. Unfortunately, this perceived inability of heap bio-oxidation to utilize smaller particle sizes has greatly limited the efficiency and thoroughness of the oxidation achievable with the process. Notably, the typical 60-70% overall gold recovery could potentially be significantly higher if the oxidation were more thorough. In addition, the time for completing the heap bio-oxidation process is typically in the range of 180-360 days, thereby adding substantially to the heap bio-oxidation capital and operating costs. This heap retention time could also potentially be greatly reduced, if smaller particles could be accommodated by the heap bio-oxidation process. One attempted solution to the above-mentioned problems with heap bio-oxidation has been agitated tank bio-oxidation. Agitated tank bio-oxidation is an alternative to heap bio-oxidation which allows for the utilization of much smaller particles (<100 microns). In this process, large quantities of oxygen and carbon dioxide are dissolved into a finely ground slurry of ore. Plugging problems which might otherwise be associated with such fine particles are avoided by utilizing a mechanically agitated tank to house the process. While such tanks are an effective way to allow very fine particles to be used in the process, they are highly expensive to purchase and to operate, and thus add greatly to the cost of the oxidation. Air addition into the agitated tank is also expensive and difficult to achieve, as the air must be added as extremely fine bubbles, and under sufficient pressure to overcome the pressure associated with the solution depth of the flooded tank. In addition to being costly, the air addition and the tank agitation render the whole process much more complex than traditional heap bio-oxidation. Ultimately, agitated tank bio-oxidation typically results in an accelerated retention time of 5-8 days, with an overall ultimate gold recovery of 85-90%. There is thus a need for a pre-treatment bio-oxidation process for refractory gold ore which would allow significantly smaller particle distributions to be utilized, thereby greatly improving overall gold recovery and shortening bio-oxidation retention times. Ideally, the process would utilize a free-drained system, and thus would avoid the cost and complexity of agitated tank bio-oxidation.
3.125
3
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Q: C - Counting number of same elements in 2 arrays Let's say we have 2 arrays: char arr1[1024]="ABDDDABAC"; char arr2[1024]="DDDABKDDJABAJJ"; and would like to determine the position at which arr2 has the maximum number of matching elements as arr1. For example if arr1[0] is compared to arr2[2], it would result in 5 matches as the code shows below. int matches=0; for (int i=0;i<strlen(arr2);i++){ if (arr1[i+2]==arr2[i]){ matches++; } } printf("matches: %d\n", matches); The code above returns the number of matches when arr1 is shifted by 2 indices, but does not calculate the number of matches at every single possible shift, and returns the shift which results in the maximum number of matching elements. A: the comparisons in for (int i=0;i<strlen(arr2);i++){ if (arr1[i+2]==arr2[i]){ matches++; } } only considers (in an expensive way) the length of arr2, there is no protection concerning arr1 and you can go out of it with an undefined behavior If you want to find the max number of matches you just have to iterate on the possible offsets in arr1 and save the best case, for instance : #include <stdio.h> #include <string.h> int main() { const char * arr1 = "ABDDDABAC"; const char * arr2 = "DDDABKDDJABAJJ"; size_t max = 0; const char * pmax; size_t ln1 = strlen(arr1); size_t ln2 = strlen(arr2); for (const char * a1 = arr1; *a1 ; ++a1) { size_t mx = 0; const char * p1 = a1; const char * p2 = arr2; while (*p1 && *p2) { if (*p1++ == *p2++) mx += 1; } printf("%d matches at offset %d\n",mx, a1 - arr1); if (mx > max) { max = mx; pmax = a1; if (mx == ln2) /* useless to continue, cannot be better */ break; } if (--ln1 < max) /* useless to continue, cannot be better */ break; } if (max == 0) puts("no match"); else printf("max matches %d at offset %d\n", max, pmax - arr1); } Compilation and execution : pi@raspberrypi:/tmp $ gcc -g -pedantic -Wextra -Wall m.c pi@raspberrypi:/tmp $ ./a.out 1 matches at offset 0 2 matches at offset 1 5 matches at offset 2 2 matches at offset 3 2 matches at offset 4 max matches 5 at offset 2 Execution under valgrind pi@raspberrypi:/tmp $ valgrind ./a.out ==10912== Memcheck, a memory error detector ==10912== Copyright (C) 2002-2017, and GNU GPL'd, by Julian Seward et al. ==10912== Using Valgrind-3.13.0 and LibVEX; rerun with -h for copyright info ==10912== Command: ./a.out ==10912== 1 matches at offset 0 2 matches at offset 1 5 matches at offset 2 2 matches at offset 3 2 matches at offset 4 max matches 5 at offset 2 ==10912== ==10912== HEAP SUMMARY: ==10912== in use at exit: 0 bytes in 0 blocks ==10912== total heap usage: 1 allocs, 1 frees, 1,024 bytes allocated ==10912== ==10912== All heap blocks were freed -- no leaks are possible ==10912== ==10912== For counts of detected and suppressed errors, rerun with: -v ==10912== ERROR SUMMARY: 0 errors from 0 contexts (suppressed: 6 from 3) Note : the code makes no supposition concerning the size of the arrays, this is why it contains if (--ln1 < max) ... which is never true with the used strings, so arr1 and arr2 can be argv[1] and argv[2] rather than hard coded if you want all the number of matches remove all the code concerning ln1 and ln2
3.078125
3
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Cancer is a major public health problem. It accounts for approximately one quarter of all deaths in the United States, and is the leading cause of death among men and women under 85 years of age. The lifetime probability of developing cancer is 46% for men and 38% for women. Many anti-cancer therapies are plagued by side effects including nausea, emesis, hair loss, fever, and risk of infection. Chemotherapy and radiotherapy both lead to high rates of oral and gastrointestinal (GI) mucositis in treated patients, and these effects can be the dose-limiting toxicities of some treatment modalities. Tumor cells acquire a high level of adaptive heat shock response. The heat shock response is an adaptive mechanism used by all living cellular organisms to survive under the conditions of so-called proteotoxic stress—the condition resulting in accumulation of misfolded proteins, which tend to aggregate leading to cell death due to global protein denaturing triggered by such aggregation. Cells can activate this protective mechanism by inducing synthesis of additional protein chaperones, known as heat shock proteins (HSP). Tumor cell viability may be dependent on heat shock response because they have higher rate of protein misfolding. However, the efficacy of thermotherapy techniques for cancer are limited by the induction of adaptive heat shock response, which can greatly diminish tumor cell sensitivity to treatment and limit the use of thermotherapy and other heat shock modulating treatments. Accordingly, there is a need for improved methods of inducing cell death.
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What is NFC Technology? Before digging into the details about how to use NFC in Android, it is useful to describe a bit about NFC technology. Near Field Technology (NFC) is a technology that enables short-range communication between two compatible devices that support this technology. NFC requires that one device behaves as the transmitter and the other one as a receiver. NFC enabled devices can be grouped in two categories: Active Passive Active NFC devices are capable of sending and receiving data and can exchange data with a passive device. Passive devices can send data to other NFC-enabled devices without a power source. A typical passive device is NFC tag that can be used as advertising system for example. NFC technology is available on the newest Android smartphones and NFC tags are used to active advertising, smart payment etc. It is important than to know how to write NFC tags in Android. Getting Started Using NFC The first thing an NFC-enabled Android app should do is verifying if the NFC is present and if it is active: Just to recall if you have not read the getting started with NFC tutorial, it is necessary to register the android app so that it receives notification when the Android device is near the NFC tag. To enable this notification we have to use NFC foreground dispatch: How To Write A NFC Tag In Android Now the Android app is ready to handle the NFC tag and when the Android smartphone gets near the NFC tag, the event is notified to the app. The next step is writing the data on the tag. The method is quite simple: This method accepts an abstract representation of the NFC tag we want to write and the NdefMessage containing the message to write. As the first step, the NFCManager class tries to get the Ndef tag (line 4). If the tag is null, the app tries to "format" the tag and the write the message. If the tag is already formatted, the Android app tries to connect to the tag abstract representation and write the NdefMessage. Write URL Into NFC Tag With Android App Now it is known how to write data into NFC tag, it is time to start writing some simple information. The code is very simple, using NdefRecord provided by Android NFC API, the Android app creates a Uri record. As we already know, a NdefMessage is an array of record, so we create an NFC Ndef Message holding only one record: the Uri record.In this case, type holds HTTP value because it is a link. If we want to write an NFC tag that holds a phone number so that when the user taps with the smartphone the tag a phone call is triggered, we have to pass as type tel:. Write Text Data Into NFC Tag The last example is writing text data in an NFC tag. In this case following NFC specs the code is very simple: Implementing The Android UI For NFC App The last step is implementing the UI so that the Android app handles different NFC record type and the user can insert the data to write. The app uses a spinner that holds the different record types and an EditText that holds the data to write and finally a button (a Floating Action Button) to start the operation. As soon as the user clicks on the button the app starts waiting for the NFC tag. When the user taps on the tag, the app starts writing the data.
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Politicians, the media, and the public express concern that immigrants depress wages by competing with native workers, but 30 years of empirical research provide little supporting evidence to this claim. Most studies for industrialized countries have found no effect on wages, on average, and only modest effects on wage differentials between more and less educated immigrant and native workers. Native workers’ wages have been insulated by differences in skills, adjustments in local demand and technology, production expansion, and specialization of native workers as immigration rises. While the literature reports a range of wage effects of immigration, most estimates are small and, on average, essentially zero. Recent evidence shows that immigration is likely to boost firm productivity and the wages of native workers in the long run by stimulating firm growth and contributing a range of skills and ideas. More open immigration policies, which allow for balanced entry of immigrants of different education and skill levels, are likely to have no adverse effects on native workers’ wages and may pave the way for productivity growth. The recent empirical literature emphasizes that to understand the impact of immigrant workers on wages, immigration and the response of firms and workers must be analyzed together. This literature focuses on how firms and local economies respond to immigrant inflows by expanding, investing, adjusting product specialization, adopting efficient technologies, and creating new businesses. A review of the literature finds little evidence of a wage-depressing effect of immigration because immigrants are absorbed into the receiving economy through a series of adjustments by firms and other workers. Once these adjustments are accounted for, the wages of native workers, even workers with skills similar to those of immigrants, do not change much in response to immigration. Many people hold the belief that immigrants “take jobs” from the native labor force in industrial countries; that they crowd out job opportunities; and that they depress wages (see Figure 1 ). This fear is often manifested in stringent immigration restrictions, especially on immigrants with little education. Such measures are defended as necessary to protect native workers. But this view is rooted in a simplified, static model of labor demand and supply in which immigration increases the supply of some workers while everything else in the economy remains fixed. An overview of the estimated wage impact of immigrants Many studies in recent decades have analyzed the effect of immigration on the wages of native workers, assessing the magnitude and direction of the impact. These studies have used both cross-sectional data and panel (cross-sectional plus longitudinal) evidence of immigration flows into regions, countries, occupation groups, and skill groups in countries that have received large inflows of immigrants, such as Canada, Germany, Spain, the UK, and the US. About a third of these studies used US data. The others used data mainly for Austria, Germany, Israel, and the UK, whilst a few used data for other European countries. Most of the studies used labor market statistics as a control. The more recent studies, which used mainly panel data analysis, included labor market and year fixed effects. Several studies, especially those based on regional variation, used econometric “instrumental variables” to separate the exogenous, supply-driven variation in immigrants from variations correlated with demand shocks, to identify the causal effect of a supply-driven change in immigrants on native wages. This paper summarizes that abundant literature, based on a review of 27 original studies published between 1982 and 2013. Most of the reviewed studies were published, and some have been quite influential. Together, the 27 studies produced more than 270 baseline estimates of the effects of an increase in the share of immigrants on the wages of natives in the same labor market. The message that emerges from these studies is illustrated in Figure 2, which shows the distribution of the average estimated wage effect for each of the 27 studies, ranging from –0.8 to +0.8, in bins of length equal to 0.1. The histogram would look very similar if it showed all the estimates from the 27 studies rather than an average for each study. Additionally, a meta-analysis of 18 studies conducted between 1982 and 2003 showed a very similar histogram, centered on 0 and populated mostly with very small estimates between –0.1 and +0.1 [1]. The values report the effects of a 1 percentage point increase in the share of immigrants in a labor market (whether a city, state, country, or a skill group within one of these areas) on the average wage of native workers in the same market. For example, an estimated effect of 0.1 means that a 1 percentage point increase in immigrants in a labor market raises the average wage paid to native workers in that labor market by 0.1 percentage point. These studies used a variety of reduced-form estimation and structural estimation methods; all the estimates were converted into the elasticity described here. While there are important qualifications to each method and a degree of imprecision in each study (some discussed below), one clear finding emerges: the largest concentration of estimated effects is clustered around zero. Furthermore, the effects are often economically very small and at least half are not statistically significant. While the full range of estimates is between –0.7 and +0.7, two-thirds of them (19 out of 27) are between –0.1 and 0.1, equally distributed over positive and negative values. The average estimated coefficient is 0.008. Applying the average value of the estimates to total immigration in the US between 1990 and 2010, a time when the share of foreign-born workers rose from 9% to 16%, would imply an impact of immigrants on the average wage of native workers of 0.056 of a percentage point (7% times 0.008), or an increase of roughly one-twentieth of a percentage point. These are extremely small changes, especially over a 20-year period, and do not support the notion that immigrants lower the wages of native workers. Two other general findings emerge from the literature. First, while some of the surveyed studies find a more significant negative effect on the wages of less educated native workers than native workers overall, most do not. The meta-analysis study does not identify any significant difference in estimated wage effects between less educated native workers and all native workers [1]. This is understandable. In many countries, immigrants are concentrated in the highly educated group or evenly distributed across skill groups, so there is no reason to believe that they will hurt the wages of less educated workers more than others. In several large immigrant-receiving economies (such as Canada, Sweden, and the UK), the college-educated group makes up the largest concentration of immigrants relative to native workers in the same group. Even in the US, where some of the estimated effects on the wages of less educated native workers are negative, this holds true only for the 1990s, a particularly low-skill-intensive time; during the period 2000–2010, net immigration was high-skill-intensive. Second, the wage effects of recent immigrants are usually negative and slightly larger for earlier immigrants than for native workers. New immigrants may be stronger labor market competitors of earlier immigrants than of native workers. Do native workers attenuate the wage effects of immigrant labor by moving? Researchers have sought to identify the mechanisms that allow immigrant-receiving economies to absorb immigrants without lowering the wages of their native workers. Since many studies have analyzed local labor markets (cities, regions, states), one proposed mechanism was the “skating-rink” model: as immigrants moved into a local economy, native workers with similar skills moved out, leaving total employment and the skill composition unchanged. In the canonical labor supply and demand model, this adjustment mechanism would weaken any detectable effect on native wages. Immigrants might still displace native workers by pushing them out of the market, but the wage effect would not be detectable in the local economy. Most studies find no empirical evidence that native workers move out in response to immigration [2]. With the exception of particularly rigid labor markets (discussed below), local economies, firms, and native workers do respond to immigration and eliminate potential adverse wage impacts, but not by moving out of the region or by becoming unemployed. Examining the effects of immigrants on wages in national labor markets and by skill Due to the fact that analyses of local labor markets might miss wage effects that diffuse beyond the local market, several recent studies have analyzed the effects over time of immigrants in national labor markets segmented by skill (usually education-age groups). Changes in the supply of one skill in a national labor market, such as an inflow of college-educated immigrants, are assumed to affect the wages of workers in that skill group. Using data for the US over the period 1960–2000, one study estimated a negative effect of –0.76 of an increased share of immigrants in one skill group on the wages of native workers in the same skill group [3]. This is the largest negative estimated effect of immigrants on native wages in any of the reviewed studies (it is the negative outlier at the left edge of the histogram in Figure 1, with a value of –0.76). What explains such a large, negative estimate, and how can it be reconciled with the much smaller and sometimes positive effects found in most of the literature? Partial versus total effects: Skill complementarities and firm investments The more recent literature using national data by skill group has emphasized the importance of three mechanisms for correctly estimating the effects of immigration on wages. Specifically these are: immigration has cross-skill effects (complementarity) that must be considered; firms respond to the increased supply of immigrant workers by adjusting capital; and immigration has potentially important overall productivity effects. Taking these adjustment mechanisms into account would therefore attenuate the negative effects estimated in the US study [3]. The first effect can be explained by the fact that different jobs are connected within a firm’s production process. Having more immigrants in one skill group (for example, engineers) allows firms to expand job opportunities (complementarities) for workers in other skill groups (for example, sales representatives and janitors). Accounting for these cross-skill effects substantially reduces the negative wage impact of immigrants, while failing to account for them isolates a partial effect of immigration without considering the total effect. The second effect is related to the first. An increase in available workers means that existing firms can grow, investing in new plant and equipment, and that new firms may start up. Unless the immigrant influx is sudden and unexpected, this mechanism operates continuously and allows the local economy to expand and absorb additional immigrant labor without lowering wages. Incorporating these two effects into the analysis requires some assumptions to be made about the extent of cross-skill complementarity and about how fast firms adjust investment. Recent studies that apply this model to the US and the UK, using a reasonable set of assumptions, find very small effects on the wages of native workers, including the less educated ones [4]. The estimates concerning the increase in US immigrants between 1990 and 2006 imply a negative effect of less than 1 percentage point for the wages of native workers with no diploma in response to a small positive effect for native workers with a high school education, and ultimately a zero effect for native workers with a college education. Productivity effects A third effect overlooked in the earlier analyses of national labor markets by skill group is the effect of immigration on productivity. In the long run, immigrants can increase the overall efficiency of the economy by bringing new skills, stimulating efficient specialization, and encouraging firm creation. In the long run this can have an important effect on wages, because productivity drives all wage growth. There is evidence of this positive effect in recent analyses at the city [4], [5], state [6], region [7], [8], and national levels. This effect has, however, been hard to identify and is often neglected. In particular, studies based on the canonical model of the labor market and the national skill-group approach ignore the possibility of an overall productivity effect and focus only on the narrow competition or complementarity effects within and between skill groups. Some studies do not explicitly consider this potential effect but simply absorb it into a fixed term [3], [9]. Moving beyond the canonical model of the labor market: Alternative mechanisms offsetting wage effects Understanding how immigrants create positive productivity effects requires moving beyond the canonical model of labor supply and demand. That model assumes that immigration is simply a shift of the labor supply for a given labor demand and given labor supply of native workers. It also assumes that native and immigrant workers of similar skills perform identical tasks, that firms do not respond to immigration (at least in the short term), and that native workers do not change occupations or specializations. More likely, as evidenced by several recent studies, immigrants bring different skills and perform different tasks than native workers [2], [4], [6]. Native workers also respond to immigration by specializing in more communication and cognitive-intensive production tasks, which complement the tasks performed by immigrants. This is important because skill diversity among workers facing a wide array of differentiated tasks increases specialization and efficiency. Skill diversity may also spur innovation and productivity growth. Firms may also expand in response to an increase in immigrant workers and create new complementary jobs filled largely by native workers. If any of these mechanisms lead to an increase in overall productivity, a canonical model applied at the national level would be unlikely to capture these effects of immigration [3], [9]. Most studies that explicitly consider these possibilities find positive, sometimes large, productivity effects of increased numbers of immigrant workers. When the impact of these mechanisms on wages is also accounted for, it seems clear that these mechanisms could offset competition effects, producing the overall nil or positive effects observed in the 27 broad studies of immigration and native wages. Recently, scholars have explored other adjustment mechanisms not included in the canonical model that might offset the negative competition effects of an increase in immigrant workers. One is the choice of appropriate firm technology. When the supply of certain skills rises in the local labor market, firms tend to choose technologies that use those skills efficiently. For example, an immigration-induced increase in the supply of less educated manual workers in some US cities has pushed firms to adopt more manual-intensive technologies in place of more mechanized technologies. This has resulted in keeping the productivity and wages of that skill group relatively high. Similarly, the larger number of foreign scientists and engineers in some US cities encouraged firms to adopt technologies that increased the productivity of native workers with these specialties. Another mechanism protecting wages and boosting the productivity of native workers is the occupational upgrading that occurs when the share of immigrant workers rises. When immigrants fill lower-skill, manual-intensive positions, native workers move into more complex, cognitive- and communication-intensive jobs [2], [10]. Similarly, when highly educated immigrants enter the labor market and take analytically intensive positions in science and technology, highly educated native workers move into managerial occupations. Finally, a large share of immigrants with specific skills are absorbed by new firms that spring up to take advantage of the availability and skills of new immigrants (for a more comprehensive overview see Why immigrants may not depress natives' wages).
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COMPUTER TODAY A computer is an electric device that is used to perform repetitive calculations at very high speed. The computer acts as a data processing device and also stores large amounts of data. This data could be text, pictures, voice, numbers, photographs and other types of information that are used by humans in their day-to-day operations. Life cannot be imagined without computers. In fact, the new millennium is the era of computers and its associated techniques, commonly known as Information Technology (IT). Computers help the school children learn new techniques of study, graphic designs, games and other useful educational applications. They help the college students in preparing reports. They help the office executives in accounts, software development, sale invoicing and manufacturing. They help the libraries in the efficient management of their operations. They run the factories and equipment. They control the satellites and nuclear weapons. They help the young and the old through the Internet sites. They are, in fact, indispensable as every operation of human life is incomplete and inefficient without them. As school-going students, we must learn computers. Computers are available in various configurations. For learning computer operations a computer with 166 MHz speed (Known as the CUP speed), a HDD of 1.2 MB storage capacity... read more
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Opioid Addiction Resources Opioids can be abused. Addiction refers to a problematic or unhealthy use of a substance. The harms from abusing opioids can range from mild to severe. Tolerance and addiction are not the same. Tolerance is when an individual requires more of a medication to get the same result as their body has become used to it. Tolerance happens with many differnet types of medications, not just opioids. 4 people found this helpful Print Share Save Addiction can be explained using the 4 C. Craving. An individual craves the use of the drug. This is not the same as wanting to reduce their pain level. Control. A individual loses control over the amount and frequency of use. They are not able to take a prescription as prescribed and would consistency run out of pills early. Compulsion. An individual has a compulsion to use the drug. This would be using the mediation even if there were no pain or no breakthrough pain. Consequences. An individual continues to use the medication despite the consequences of use. So, they continue to use it despite family issues, despite no longer being able to get the medication from a doctor or in any legal way. Addiction occurs as a result of many factors. These factors include: genetics, environment, mental health issues, coping with difficult situations and how the medication interacts with the brain. An individual may turn to illicit sources when they are refused by their doctor. The danger of illegal drugs is that they may contain contaminants and much stronger opioids. Other concerning activities includes consuming the medication in a different way from how it would be normally prescribed. Crushing the pill so that it can be snorted or injected are examples and have lead to the development of abuse-resistant medications. Finding resources for individuals who have chronic pain and have concerns about opioid addiction can be difficult. The Substance Abuse & Mental Health Services Administration National Helpline is a free, confidential, 24/7, 365-day-a-year treatment referral and information service (in English and Spanish) for individuals and families facing mental and/or substance use disorders. 1-800-662-HELP (4357)
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Q: How Virtual Memory isolate different processes? Lets say I have two processes, process A and process B When the system is in Process A, CPU generates a virtual address let's say 0x800000. And the it switches to process B via context switch, the CPU also generates a same virtual address 0x800000. so if we write something to the page, how OS know it should be a page in Process B need to be modified rather than Process A? A: It is logical memory translation that separates processes; not virtual memory. Processes see logical memory addresses and have no access to the underlying physical memory. Each process has tables that tell the CPU how to translate logical addresses to physical addresses. The operating system maintains these tables. The location the tables are identified using protected hardware registers. When Process A switches out and Process B switches in, the operating system (assisted by the underlying hardware) changes the value of the registers so that B's tables are used. After that, the logical address 0X800000 no longer refers to "A"s physical memory location and instead points to "B"'s.
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Utility meters are used to determine the amount of a utility, such as electricity, gas or water, consumed at a given site. In particular, conventional residential electric meters are watt-hour meters which measure total energy consumed at the site and indicate the usage in standard kilowatt hours. Modern residential electric meters typically include solid-state electronics for monitoring, storing and displaying utility usage data over time. Total energy consumed, as well as other data, is digitally displayed. For billing and management purposes, a utility provider periodically sends a meter reader to the site to directly view and report the meter display. Data from the meter may also be downloaded from the meter into a handheld device. This is a time-consuming and costly process which has produced a growing demand for more cost-efficient methods of utility accounting. In response to the growing demand, automatic meter reading (AMR) technologies have been introduced, including radio-based, telephone line based, and power line based systems. Known radio-based apparatus and methods include meters equipped with low power radio frequency transmitters to transmit utility usage data from the meter to a central location such as a mobile van unit, or a central building. Optimal transmission efficiency requires an antenna equal in length to about 1/4 the wavelength of the transmission frequency. In particular, at the low frequencies typically used in remote meter assemblies, optimal transmission efficiency requires the use of antennas having lengths which are difficult to incorporate within a standard meter housing. Known radio meter assemblies address this problem by using a non-standard meter housing having towers or projections to accommodate an antenna projecting from the meter assembly. However, the manufacture of such specially designed, non-standard meter housings is costly. Further, the towers or projections can present obstacles for individuals passing or working near the meter assembly. Thus it would be desirable to provide a utility meter apparatus which includes a suitable antenna within a standard type meter housing. It would be further desirable to provide such apparatus which is simple and inexpensive to manufacture. In addition, it is generally desirable in providing meter apparatus to minimize the number and size of components and mounting hardware to minimize costs and labor. It would also therefore be desirable to provide utility meter apparatus which integrates a suitable antenna with other meter components, to minimize costs and labor.
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Q: Luke 23:54 - Historical Evidence that the Jewish Calendar Day began at Sunrise? Closely Related: - Historical Evidence that the Jewish Calendar Day Began at Sunset? - Luke 23:54 - How should "Sabbath Dawning" be Interpreted? - Historical Evidence of the Sabbath Rest Beginning the Preceding Night? What are the earliest textual evidences substantiating if a Jewish Calendar day may have begun at sunrise in ancient Israel? In view of the question : Luke 23:54 - How should "Sabbath Dawning" be Interpreted? A: Note: As the author of the question - I feel that a stronger answer would be to point to historical evidences outside of Scripture, and evidences earlier than the Talmud. For example, evidences regarding Beit Hillel would be helpful. 1. Question Restatement : What are the earliest textual evidences that a day in ancient Israel began at sunrise? Answers : Section #2. Rabbinic Literature; Section #3. the New Testament ... This answer presupposes a Christian authority to challenge and disregard Rabbinic authority and tradition : NASB, Titus 1:13-14 - This testimony is true. For this reason reprove them severely so that they may be sound in the faith, 14 not paying attention to Jewish myths and commandments of men who turn away from the truth. Note: These texts are generally accepted as reasonable bases to question whether a day was reckoned from sunset, or sunrise - objections notwithstanding. 2. Rabbinic Literature : MISHNA Pesahim IV - And the Sages say, "In Yehuda, they would do work on the eve of Pesach until noon; and in the Galilee they did not work at all [on that day]." And [with respect to] the evening [of the fourteenth of Nissan in places like the Galilee], Beit Shammai forbids [work], but Beit Hillel permits [it] until the sunrise. B. Talmud, Book 9 - Tracts Maccoth, Shebuoth, Eduyoth, Abuda Zara, and Horioth - R. Simlayi lectured: Six hundred and thirteen commands were said to Moses; three hundred and sixty-five of them negatives, corresponding to the number of days in a year counting according to sunrise; and two hundred and forty-eight positives, B. Talmud, Chulin 83a - GEMARA. Our Rabbis taught: This was expounded by R. Simeon b. Zoma: Since the whole passage deals only with the laws concerning consecrated animals, [27] and with regard to consecrated matters [a day means] the day and the night following it ... [28 For in connection with the eating of sacrificial meat it is written (ibid. VII, 15). It shall be eaten on the day of his offering; he shall not leave any of it until the morning. Thus it may be eaten the whole of the night following the day.] 3. The New Testament : NASB, Matthew 27:57-62 - 57 When it was evening, there came a rich man from Arimathea, named Joseph ... 59 And Joseph took the body [Mark 15:46 bought a linen cloth] ... and wrapped it in a clean linen cloth ... 62 Now on the next day, the day after the preparation, NASB, Matthew 28:1 - Now after the Sabbath, as it began to dawn toward the first day of the week, Mary Magdalene and the other Mary came to look at the grave. Greek Interlinear, Luke 23:54 - Indeed, it was the Day of Preparation, and Sabbath dawning. NASB, John 20:19 - So when it was evening on that day, the first day of the week ... 4. The Old Testament Genesis 1:6-8 - Then God [made the sky] and there was evening (ending the daytime), and there was morning (ending the nighttime), [making] the second day. Note: From Rabbi Samuel ben Meir's Peshat of Genesis 1:8, (@emory.edu) and Can The Torah Contradict Halacha (Jewish Law)?) NASB, Genesis 19:34 - On the following day, the firstborn said to the younger, “Behold, I lay last night with my father; let us make him drink wine tonight also; then you go in and lie with him, NASB, Exodus 16 - 23 then he said to them, “This is what the Lord meant: Tomorrow is a sabbath observance, a holy sabbath to the Lord. Bake what you will bake and boil what you will boil, and all that is left over put aside to be kept until morning.” 24 So they put it aside until morning, as Moses had ordered ... 27 It came about on the seventh day that some of the people went out to gather, but they found none. NASB, Leviticus 7:15 - ‘Now as for the flesh of the sacrifice of his thanksgiving peace offerings, it shall be eaten on the day of his offering; he shall not leave any of it over until morning. NASB, Leviticus 22:30 - It shall be eaten on the same day, you shall leave none of it until morning; I am the Lord. NASB, Leviticus 23:26-32 - 26 The Lord spoke to Moses, saying, 27 “On exactly the tenth day of this seventh month is the day of atonement; 32 It is to be a sabbath of complete rest ... on the ninth of the month at evening, from evening until evening you shall keep your sabbath.” Note: If presupposing "calendar days according to evenings" - then this passage would exclude the daytime of the 10th - internally contradicting itself. NASB, Numbers 33:3 - They journeyed from Rameses in the first month, on the fifteenth day of the first month; on the next day after the Passover the sons of Israel started out boldly in the sight of all the Egyptians, NASB, Deuteronomy 21:22 - “If a man has committed a sin worthy of death and he is put to death, and you hang him on a tree, 23 his corpse shall not hang all night on the tree, but you shall surely bury him on the same day (for he who is hanged is [s]accursed of God), so that you do not defile your land which the Lord your God gives you as an inheritance. NASB, 1 Samuel 19:10-11 - 10 ... And David fled and escaped that night. 11 Then Saul sent messengers to David’s house to watch him, in order to put him to death in the morning. But Michal, David’s wife, told him, saying, “If you do not save your life tonight, tomorrow you will be put to death.” NASB. 1 Samuel 20 - 18 Then Jonathan said to him, “Tomorrow is the new moon [first of the month], and you will be missed because your seat will be empty. 19 When you have stayed for three days, you shall go ... 34 Then Jonathan ... did not eat food on the second day of the new moon [the month] ... 35 Now it came about in the morning that Jonathan went out into the field for the appointment with David [on the third of the month]. NASB, 2 Chronicles 35 - 1 Then Josiah celebrated the Passover ... and they slaughtered the Passover animals on the fourteenth day of the first month. ... 10 So the service was prepared ... 11 They slaughtered the Passover animals ... 13 So they roasted the Passover animals ... 16 So all the service of the Lord was prepared on that day to celebrate the Passover, and to offer burnt offerings on the altar of the Lord according to the command ... NASB, Jonah 4:7 - But God appointed a worm when dawn came the next day and it attacked the plant and it withered. ... etc, etc. Note: See also a compelling argument at http://www.iahushua.com/ST-RP/twt.htm; But, the primary reference needs confirmation, (RABBINICAL ESSAYS BY JACOB Z. LAUTERBACH HEBREW UNION COLLEGE PRESS CINCINNATI 1951).
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The moon was formed by a violent, head-on collision between the early Earth and a “planetary embryo” called Theia approximately 100 million years after the Earth formed, UCLA geochemists and colleagues report. Scientists had already known about this high-speed crash, which occurred almost 4.5 billion years ago, but many thought the Earth collided with Theia (pronounced THAY-eh) at an angle of 45 degrees or more — a powerful side-swipe (simulated in this 2012 YouTube video). New evidence reported Jan. 29 in the journal Science substantially strengthens the case for a head-on assault. The researchers analyzed seven rocks brought to the Earth from the moon by the Apollo 12, 15 and 17 missions, as well as six volcanic rocks from the Earth’s mantle — five from Hawaii and one from Arizona. Christelle Snow/UCLA Paul Warren, Edward Young (holding a sample of a rock from the moon) and Issaku Kohl The key to reconstructing the giant impact was a chemical signature revealed in the rocks’ oxygen atoms. (Oxygen makes up 90 percent of rocks’ volume and 50 percent of their weight.) More than 99.9 percent of Earth’s oxygen is O-16, so called because each atom contains eight protons and eight neutrons. But there also are small quantities of heavier oxygen isotopes: O-17, which have one extra neutron, and O-18, which have two extra neutrons. Earth, Mars and other planetary bodies in our solar system each has a unique ratio of O-17 to O-16 — each one a distinctive “fingerprint.” In 2014, a team of German scientists reported in Science that the moon also has its own unique ratio of oxygen isotopes, different from Earth’s. The new research finds that is not the case. “We don’t see any difference between the Earth’s and the moon’s oxygen isotopes; they’re indistinguishable,” said Edward Young, lead author of the new study and a UCLA professor of geochemistry and cosmochemistry. Young’s research team used state-of-the-art technology and techniques to make extraordinarily precise and careful measurements, and verified them with UCLA’s new mass spectrometer. The fact that oxygen in rocks on the Earth and our moon share chemical signatures was very telling, Young said. Had Earth and Theia collided in a glancing side blow, the vast majority of the moon would have been made mainly of Theia, and the Earth and moon should have different oxygen isotopes. A head-on collision, however, likely would have resulted in similar chemical composition of both Earth and the moon. “Theia was thoroughly mixed into both the Earth and the moon, and evenly dispersed between them,” Young said. “This explains why we don’t see a different signature of Theia in the moon versus the Earth.” Theia, which did not survive the collision (except that it now makes up large parts of Earth and the moon) was growing and probably would have become a planet if the crash had not occurred, Young said. Young and some other scientists believe the planet was approximately the same size as the Earth; others believe it was smaller, perhaps more similar in size to Mars. Another interesting question is whether the collision with Theia removed any water that the early Earth may have contained. After the collision — perhaps tens of millions of year later — small asteroids likely hit the Earth, including ones that may have been rich in water, Young said. Collisions of growing bodies occurred very frequently back then, he said, although Mars avoided large collisions. A head-on collision was initially proposed in 2012 by Matija Ćuk, now a research scientist with the SETI Institute, and Sarah Stewart, now a professor at UC Davis; and, separately during the same year by Robin Canup of the Southwest Research Institute. Co-authors of the Science paper are Issaku Kohl, a researcher in Young’s laboratory; Paul Warren, a researcher in the UCLA department of Earth, planetary, and space sciences; David Rubie, a research professor at Germany’s Bayerisches Geoinstitut, University of Bayreuth; and Seth Jacobson and Alessandro Morbidelli, planetary scientists at France’s Laboratoire Lagrange, Université de Nice. The research was funded by NASA, the Deep Carbon Observatory and a European Research Council advanced grant (ACCRETE).
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Switching stem cell state through programmed germ cell reprogramming. Depending on their origin, embryo-derived stem cells have distinct properties that largely correspond to their counterpart in vivo. Mouse epiblast stem cells derived from post-implantation embryos differ from embryonic stem cells derived from blastocysts in their transcriptional and epigenetic profile, their morphology and culture requirements. When maintained in appropriate conditions, the cells keep self-renewing and do not adopt a different state. Recent studies, however, show that it is possible to convert between stem cell states. Here we review recent advances to induce stem cell state changes and we consider the potential of germ cell-mediated reprogramming for the conversion. Since the properties of mouse epiblast stem cells are similar to human embryonic stem cells, we discuss the significance of stem cell conversion and germ cell-mediated reprogramming in humans.
3.03125
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How to Choose and Store Fruit for Maximum Freshness and Flavor Do you stand in the produce section poking and prodding your fruit before making your picks? That's OK in some instances, since many fruits continue ripening after they've been picked. But not all fruits are created equal. For some, the ripening process stops once they're plucked from the plant from which they came. How do you know which fruits continue ripening and which don't? Take a look at our list of fruits that get better with age and those that come as they are. (See also: Produce Worker's Guide to Choosing Fruits and Veggies) Fruits That Ripen After Picking These fruits, called climacteric fruits, continue to ripen after picking because of the natural chemicals they contain — primarily ethylene gas — that are produced from within the fruit. These chemicals release enzymes called amylases, which turn stored starch into sugar making the fruits sweeter. Other enzymes — hydrolases — break down the fruit's chlorophyll, resulting in richer color. The fruit also becomes softer, which can lead to "over-ripening," as the amount of pectin is lessened by enzymes called pectinases. Once you bring them home, here's how to store climacteric fruits to ensure that they ripen properly, courtesy of The Fruitguys Almanac: Melons Store at room temperature until ripe, then refrigerate for up to 10 days. Peaches and Nectarines You can speed up the ripening process of peaches and other stone fruits by placing them in a paper bag. Otherwise, they should be stored at room temperature and away from direct sunlight and heat. Apples Store in a cool, dry place away from sunlight and heat. Apples can last up to six weeks in the fridge. (See also: 23 Great Ways to Use Apples) Avocados Store at room temperature until ripe. A ripe avocado will yield to firm gentle pressure, and the color will be almost black. To speed up the ripening process if you've bought under-ripe avocados, place them in a paper bag for a couple of days. Mangoes Store at room temperature until ripe, then store in a plastic bag in the refrigerator for up to seven days. Pears Pears are normally picked before peak ripeness to avoid bruising during transit. Store at room temperature away from sunlight and heat. When a pear gives to touch, it's ready to eat. Tomatoes Do not refrigerate tomatoes until they're fully ripe; allowing to ripen at room temperature with the stem side down will result in more flavorful tomatoes. Bananas Store bananas at room temperature away from direct sunlight and heat. Bananas should not be placed in the fridge as this will turn the skin black. To speed up the ripening process for not-quite-ripe bananas, place them in a paper bag with an apple overnight. Once they're ripe though, keep them longer by wrapping the stems in plastic. Plums Like peaches and pears, plums are sweet and delicious when they give softly to gentle touch. Store away from direct sunlight and heat. Guava Store at room temperature until ripe, then in the fridge for up to four days. Cantaloupes Store at room temperature until ripe, then store in the refrigerator for up to 10 days. Kiwis Store at room temperature until ripe. A ripe kiwi will stay fresh in the fridge for a few days, while a very firm unripe kiwi will keep in the fridge for up to two months. Fruits That Don't Ripen After Picking These fruits, called non-climacteric fruits, ripen only while they're still attached to the plant. Once they're picked, the ripening process stops. Unlike climacteric fruits that you can allow to ripen at home if they're under-ripe when you buy them (giving you an increased amount of time to consume them), when non-climacteric are picked at the peak of ripeness, the rapid-rot potential is hastened. On the flip side, if these fruits are picked when they're not quite ripe yet, the result could be a harder, tarter fruit than you'd like. Wrap cut up melon tightly in plastic or foil or store in an air-tight container in the fridge for up to four days. Cherries Do not wash cherries until you're ready to eat. Excess can be stored in the fridge in a plastic bag for up to a week. Figs Another non-climacteric fruit, figs are picked ripe. Enjoy them right away or store them in the fridge until you're ready to eat them. Grapes Do not wash grapes until you're ready to eat. Excess can be stored in the fridge in a perforated plastic bag (what they usually come in from the supermarket) for up to a week. Grapefruit Grapefruits will stay fresh at room temperature for a week and up to several weeks in the fridge. Oranges and Tangerines Store at room temperature for a couple weeks or in the fridge for up to several weeks. Lemons and Limes Store at room temperature for a couple weeks or in the fridge for up to several weeks. Pineapple Wrap cut up pineapple tightly in plastic or foil or store in an air-tight container in the fridge for up to four days. How to Pick the Best Fruit at the Supermarket I found this handy guide to picking fruit (from wikiHow) that may help you take home the best produce available the next time you're shopping. Three tips include: 1. Buy in Season Out-of-season fruit has a longer distance to travel because it comes from further away, so it's always best to buy in-season produce to ensure a higher quality of freshness and flavor. (See also: Fresh Fruits and Veggies By the Month) 2. Use Your Senses Employ your senses of touch, smell, and sight to pick the best produce. Instituting a little common sense doesn't hurt either. If there are a lot of bruises or (eek!) mold, steer clear. 3. Check the Stem If your fruit has a stem on it, use it as a guide to determine freshness. A green stem on ripe fruit is a winner; a green stem on hard fruit permits caution. Do you have other tips for choosing the best fruits and how to store them properly? Let me know in the comments below.
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1. Introduction {#sec1-foods-09-00324} =============== *Saccharomyces cerevisiae* (typically known as baker's yeast) is a single-cell eukaryote that is often utilized in research. *S. cerevisiae* has proven to be an ideal organism for research applications especially after releasing its genome sequence was released to the scientific community \[[@B1-foods-09-00324],[@B2-foods-09-00324]\]. This yeast can be stored, and its genome sequence and translated proteins are similar in action to those of other organisms. Its proteome contains cell cycle and signaling proteins \[[@B3-foods-09-00324]\]. In the past few years, biologically active peptides have been produced in different sources such as food, plants, animals and microorganisms. Many studies have focused on the production, isolation, and purification of the antimicrobial peptides \[[@B4-foods-09-00324]\]. Antimicrobial peptides (AMPs) are small oligopeptides (AMPs) that typically contain 10--100 amino acids, with a net positive charge and an amphipathic structure \[[@B5-foods-09-00324]\]. Antimicrobial peptides have a broad spectrum of inhibition activity against microorganisms such as bacteria, molds, yeasts, parasites, and some viruses. Many living organisms such as microorganisms, invertebrates, and other species belonging to the animal and plant kingdoms produce antimicrobial peptides \[[@B6-foods-09-00324]\]. In addition, bioactive peptides produced during the fermentation process by different microorganisms have been used as antibacterial, antioxidant, antihypertensive, anticancer, and immunomodulatory agents, in addition to containing lipid-reducing properties \[[@B7-foods-09-00324]\]. Several studies have investigated the production of antimicrobial peptides from lactic acid, however, few studies focus on the production of antimicrobial peptides from yeasts in a medium \[[@B7-foods-09-00324],[@B8-foods-09-00324]\]. In previous studies, metabolic compounds of *Saccharomyces boulardii* were separated and examined against 26 bacterial isolates in order to study the compounds' antimicrobial activity. The extracted peptide from *Saccharomyces boulardii* has ben shown to exhibit high inhibition activity toward *Bacillus cereus* \[[@B9-foods-09-00324]\]. It has been reported that some *S. cerevisiae* strains have the ability to produce antimicrobial peptides. Recent studies demonstrated that the isolated *S. cerevisiae* CCMI 885 produced small peptides (\<10 kDa) that exhibit antimicrobial activity against some yeasts such as *Hanseniaspora guilliermondii*, *Torulaspora delbrueckii*, *Kluyveromyces marxianus,* and *Lachancea thermotolerans* \[[@B10-foods-09-00324]\]. The ultrafiltration process with a 10 kDa cut-off was used to extract the antimicrobial peptide from *Candida intermedia* after growth on YPD agar at 28 °C over 7 days. The molecular weight of the peptide was 5 kDa exhibiting an inhibition activity against *Brettanomyces bruxellensis* \[[@B11-foods-09-00324]\]. Several authors have noted alternate strategies for biocontrol, such as the use of peptide-based killer toxins. For example, *Saccharomyces cerevisiae* produces peptide-based killer toxins that are able to inhibit the growth of different species of bacteria \[[@B12-foods-09-00324]\]. Similar results were reported for bioactive peptide production by *S. cerevisiae* CCMI 885 at 30 °C for 48 h. These peptides were used to inhibit the growth of some wine-related yeasts \[[@B8-foods-09-00324]\]. Past research including both in vitro and in vivo studies indicated that *Saccharomyces cerevisiae* inhibited intestinal tract infections from *Bacillus subtilis*, *B. cereus*, *Escherichia. coli*, *Proteus vulgaris*, *Pseudomonas aeruginosa*, *Salmonella typhimurium*, *Salmonella typhi*, *Staphylococcus aureus*, *Yersinia enterocolitica*, and some yeasts such as *Candida albicans* \[[@B13-foods-09-00324]\]. *Saccharomyces cerevisiae* yeast exhibits antibacterial activity against *E. coli*, *Pseudomonas* sp. *Salmonella* sp., *Staphylococcus aureus,* and *Vibrio cholera.* In addition, this yeast strain has antimicrobial activity against other pathogenic bacteria species, yeasts, and molds \[[@B14-foods-09-00324]\]. Many studies have described the effect of these antimicrobial activities on inhibition zones (zones free of growth). To date, however, very limited information is available about bioactive peptides from *Saccharomyces cerevisiae*. Thus, the aim of this study was to investigate the antimicrobial components from a full extract of *Saccharomyces cerevisiae,* isolate antibacterial peptides, and test their thermostability characteristics which are very important aspect in food production including for sterilization and thermal processes. 2. Materials and Methods {#sec2-foods-09-00324} ======================== 2.1. Microbial Strains {#sec2dot1-foods-09-00324} ---------------------- *Saccharomyces cerevisiae* ATCC 36858 was obtained from a local scientific store in Basrah, Iraq. *Bacillus subtilis* ATCC 23857, *E. coli* ATCC 25922, *Klebsiella aerogenes* ATCC 13048, and *Staphylococcus aureus* ATCC 25923 were supplied by the Food Science Department/College of Agriculture/University of Basrah, Iraq and used as indicator strains. 2.2. Antibacterial Peptide Production {#sec2dot2-foods-09-00324} ------------------------------------- First, 1 mL (6 log cfu/mL) of activated yeast (36 h) was added to 250 mL of glucose yeast peptone broth (GTPB) medium (Himedia, Mumbai, India) and incubated at 20, 25, 30, and 35 °C for 24, 48, 72, and 96 h, respectively. After incubation, *S. cerevisiae* cells were removed by centrifugation at 6000 rpm for 20 min at 4 °C, and the cell free yeast supernatant was filtered with 0.45 µm cellulose acetate membranes (Merck company, Watford, UK) \[[@B9-foods-09-00324]\]. In order to isolate the peptides that were released from the yeast in the medium, the filtered metabolic yeast extract was passed through ultrafiltration membranes with pore sizes of 10 kDa (cut-off 10 kDa, Millipore and Amicon, USA) and then concentrated (100-fold) with 2 kDa (cut-off 2 kDa) membranes. The concentrated metabolic yeast extract was lyophilized by freeze-drying (Heto Lab Equipment, Denmark). Next, 100 mg/mL of lyophilized metabolic yeast was tested against four indicator strains (*Bacillus subtilis* ATCC 23857, *E. coli* ATCC 25922, *Klebsiella aerogenes,* and *Staphylococcus aureus* ATCC 25923) using the agar well diffusion agar method, and then 100 µL of lyophilized peptide was added to the wells (6 mm) in Nutrient agar (Himedia, Mumbai, India). After incubation, the clear zones were measured in millimeters \[[@B15-foods-09-00324],[@B16-foods-09-00324]\]. 2.3. Purification of the Antibacterial Peptide from Yeast {#sec2dot3-foods-09-00324} --------------------------------------------------------- An ÄKTA Pure 25 System (GE Healthcare Life Sciences, Germany) was used to purify the antibacterial peptides from lyophilized metabolic extracts of *S. cerevisiae*. The specific column Superdex 200 (10/300GL) was used with a column volume set at 23.562 mL and a column diameter set at 10 mm with a pressure of 1.5 MPa. The column was filled with agarose and dextran. A 0.5 M acetate phosphate buffer (pH 5.0) at 0.5 mL/min was used for elution, and a 280 nm UV detector was used to determine the isolated peaks \[[@B17-foods-09-00324],[@B18-foods-09-00324]\]. Peak fractions were collected, and the antibacterial activity against two indicator strains (*E. coli* ATCC 25922 and *Staphylococcus aureus* ATCC 25923) was determined. 2.4. Characterization of the Antibacterial Peptide {#sec2dot4-foods-09-00324} -------------------------------------------------- ### 2.4.1. Thermal Stability of the Antibacterial Peptide {#sec2dot4dot1-foods-09-00324} To determine the thermal stability of the extracted antibacterial peptide from *S. cerevisiae,* 5 mL (10 mg/mL) of the active peptide was heated at 50, 60, 70, 80, 90, 100, 110, and 120 °C for 30 min. The antibacterial activity was estimated by the agar well diffusion agar activity against *E. coli* ATCC 25922 and *Staphylococcus aureus* ATCC 25923. Next, 100 μL of the extracted bioactive peptide was transferred to three wells in a Petri dish containing a Nutrient agar medium. The non-heated bioactive peptide was used as a control sample. The percentage of antibacterial activity was calculated using the following equation: where Ac is the inhibition zone of control sample, and As is the inhibition zone of test sample. ### 2.4.2. pH Stability of the Antibacterial Peptide {#sec2dot4dot2-foods-09-00324} The lyophilized purified antibacterial peptide from *S. cerevisiae* was dissolved in distilled water at 10 mg/mL and adjusted with 1N NaOH or 1N HCl to different pH values of 2, 3, 4, 5, 6, 7, 8, 9, and 10. After incubation for 24 h at 4 °C and 25 °C, the solutions containing the samples were adjusted to pH 7.0 ± 0.02 with a 0.5 M sodium citrate buffer. The inhibition activity of the peptide was then determined using the agar well diffusion agar method against *E. coli* ATCC 25922 and *Staphylococcus aureus* ATCC 25923. After incubation for 24 h at 37 °C, the percentage of antibacterial activity was calculated \[[@B19-foods-09-00324]\]. ### 2.4.3. Molecular Weight of the Antibacterial Peptide {#sec2dot4dot3-foods-09-00324} The molecular weights of the antibacterial peptide extracted from *S. cerevisiae* were analyzed using sodium dodecyl sulphate with 15% polyacrylamide gel electrophoresis (SDS-PAGE) as described by Judd \[[@B20-foods-09-00324]\]. Then, 1 mg/mL of the antibacterial peptide and standard proteins (α-Lactalbumin 14.4 kDa, Aprotinin 6.5 kDa, Glucagon 3.8 kDa, and Insulin-A 2.5 kDa) (Promega Company, Madison, WI, USA) were dissolved in a phosphate buffer and transferred to a vertical slab chamber (10 cm × 10 cm × 0.6 mm). The gel was run at 50 mA and 50--70V for 3 h. The molecular weight of the extracted antibacterial peptide was determined after the relative mobility (Rm) of the antibacterial peptide and marker proteins were determined per the following equation: Rm = the traveled distance of the peptide or marker proteins/traveled distance of methylene blue dye 2.5. Mode of Action {#sec2dot5-foods-09-00324} ------------------- The modes of action (bacteriostatic) of the extracted antibacterial peptide from *S. cerevisiae* were assayed as described by \[[@B10-foods-09-00324]\]. The 6 log cfu/mL cultures of four indicator strains were cultivated into 100 mL of Nutrient broth (Himedia, Mumbai, India). The lyophilized purified antibacterial peptide was added to the indicator strain cultures at a final concentration of 0.01% (*w:v*). The samples and the control sample (without antibacterial peptide) were incubated at 37 °C. Indicator strain suspensions were taken at 3, 6, 12, 18, and 24 h, and the absorbance was measured by spectrophotometry (Sunny UV.7804C, Tokyo, Japan) at OD~600~. The viable bacteria cells were determined on the nutrient agar at various incubation periods \[[@B12-foods-09-00324],[@B21-foods-09-00324]\]. 2.6. Statistical Analysis {#sec2dot6-foods-09-00324} ------------------------- Statistical analyses of the different treatments cited above were conducted using the SPSS Statistics V22.0 (Statistical Package for Social Sciences, San Antonio, TX, USA). An analysis of the variance (ANOVA table) of the data was conducted and means for treatment values were analyzed (*p* ≤ 0.05) with least significant difference (LSD). Differences were considered significant at *p* ≤ 0.05. 3. Results and Discussion {#sec3-foods-09-00324} ========================= 3.1. Optimum Conditions of for Antibacterial Peptides Production {#sec3dot1-foods-09-00324} ---------------------------------------------------------------- Both gram-negative bacteria tested including *E. coli* and *Klebsiella aerogenes* were inhibited by the presence of the antibacterial peptides produced from *Saccharomyces cerevisiae* in all the conditions tested (at the four time points and four different temperatures). This was not the case when testing the other two gram-positive bacteria including *Bacillus subtilis* and *Staphylococcus aureus,* which better tolerated the presence of the antibacterial peptides produced from *Saccharomyces cerevisiae.* This could be explained in part by the presence of cell walls comprised of thick layers of peptidoglycan in the case of Gram-positive bacteria. However, Gram-negative bacteria are known to have cell walls with a thin layer of peptidoglycan. The optimum conditions for the production of active peptides from yeast were 25--30 °C for 48 h, resulting in the highest inhibition towards *E. coli* and *Klebsiella aerogenes*. At 20 °C and 35 °C, the detected antibacterial activity was negligible with no effect against the four indicator strains (*Bacillus subtilis*, *E. coli*, *Klebsiella aerogenes*, and *Staphylococcus aureus*) especially at 24, 72, and 96 h ([Table 1](#foods-09-00324-t001){ref-type="table"}). 3.2. Purification of the Antibacterial Peptide {#sec3dot2-foods-09-00324} ---------------------------------------------- The extracted yeast peptides were passed through super filtration membranes of 10 kDa and 2 kDa and then freeze-dried. For further purification of the antibacterial peptide fractions, an ÄKTA purifier system was employed. Three peaks appeared after the ÄKTA Pure treatment. Fractions of 21--22 mL (peak 2) and 23--25 mL (peak 3) did not show growth inhibition activity against the two tested bacterial strains, while fractions of 16--20 mL (peak 1) showed the highest growth inhibition ([Figure 1](#foods-09-00324-f001){ref-type="fig"}). The yield of the antibacterial peptide was 155 mg/100 mL of the culture medium. The inhibition zones were 24 and 20 mm for *E. coli* ATCC 25922 and *Staphylococcus aureus* ATCC 25923, respectively. Gram-negative bacteria (*E. coli*) appeared to be more sensitive to antibacterial peptide fractions than gram-positive (*S. aureus*) bacteria. These results were in agreement with Fakruddin et al. \[[@B13-foods-09-00324]\] who reported that Gram-negative bacteria were more sensitive to yeast peptides when compared to gram-positive bacteria. The inhibition activity of peptides increased proportionally with the α-helix of hydrophobic C-terminal peptides. This feature may be related to the composition of the amphipathic amino acids that are necessary for binding the bacterial cell membranes \[[@B19-foods-09-00324],[@B22-foods-09-00324]\]. 3.3. Characterization of the Antibacterial Peptide {#sec3dot3-foods-09-00324} -------------------------------------------------- ### 3.3.1. Thermal Stability of the Antibacterial Peptide {#sec3dot3dot1-foods-09-00324} The effect of temperature on the *S. cerevisiae* antibacterial peptide was determined ([Figure 2](#foods-09-00324-f002){ref-type="fig"}). The results showed that the antibacterial peptide from yeast was stable at different temperatures ranging from 50 to 90 °C during 30 min of treatment. Interestingly, an antibacterial activity of 93% and 95% for *E. coli* and *S. aureus* was sustained even at 100 °C during 30 min of treatment. After 120 °C for 30 min, the antibacterial activity of the peptide was 68% and 77% for *E. coli* and *S. aureus*, respectively. This thermostable property makes this antibacterial peptide suitable for use in sterilization and thermal processes. The thermal stability of this small peptide could be related to the nature and chemical structures of such peptides, including the primary protein's structure and with low molecular weight. Similar reports have shown that antibacterial peptides isolated from different microbial sources are able to persist at high temperatures without any change in the antimicrobial activity \[[@B23-foods-09-00324],[@B24-foods-09-00324]\]. ### 3.3.2. Effect of pH on the Antibacterial Peptide {#sec3dot3dot2-foods-09-00324} In order to address the pH properties including dependent and independent effects, the above fragments were estimated for antibacterial activity inhibition against two indicator strains; *E. coli* ATCC 25922 and *Staphylococcus aureus* ATCC 25923. The effects of the pH values on the stability of the antibacterial peptide from *S. cerevisiae* are shown in [Figure 3](#foods-09-00324-f003){ref-type="fig"}. An evaluation of the pH value stability revealed that the antibacterial peptide remained stable after 24 h at 4 °C and 25 °C at pH values ranging from 4.0 to 7.0. The inhibition activity of the peptide with extreme pH values 2, 3, 8, 9, and 10 against bacterial strains was also tested ([Figure 3](#foods-09-00324-f003){ref-type="fig"}). Similar properties were previously studied for active peptides produced from yeasts, which were easily inactivated by strong acidic and alkaline conditions in different media. These characteristics limit the usage of peptides in food production with acidic and alkaline food. The antibacterial activity of this peptide was evaluated at different pH values at two temperatures (4 °C and 25 °C). The produced peptide was more effective at 4 °C within a pH range from 4 to 7 against the bacterial strains tested when compared to 25 °C. There was no significant difference (p \> 0.05) between samples of *S. aureus* when tested at 4 °C and 25 °C at pH value 2, while there was a significant difference (*p* \< 0.05) between samples of *E. coli* tested under the same conditions. In contrast, a significant difference (*p* \< 0.05) between samples of *S. aureus* and *E. coli* tested at 4 °C and 25 °C at a pH value of 2 was observed. Furthermore, the analysis showed the presence of significant differences (*p* \< 0.05) between samples of *S. aureus* tested at 4 °C and 25 °C at pH value 3. We also observed a significant difference (*p* \< 0.05) between samples of *E. coli* when tested at 4 °C and 25 °C at pH 3. When comparing the two bacterial strains, we observed the absence of any significant difference (*p* \> 0.05) between samples of *S. aureus* and *E. coli* tested at 4°C and pH 3. The presence of significant differences (*p* \< 0.05) between samples of *S. aureus* tested at 4°C at pH 10 were also observed. However, no significant differences (*p* \> 0.05) between samples of *S. aureus* tested at 25 °C and *E. coli* tested at 4 °C at pH value of 10 were observed. Interestingly, the lowest inhibition (%) value was observed in *E. coli* when tested at 25 °C and at pH 10. Overall, the newly discovered produced peptide possessed high thermal stability and a wide range of pH stability when compared to other peptides produced from microorganisms (e.g., bacteriocins) as described in previous studies \[[@B25-foods-09-00324],[@B26-foods-09-00324]\]. Moreover, antibacterial peptides acting in neutral and acidic environments are expected to provide protection from many unacceptable microorganisms that grow in these environments, contaminating food and causing spoilage \[[@B27-foods-09-00324]\]. ### 3.3.3. Molecular Weight of the Peptide {#sec3dot3dot3-foods-09-00324} The purified antibacterial peptide from active fractions (peak1) was analyzed using SDS-PAGE and showed a single band. The molecular weight of the antibacterial peptide, as determined by relative mobility, was approximately 9770 Da ([Figure 4](#foods-09-00324-f004){ref-type="fig"}), which is similar to the small molecular weight of other isolated peptides from *Klebsiella pneumonia,* as described in previous studies \[[@B28-foods-09-00324]\]. Thus, our results strongly suggest that peak 1 (9770Da) correspond to this peptide and might match the antibacterial activity produced by *S. cerevisiae* and thus be responsible for the bioactive activity shown against the different bacterial strains tested. In this sense, to better understand the role of molecular weight distribution in the inhibition of antibacterial activity of brewer's yeast, a fraction analysis using ultrafiltration with 10 kDa cutoff membranes was performed. The results showed that 3--10 kDa fractions were fundamentally comprised of smaller peptides with biological activity, which is in agreement with past studies that indicated that antibacterial peptides are small peptides \[[@B9-foods-09-00324]\]. 3.4. Mode of Action {#sec3dot4-foods-09-00324} ------------------- The antibacterial peptide effect of *S. cerevisiae* on cell viability (kill time) from four indicator strains is shown in [Figure 5](#foods-09-00324-f005){ref-type="fig"}. The antibacterial peptide reduced the viability of target bacteria compared to the control sample. The antibacterial peptide's efficacy depended on both the concentration of added peptide and exposure time. Additionally, the movement of small peptide and their spread during agar well diffusion appeared 3 h following the addition of the antibacterial peptide with 5.8, 5.5, 5.6, and 5.8 log (cfu/mL) reduction of *B. subtilis*, *E. coli*, *K. aerogenes,* and *S. aureus*, respectively. The statistical analysis of log (cfu/mL) reduction for each bacteria strain was estimated at interval times of 3, 6, 12, 18, and 24 h. The result showed that the antibacterial peptide effect on decreasing the viable cell counts was significant (*p* \< 0.05) between the control samples and all four bacterial strains among the five interval times tested. In contrast, there was no significant difference (*p* \> 0.05) between either Gram-positive strains or Gram-negative strains. In addition, the peptide's inhibition effect on Gram-negative strains was highly significant (*p* \> 0.05) when compared with Gram-positive strains. After 24 h of incubation, the peptide's inhibition effect on Gram-negative strains was high compared with that of Gram-positive strains. The antibacterial peptide caused a decrease in the viable cell counts of gram-negative strains ranging from 2 to 2.3 log. units along the evaluated times in comparison to gram-positive strains which ranged from 1.5 to 1.8 log. units. The kill-time of this peptide was in agreement with that from earlier reports \[[@B29-foods-09-00324],[@B30-foods-09-00324]\]. The mode of action of antimicrobial peptides fundamentally depends on the reaction of bioactive peptides with the membrane of bacteria cells and the cells' internal composition \[[@B31-foods-09-00324]\]. Generally, the antimicrobial peptides were effective due to the electrostatic reaction with the cell membranes. In order to understand the mechanism behind antimicrobial peptides, the results of various methods have suggested that adsorption of bioactive peptides will occur on the bacterial cell membrane, leading to complete damage to the membrane. For example, the brave straw model, aggregate model, carpet model, and toroid pore model are critically considered models of bioactive peptides as antibacterial compounds \[[@B27-foods-09-00324],[@B32-foods-09-00324]\]. 4. Conclusions {#sec4-foods-09-00324} ============== *S. cerevisiae* belongs to the eukaryotic kingdom is nonpathogenic, and due to its long history of use in the production of consumable products such as ethanol, many baked products, and pastries, it has been classified as a generally regarded as safe organism (GRAS). In this study, antibacterial peptide was produced and isolated from *Saccharomyces cerevisiae* (Baker's yeast) by an ultrafiltration process (two membranes with cut-offs 2 and 10 kDa) and purified using the ÄKTA Pure 25 system. The antibacterial peptide activity was then characterized and studied against four bacterial strains. The results showed that the peptide produced by *Saccharomyces cerevisiae* had a molecular weight of 9.77 kDa and exerted inhibition activity against both Gram-negative and Gram-positive bacteria. The produced peptide was more effective at 4 °C within a pH range of 4-7 against the bacterial strains tested when compared to 25 °C, while the lowest inhibition (%) was observed in *E. coli* when tested at 25 °C and at a pH value of 10. In addition, the peptide was thermostable and steady with pH values ranging from 4--7, which is a very important aspect in food production for sterilization and thermal processes. The isolated antibacterial peptide demonstrated its potential as a bio-preservative in food manufacturing. Although the current study isolated a peptide containing a novel bioactive compound from *Saccharomyces cerevisiae*, additional research regarding the amino acid sequence and structure of this antibacterial peptide is warranted. Investigation, S.T.G.A.-s.; designing and planning the experiments, A.B.A.; Supervision, A.J.A.A.-M.; Methodology, A.K.N.; Writing-review & editing, N.L.; Writing original draft, S.A.I. All authors have read and agreed to the published version of the manuscript. This research received no external funding. The authors declare no conflicts of interest. ![Chromatogram of gel filtration for antibacterial peptides from *Saccharomyces cerevisiae* by ÄKTA Pure 25 using Superdex 200 10/300 GL. (**A**) Inhibition zones of *E. coli* by peak1, (**B**) non-inhibition zone of *E. coli* by peak2 and peak3.](foods-09-00324-g001){#foods-09-00324-f001} ![The thermal stability of the antibacterial peptide production from *Saccharomyces cerevisiae*.](foods-09-00324-g002){#foods-09-00324-f002} ![Stability of antibacterial peptide production from *Saccharomyces cerevisiae* under different pH and temperature conditions.](foods-09-00324-g003){#foods-09-00324-f003} ###### The molecular weight of antibacterial peptide production from *Saccharomyces cerevisiae* was determined by electrophoresis method. (**A**) Sodium dodecylsulfate polyacrylamide gel electrophoresis of standard proteins and the antibacterial peptide. (**B**) Relative mobility of standard proteins and the antibacterial peptide. ![](foods-09-00324-g004a) ![](foods-09-00324-g004b) ![The mode of action of the antibacterial peptide from *Saccharomyces cerevisiae* against the four indicator bacteria strains.](foods-09-00324-g005){#foods-09-00324-f005} foods-09-00324-t001_Table 1 ###### The optimum conditions for antibacterial peptides produced from Saccharomyces *cerevisiae.* Strains 24 h 48 h 72 h 96 h ------------------------------------ ------ ------ ------ ------ ---- ----- ----- ----- ---- ---- ---- ---- ---- ---- ---- ---- *Bacillus subtilis* ATCC 23857 \- \- \+ \+ \+ \+ ++ ++ \- \- \+ \+ \- \- \+ \- *Escherichia coli* ATCC 25922 \+ \+ ++ \+ ++ +++ +++ ++ \+ \+ ++ \+ \+ \+ \+ \- *Klebsiella aerogenes* ATCC 13048 \+ \+ ++ ++ ++ +++ +++ +++ \+ ++ ++ ++ \+ \+ ++ \+ *Staphylococcus aureus* ATCC 25923 \- \- \+ \+ \+ \+ ++ \+ \- \- \+ \- \- \- \+ \- Diameter of inhibition zone (mm): +++: 16--20; ++: 12--16; +: 8--12; −:no inhibitory activity (including the 6mm diameter of each well).
3
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Erald Kolasi received his PhD in physics from George Mason University in 2016. People tend to think of capitalism in economic terms. Karl Marx argued that capitalism is a political and economic system that transforms the productivity of human labor into large profits and returns for those who own the means of production.1 Its proponents contend that capitalism is an economic system that promotes free markets and individual liberty.2 And opponents and advocates alike most often measure capitalism’s impact in terms of wealth and income, wages and prices, and supply and demand. However, human economies are complex biophysical systems that interact with the wider natural world, and none can be fully examined apart from their underlying material conditions. By exploring some fundamental concepts in physics, we can develop a better understanding of how all economic systems work, including the ways that the energy-intensive activities of capitalism are changing humanity and the planet. This article will explain how the fundamental features of both our natural and economic existence depend on the principles of thermodynamics, which studies the relationships between quantities such as energy, work, and heat.3 A firm grasp of how capitalism works at a physical level can help us understand why our next economic system should be more ecological, prioritizing long-run stability and compatibility with the global ecosphere that sustains humanity. Such an understanding requires a glance at some central concepts in physics. These include energy, entropy, dissipation, and the various rules of nature that bind them together. The central features of our natural existence, as living organisms and as human beings, emerge from the collective interactions described by these core physical realities. Although these concepts can be difficult to define without reference to specific models and theories, their general features can be outlined and analyzed to reveal the powerful intersection between physics and economics. The exchange of energy between different systems has a decisive influence on the order, phase, and stability of physical matter. Energy can be defined as any conserved physical property that can produce motion, such as work or heat, when exchanged among different systems.4 Kinetic energy and potential energy are two of the most important forms of energy storage. The sum of these two quantities is known as mechanical energy.5 A truck speeding down the highway packs a good amount of kinetic energy—that is, energy associated with motion. A boulder teetering at the edge of a cliff has great potential energy, or energy associated with position. If given a slight push, its potential energy transforms into kinetic energy under the influence of gravity, and off it goes. When physical systems interact, energy is converted into many different forms, but its total quantity always remains constant. The conservation of energy implies that the total output of all energy flows and transformations must equal the total input. Energy flows among different systems represent the engine of the cosmos, and they happen everywhere, so often that we hardly notice them. Heat naturally flows from warmer to colder regions, hence our coffee cools in the morning. Particles move from high-pressure areas to low-pressure areas, and so the wind starts to howl. Water travels from regions of high potential energy to regions of low potential energy, making rivers flow. Electric charges journey from regions of high voltage to regions of low voltage, and thus currents are unleashed through conductors. The flow of energy through physical systems is one of the most common features of nature, and as these examples show, energy flows require gradients—differences in temperature, pressure, density, or other factors. Without these gradients, nature would never deliver any net flows, all physical systems would remain in equilibrium, and the world would be inert—and very boring. Energy flows are also important because they can generate mechanical work, which is any macroscopic displacement in response to a force.6 Lifting a weight and kicking a ball are both examples of performing mechanical work on another system. An important result from classical physics equates the quantity of work to the change in the mechanical energy of a physical system, revealing a useful relationship between these two variables.7 Although energy flows can produce work, they rarely do so efficiently. Large macroscopic systems, like trucks or planets, routinely lose or gain mechanical energy through their interactions with the external world. The lead actor in this grand drama is dissipation, defined as any process that partially reduces or entirely eliminates the available mechanical energy of a physical system, converting it into heat or other products.8 As they interact with the external environment, physical systems often lose mechanical energy over time through friction, diffusion, turbulence, vibrations, collisions, and other similar dissipative effects, all of which prevent any energy source from being converted entirely into mechanical work. A simple example of dissipation is the heat produced when we rapidly rub our hands together. In the natural world, macroscopic energy flows are often accompanied by dissipative losses of one kind or another. Physical systems that can dissipate energy are capable of rich and complex interactions, making dissipation a central feature of the natural order. A world without dissipation, and without the interactions that make it possible, is difficult to imagine. If friction suddenly disappeared from the world, people would slip and slide everywhere. Our cars would be useless, as would the very idea of transportation, because wheels and other mechanical devices would lack any traction with the ground and other surfaces. We would never be able to hold hands or rock our babies. Our bodies would rapidly deteriorate and lose their internal structure. The world would be alien and unrecognizable. Dissipation is closely related to entropy, one of the most important concepts in thermodynamics. While energy measures the motion produced by physical systems, entropy tracks the way that energy is distributed in the natural world. Entropy has several standard definitions in physics, all of them essentially equivalent. One popular definition from classical thermodynamics states that entropy is the amount of heat energy per unit of temperature that becomes unavailable for mechanical work during a thermodynamic process.9 Another important definition comes from statistical physics, which looks at how the microscopic parts of nature can join to produce big, macroscopic results. In this statistical version, entropy is a measure of the various ways that the microscopic states of a larger system can be rearranged without changing that system.10 For a concrete example, think of a typical gas and a typical solid at equilibrium. Energy is distributed very differently in these two phases of matter. The gas has a higher entropy than the solid, because the former’s particles have far more possible energy configurations than the fixed atomic sites in solids and crystals, which have only a small range of energy configurations that will preserve their fundamental order.11 We should emphasize that the concept of entropy does not apply to a specific configuration of macroscopic matter, but rather applies as a constraint on the number of possible configurations that a macroscopic system can have at equilibrium. Entropy has a profound connection to dissipation through one of the most important laws of thermodynamics, which states that heat flows can never be fully converted into work.12 Dissipative interactions ensure that physical systems always lose some energy as heat in any natural thermodynamic process, where friction and other similar effects are present. Real-world examples of these thermodynamic losses include emissions from car engines, electric currents encountering resistance, and interacting fluid layers experiencing viscosity. In thermodynamics, these phenomena are often considered irreversible. The continuous production of heat energy from irreversible phenomena gradually depletes the stock of mechanical energy that physical systems can exploit. According to the definition of entropy, depleting useful mechanical energy generally implies that entropy increases. Formally stated, the most important consequence of any irreversible process is to increase the combined entropy of a physical system and its surroundings. For an isolated system, entropy continues to rise until it reaches some maximum value, at which point the system settles into equilibrium. To clarify this last concept, imagine a red gas and a blue gas separated by a partition inside a sealed container. Removing the partition allows the two gases to mix together. The result would be a gas that looks purple, and that equilibrium configuration would represent the state of maximum entropy. We can also relate dissipation to the concept of entropy in statistical physics. The proliferation of heat energy through physical systems changes the motion of their molecules into something more random and dispersed, increasing the number of microstates that can represent the macroscopic properties of the system. In a broad sense, entropy can be seen as the tendency of nature to reconfigure energy states into distributions that dissipate mechanical energy. The traditional description of entropy given above applies in the regime of equilibrium thermodynamics. But in the real world, physical systems rarely exist at fixed temperatures, in perfect states of equilibrium, or in total isolation from the rest of the universe. The field of non-equilibrium thermodynamics examines the properties of thermodynamic systems that operate sufficiently far from equilibrium, such as living organisms or exploding bombs. Non-equilibrium systems are the lifeblood of the universe; they make the world dynamic and unpredictable. Modern thermodynamics remains a work in progress, but it has been used to successfully study a broad spectrum of phenomena, including heat flows, interacting quantum gases, dissipative structures, and even the global climate.13 There is no universally accepted meaning of entropy in non-equilibrium conditions, but physicists have offered several proposals.14 All of them include time when analyzing thermodynamic interactions, allowing us to determine not just whether entropy goes up or down, but also how quickly or slowly physical systems can change on their path to equilibrium. The principles of modern thermodynamics are therefore essential in helping us understand the behavior of real-world systems, including life itself. The central physical objective of all life forms is to avoid thermodynamic equilibrium with the rest of their environment by continuously dissipating energy, as the physicist Erwin Schrödinger suggested in the 1940s, when he used non-equilibrium thermodynamics to study the key features of biology.15 We may call this vital objective the entropic imperative. All living organisms consume energy from an external environment, use it to fuel vital biochemical processes and interactions, and then dissipate most of the energy consumed back to the environment. The dissipation of energy to an external environment allows organisms to conserve the order and stability of their own biochemical systems. The essential functions of life critically depend on this entropic stability, including functions like digestion, respiration, cell division, and protein synthesis. What makes life unique as a physical system is the sheer variety of dissipation methods that it has developed, including the production of heat, the emission of gases, and the expulsion of waste. This sweeping capacity to dissipate energy is what helps life to sustain the entropic imperative. Indeed, physicist Jeremy England has argued that physical systems in a heat bath flooded with large amounts of energy can tend to dissipate more energy.16 This “dissipation-driven adaptation” can lead to the spontaneous emergence of order, replication, and self-assembly among microscopic units of matter, providing a potential clue into the very dynamics of the origin of life. Organisms also use the energy they consume to perform mechanical work by, for example, walking, running, climbing, or typing on a keyboard. Those organisms with access to many energy sources can do more work and dissipate more energy, satisfying the central conditions of life. The thermodynamic relationships among energy, entropy, and dissipation likewise impose powerful constraints on the behavior and evolution of economic systems.17 Economies are dynamical and emergent systems compelled to function in certain ways by their underlying social and ecological conditions. In this context, economies are non-equilibrium systems capable of rapidly dissipating energy to some external environment. All dynamical systems gain strength from some energy reservoir, reach peak intensity by absorbing a regular supply of energy, then unravel from internal and external changes that either disrupt vital energy flows or make it impossible to keep dissipating more energy. They can even experience long-term undulations by growing for some time, then shrinking, then growing again, before finally collapsing. Interactions between dynamical systems can produce highly chaotic results, but energy expansions and contractions are the core features of all dynamical systems. The energy consumed by all economic systems is either converted into mechanical work and the physical products derived from that work, or is simply wasted and dissipated to the environment. We can define the collective efficiency of an economic system as the fraction of all energy consumed that goes into creating mechanical work and electrical energy. Economies that increase the amount of mechanical work they generate can produce more goods and services. But however important it may be, mechanical work represents a relatively small fraction of total energy use in any economy; the vast majority of the energy consumed by all economies is routinely squandered to the environment through waste, dissipation, and other kinds of energy losses. Throughout history, economic growth has depended heavily on people consuming more energy from their natural environments.18 When humans were hunters and foragers, the primary asset that performed mechanical work was the human muscle.19 Our nomadic way of life lasted for some 200,000 years, but underwent significant disruptions after the Ice Age. Over millennia, changing ecological conditions around the world compelled numerous groups to adopt pastoralist and agricultural strategies. Agrarian economies relied heavily on cultivated plants and domesticated animals to help generate surpluses of food and other goods and resources. These agrarian modes of production and consumption dominated human societies for almost ten thousand years, but were eventually replaced by a new economic system. Capitalism emerged and spread through colonial expansion, waves of industrialization, the proliferation of epidemic diseases, genocidal campaigns against indigenous populations, and the discovery of new energy sources. The global economy has since become an interconnected system of finance, computers, factories, vehicles, machines, and much more. Creating and sustaining this system required a major upward transition in the rate of energy throughput from our natural environments. In our nomadic days, the daily rate of per capita energy consumption was around 5,000 kilocalories.20 By 1850, per capita consumption had risen to roughly 80,000 kilocalories per day, and has since ballooned to about 250,000 kilocalories today.21 From a physics perspective, the fundamental feature of all capitalist economies is an excessive rate of energy consumption focused on boosting economic growth and material surpluses. The collective deployment of capital assets can generate incredible levels of mechanical work, allowing people to produce more, travel great distances, and lift heavy objects, among other tasks. Capitalism is far more energy-intensive than any previous economic system, and it has wrought unprecedented ecological consequences that may threaten its very existence. It remains uncertain how long humanity can sustain capitalism’s energy-intensive activities, but there is no doubt that the fantasy of endless growth and easy profits cannot continue. All dynamical systems must eventually come to an end. Over the last two centuries, inefficient capitalist economies have unloaded large amounts of energy losses to their natural environments in the forms of waste, chemicals, pollutants, and greenhouse gases. The aggregate effect of all this waste and dissipation has been fundamentally to alter critical energy flows throughout the ecosphere, triggering a major social and ecological crisis in the natural world. This socioecological crisis is still in its early phases, but has already spawned calamities like deforestation, global warming, ocean acidification, and substantial losses in biodiversity.22 Barring revolutionary changes to our socioeconomic system, this crisis will only continue and intensify. As this occurs, accumulating problems in the natural world will threaten the long-term viability of global civilization. The products we dissipate to the environment may be useless to us, but they often serve as energy reservoirs for other dynamical systems. Energy losses often have an amplifier effect on human civilization, meaning their true costs are far greater than may be visible or superficially understood. Consider the unsanitary conditions in cities throughout much of human history. Cities in pre-modern economies were typically filthy, with trash and waste overwhelming many public spaces. Yet these energy losses were a critical source of food and nourishment for a wide variety of other living organisms, especially insects and other small animals that could survive in the midst of human civilization. When these creatures became hosts to deadly diseases, human waste helped to concentrate their numbers in precisely the worst places: high-density areas like cities. As a consequence, epidemic diseases usually generated far larger death tolls than they would have otherwise, with the unimaginable carnage of the Black Death as a primary example.23 Today we face our own versions of this ancient problem, but on a much bigger scale. There are several kinds of gases in the atmosphere, known as greenhouse gases, able to absorb outgoing heat radiation.24 When these gases in the atmosphere trap and emit radiation back to the surface of the planet, large numbers of photons excite the electrons, atoms, and molecules on the surface to higher energy states, in a process called the greenhouse effect. These additional excitations and fluctuations at the microscopic level collectively represent the warmth we experience at the macroscopic level. The greenhouse effect is critical because it makes the Earth warm enough to be habitable.25 Over the last two centuries, however, wealthy and industrialized nations have been reinforcing this natural process by pumping vast amounts of new greenhouse gases into the atmosphere, in turn causing more global warming. This artificial reinforcement of the greenhouse effect has already had profound consequences for our species and others. Thermal excitations from an amplified greenhouse effect often act as a powerful energy reservoir for other dynamical systems and natural phenomena, including storms, floods, droughts, cyclones, wildfires, insects, viruses, bacteria, and algae blooms.26 A warming planet could also reinforce positive feedback mechanisms in the climate capable of inducing even more warming, beyond that already caused by our greenhouse gas emissions. These mechanisms, such as melting sea ice and thawing permafrost, would allow the planet to absorb more solar energy while naturally emitting vast quantities of greenhouse gases.27 The resulting chaos would render any human attempts to mitigate global warming futile. This is precisely what should worry us: the chaos we are unleashing on the planet through the capitalist system will find a way to produce a new kind of order, one that threatens human civilization itself. As capitalism expands, the ecological crisis will worsen. The intensifying dynamical systems of nature will increasingly interact with our civilizations and could severely disrupt the vital energy flows that support social reproduction and economic activities. Regions with high population densities subject to recurring natural disasters are especially vulnerable. Cyclone Bhola killed about 500,000 people when it struck East Pakistan in 1970, triggering a series of massive riots and protests that culminated in a civil war and contributed to the establishment of a new country, Bangladesh.28 Numerous studies have concluded that the worst drought to strike Syria in almost a thousand years was partly responsible for the social and political tensions that culminated in the current civil war.29 The climate is a resilient dynamical system capable of assimilating many different physical changes, but this resilience has its limits, and humanity will be in deep trouble if it keeps trying to transgress them. These arguments highlight one of the deepest flaws in modern economic theory: it lacks a scientific foundation. Orthodox economic philosophies, from monetarism to the neoclassical synthesis, focus on describing the transient financial features of capitalism, mistaking these for immutable and universal laws of nature. Capitalist economics has largely been transformed into a metaphysical philosophy whose goal is not to provide a scientific foundation for economics, but to produce sophisticated propaganda designed to protect the wealth and power of a global elite. Any scientific explanation of economics must begin with the realization that energy flows and ecological conditions—not any “invisible hand” of the market—dictate the long-term macroscopic parameters of all economies. Important contributions along these lines have come from the field of ecological economics, especially in seminal works by the economists Nicholas Georgescu-Roegen and Herman Daly, but also from the systems ecologist Howard Odum.30 Marx himself incorporated ecological concerns into his economic and political thought.31 The contributions of these and other thinkers revealed that the economic features of the world are emergent properties shaped by underlying physical realities and ecological conditions, making an understanding of these conditions critical to any basic understanding of economics. Ecological thought differs from the orthodox schools of economics in fundamental ways. Most importantly, ecological theory contends that we can no longer treat waste and dissipative losses as “externalities” and “costs of doing business,” given how important these energy losses can be in shaping the dynamical evolution of economic systems. What mainstream economists call “externalities” include the physical products we dump into the environment—everything from pollutants and plastic trash to toxic chemicals and greenhouse gases. The consequences of extreme energy losses can have a profound effect on the future evolution of dynamical systems. As scientists continually stress, the energy losses from our modern economies are so large and intense that they are starting to fundamentally alter the energy flows of the entire ecosphere, from the reinforcement of the greenhouse effect to the changing chemistry of the oceans. Some of these new concentrations of energy then act as reservoirs that power the formation and operation of other dynamical systems, which often disrupt the normal activities of civilization. Hence the fundamental reason our economic actions cannot be decoupled from the natural world: if the effects associated with our energy losses become powerful enough to destroy the normal functions of our civilizations, then no number of ingenious economic policies will save us from the wrath of nature. Most people in power today believe we can carefully manage capitalism and prevent the worst effects of the ecological crisis. A popular strain of technological optimism holds that innovation can solve the fundamental ecological problems that humanity faces. Several different solutions have been proposed to fix our ecological woes, from the adoption of renewable energy sources to more outlandish programs like carbon storage and sequestration. All these ideas share the presumption that capitalism itself does not have to change, because technological solutions will always be available to deliver more economic growth and a healthier environment. From Beijing to Silicon Valley, technocapitalists are fond of arguing that capitalism can keep humming along through gains in energy efficiency.32 The ultimate reason why this strategy will fail over the long run is that nature imposes absolute physical limits on efficiency that no extent of technological progress can overcome. The recent breakdown in Moore’s Law because of quantum effects is a notable example.33 Another is the efficiency barrier that the Carnot cycle poses for all practical heat engines.34 But our most pressing concerns have to do with the underlying relationships between technological innovation and economic growth. Faith in technological solutions helps to foster further technological innovation and economic growth, increasing the overall demands placed on the biophysical world and the dissipation associated with the capitalist system. We can examine these relationships by first looking at how people and economic systems respond to efficiency gains. For a sense of whether capitalism can deliver major improvements in efficiency, we need to develop a general theory that explains how the collective efficiency of our economic systems changes over time. When fuel efficiency improves, we often drive longer distances. When electricity becomes cheaper, we often power more appliances. Even those who proudly save energy at home through recycling, composting, and other activities are more than happy to jump on an airplane and fly halfway around the world for a vacation. People often take savings in one area and exchange them for expenses in another. What we end up doing with efficiency gains can sometimes be just as important as the gains themselves. In ecological studies, this phenomenon is generally known as the Jevons Paradox, which reveals that the intended effects of efficiency improvements do not always materialize.35 First formulated in the mid-nineteenth century by the British economist William Stanley Jevons, the paradox states that increases in energy efficiency are generally used to expand accumulation and production, leading to greater consumption of the very resources that the efficiency improvements were supposed to conserve. Boosting efficiency leads to cheaper goods and services, which encourages more demand and more spending, leading to the consumption of more energy.36 Jevons first described this effect in the context of coal power and steam engines. He observed that efficiency improvements in steam engines had encouraged more consumption of coal in Britain, implying that increased energy efficiency did not actually yield energy savings. Variations of this paradox are known in economics as the rebound effect. Most economists accept that some versions of the effect are real, but disagree over the size and the scope of the problem. Some believe rebound effects are irrelevant, arguing that efficiency improvements do encourage lower levels of energy consumption in the long run.37 In a comprehensive review of the literature on the subject, the UK Energy Research Centre determined that the most extreme versions of the rebound effect probably no longer apply to developed economies. However, they also argued that large rebound effects across our economies can still occur. They reached the following conclusion: “it would be wrong to assume that…rebound effects are so small that they can be disregarded. Under some circumstances (e.g. energy efficient technologies that significantly improve the productivity of energy intensive industries) economy-wide rebound effects may exceed 50% and could potentially increase energy consumption in the long-term.”38 The fact that significant economy-wide rebound effects are possible should give us pause about the utility of efficiency strategies in combating the ecological crisis and climate change. In fact, this entire argument obscures a more important uncertainty: the problem of whether efficiency improvements can come fast enough to alleviate the worst consequences of the ecological crisis, which are still ahead of us. Given the mechanics and incentives of capitalism, we should beware the current infatuation with efficiency optimism. To clarify these arguments, we need a theory that explains the role of efficiency in the wider context of technological progress. The rebound effect and the Jevons Paradox focus on understanding how people and economic systems behave in response to efficiency gains. More fundamental, however, is the task of understanding the general evolution of collective efficiencies over long periods of time. The dominant theme of technological innovation throughout history has been the effort to shift the burden of energy use from human muscles to other physical and biological systems, such as animals, machines, and computers. Consider cars, bicycles, airplanes, microwaves, dishwashers, vacuum cleaners, and virtually all the “wonders” of modern life: their central goal is to exploit energy and perform tasks that would normally require the exertion of human muscles. Robots and artificial intelligence have recently become all the rage, ready to swoop in and perform menial tasks that we have no desire to do. The expansion in mechanical output facilitated by technological progress typically leads to more energy-intensive societies where those who control the means of production can generate greater surpluses and profits. Technological innovation under capitalism in particular has boosted the collective amount of mechanical work that economies can generate, and has also ballooned the rate of energy consumption from our natural environments. But it has not fundamentally changed collective efficiencies, implying that higher rates of economic growth have usually been accompanied by larger energy losses. Economic systems typically use new sources of energy to expand production, consumption, and accumulation, not to fundamentally improve efficiency. From the cultivation of plants and the domestication of animals to the burning of fossil fuels and the invention of electricity, the mastery and discovery of new energy sources has generally produced more energy-intensive societies. Although any economic system may make efficiency gains, these are incidental and secondary to the wider goal of accumulation. The overall efficiency of an economic system is highly inertial, changing at a glacial pace. We see this very process playing out now with greenhouse gas emissions, although the ecological crisis extends far beyond this problem. Political and business leaders have hoped for years that technological progress will somehow deliver both higher rates of economic growth and a sharp reduction in greenhouse gas emissions. Things have not gone according to plan. The year 2017 saw a substantial global rise in harmful emissions, defying even the modest goals of the Paris Agreement.39 Even before that, the United Nations had warned of an “unacceptable” gap between government pledges and the emission reductions needed to prevent some of the worst consequences from climate change.40 The challenges of boosting efficiency are more apparent when we view capitalism on a global scale: although many developed nations have made modest but measurable improvements in their collective efficiencies, these gains have been undercut by developing economies still in the process of industrialization.41 Evidently, substantial changes in the collective efficiency of any economic system rarely materialize in short periods of time. Technological growth under the regime of capitalism will deliver some additional progress on efficiency, but certainly not enough to prevent the worst consequences of the ecological crisis. One of the best ways to understand the inertia of collective efficiencies is to compare energy efficiencies under capitalism with those of humanity’s nomadic days, more than ten thousand years ago. Recall that human muscles performed most of the work in nomadic societies, and the efficiency of our muscles is roughly 20 percent, perhaps much more under special circumstances.42 For comparison, most gasoline-powered combustion engines have an efficiency of roughly 15 percent, coal-fired power plants come in at a global average of about 30 percent, and the vast majority of commercial photovoltaics are somewhere around 15 to 20 percent.43 All these figures vary depending on a wide array of physical conditions, but when it comes to efficiency, we can safely conclude that the dominant assets of capitalism hardly do better than human muscles, even after three centuries of rapid technological progress. Cost and convenience are the main reasons why technological innovation works this way, emphasizing mechanical output and the scale of production at the expense of efficiency. Large gains in efficiency are extremely difficult to achieve, in both physical and economic terms. From time to time, a James Watt or an Elon Musk comes along with an amazing invention, but such products do not represent the entire economy. The Watt steam engine was a major improvement over previous models, but its thermal efficiency was only 5 percent at best.44 And although Musk’s Tesla motors have a phenomenal operating efficiency, the electricity needed to run them often comes from much more inefficient sources, such as coal-fired power plants. If you drive a Tesla in Ohio or West Virginia, the dirty sources of energy powering it mean that your amazing technological product produces roughly the same carbon emissions as a Honda Accord.45 The collective efficiency of capitalist economies remains relatively low because these economies are interested in growing their profits and production levels, not in making the enormous investments needed for significant improvements in efficiency. In November 2017, a group of 15,000 scientists from more than 180 nations signed a letter sounding the alarm on the ecological crisis and what awaits us in the future.46 Their prognosis was grim, and their proposals—intentionally or not—amounted to a wholesale repudiation of modern capitalism. Among their many useful recommendations was a call for “revising our economy to reduce wealth inequality and ensure that prices, taxation, and incentive systems take into account the real costs which consumption patterns impose on our environments.” Our fundamental problem is easy to state: modern civilization uses far too much energy. And the solution to this problem is equally easy to state, but very difficult to implement: humanity must reduce the rate of energy consumption that has prevailed in modern times. The best way to drive down that rate is not through messianic delusions of technological progress, but rather by breaking the structures and incentives of capitalism, with their drive for profits and production, and establishing a new economic system that prioritizes a compatible future with our natural world. Governments and popular movements around the world should develop and implement radical measures that will help to move humanity from capitalism toward ecologism. These measures should include punitive taxes and caps on extreme wealth, the partial nationalization of energy-intensive industries, the vast redistribution of economic goods and resources to poor and oppressed peoples, periodic restrictions on the use of capital assets and technological systems, large public investments in more efficient renewable energy technologies, sharp reductions in work hours, and perhaps even the adoption of mass veganism among industrialized nations that no longer rely on animals for food production. The economic priorities of the ecological project should focus on improving our existing quality of life, not on trying to generate high levels of economic growth to boost capitalist profits. If human civilization is to survive for thousands of years, and not just a few more centuries, then we must drastically scale back our economic ambitions and focus instead on improving the quality of life in our communities, including our community with nature. Rather than trying to dominate the natural world, we should change course and coexist with it. Notes
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Are Specific Varieties Of Hearing Loss Hereditary? Can hearing loss be written into your family genes? Without a doubt, the answer is “Yes.” Genetic abnormalities actually lay at the root of most types of hearing loss. Furthermore, developmental experts consider genetic hearing loss to be the most frequently occurring birth defect in developed countries. A primer on genetics. They way your body looks and functions is governed by the genetic code of your DNA – your genes. Researchers have discovered more than 100 genes that can impact hearing. Hearing loss can result from any one of these genes being missing or altered. When an individual having these irregular gene sequences has a child, the abnormal gene or genes can be passed on to the child too. Types of genetic hearing loss. Genetic hearing loss can affect the outer ear, inner ear or both. Depending on the particular cause, the ensuing hearing loss is classified as conductive, senorineural or mixed (which is a combination of the two). Additionally, some genes may cause hearing loss before a child learns to talk (prelingual hearing loss), and other genes cause hearing impairments that show up after speech is learned (postlingual hearing loss). Usher syndrome affects over fifty percent of the deaf-blind population, making it one of the most widespread causes of hearing loss. Waardenburg syndrome is another prevalent disorder that affects hearing in the inner ear but also causes pale skin, a streak of white hair, and light-colored or multi-colored eyes. Is there any good news? While it’s true that parents with hearing loss genes may pass them on to their children, it doesn’t necessarily mean that the children will have a hearing problem. Most genes related to hearing loss are recessive, which means that even when an individual has an irregular gene, that gene will not always cause a problem so long as a normal copy is received from the other parent. Even if both parents have hearing loss, their kids may still not be affected because different genes may be responsible in each parent. Individuals concerned with genetic hearing loss can see a doctor for genetic testing that can help identify potential risks.
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It is now well established that putting an infant to sleep on his or her back is the single most important step in reducing the risk of sudden infant death syndrome (SIDS). Recent research also suggests that a baby's risk for SIDS can be greatly reduced by using a pacifier. Medical research also shows that babies who can satiate their natural sucking reflex sleep better. Experts recommend giving babies a pacifier every time they are placed to sleep. The exact reason that pacifiers reduce the risk of SIDS is not known. One suggestion is that the presence of a pacifier in the mouth may discourage babies from turning over onto their tummy because turning or moving may dislodge the pacifier. Another suggestion is that pacifier use and/or the sucking reflex helps keep the tongue positioned forward, keeping the airways open. Yet another suggestion is that pacifiers stimulate upper airway muscles and saliva production, so using pacifiers may keep babies from falling into a deep sleep, which is protective against SIDS. One of the factors that has led to a revival in the ancient practice of swaddling is the practice of putting babies to sleep on their backs as this helps to reduce the incidence of SIDS. However, babies tend to sleep better on their tummies than on their backs. Swaddling has been found to assist infants sleep more comfortably on their backs and to assist in easing colic, which also improves sleep. Swaddling is the practice of wrapping infants tightly in a blanket or cloth so that movement of the limbs is restricted. Medical research has shown that swaddling and sleeping supine (on the back) promotes more efficient sleep, with fewer spontaneous awakenings compared with sleeping supine but unswaddled. Swaddling seems to inhibit each step from sighs through startles to full arousal in the arousal pathway. This results in swaddled babies sleeping longer and being more likely to return to sleep on their own: Swaddling: a systematic review, Bregje E. van Sleuwen, et al, Pediatrics vol 120, number 4, October 2007. To achieve the benefits of swaddling, infants need to be wrapped sufficiently tight to restrain the limbs and inhibit the movements associated with a full startle reflex, which can wake babies from sleep. The startle reflex is seen in infants from birth to around 6 months of age (some sources indicate it can occur in infants as old as eight months). The startle reflex is a natural reflex that babies are born with, and can be triggered by loud noise or sudden movement. In response to the trigger, the baby throws back his/her head, extends out the arms and legs, cries, then pulls the arms and legs back in. A baby's own cry can trigger the reflex. It can also be triggered during sleep, causing the baby to wake. Care needs to be taken not to swaddle too tightly because this can compress the chest and make breathing difficult. There is also an increased risk of overheating especially when the head is covered or when there is infection. Improper swaddling can also lead to a risk of hip dysplasia (including hip dislocation) especially when swaddling with the hips and legs in extension and adduction (i.e. drawn toward the midline or sagittal plane of the body). Other risks associated with swaddling babies includes an increased risk of SIDS when a swaddled infant is placed prone (on his or her front) or able to turn to prone position. The SIDS risk seems to be increased by swaddling with the head covered. There is also a slightly increased risk of acute respiratory infections, which seems to be related to the tightness of swaddling. These are discussed in the systematic review of swaddling referred to above. Therefore, to swaddle properly and effectively, and to achieve the desired result, the blanket must be snug enough to immobilise the infant's arms, and to a certain degree its legs, but loose enough that it is still comfortable and not increase the risk of hip dysplasia or suppressed respiration. Many parents and carers experience difficulty with swaddling due to unfamiliarity with swaddling techniques. If not swaddled correctly, the infant often wriggles free of the swaddle thus becoming exposed to a risk of suffocation or SIDS-related issues due to loose bedding and unrestricted positioning of the infant. However, swaddling alone cannot eliminate these risks. This is especially true for infants that are more than around six weeks old, when they are stronger and more active than newborns. Even when swaddled tightly with all limbs securely enclosed, infants can potentially roll, becoming entrapped in the swaddling blanket or trapped face down while still wrapped in the blanket. To overcome the difficulty faced by parents and carers in learning proper swaddling techniques and to address the problems of improper swaddling, various swaddling suits have been developed. Swaddling suits such as the infant safety suit of WO 2007/098558 (the Snuggo), the Ergococcoon and the Woombi address the problems of wrapping too loosely or too tightly since the degree of wrapping is predetermined by the suit. As mentioned above, recent evidence shows that sucking on a pacifier is protective against SIDS. In addition, supplemental non-nutritive sucking (that is, sucking in addition to that required for feeding) is known to help to soothe an infant. Researchers have discovered that there is a clear reflex connection between the hand and mouth of a human fetus as early as 12-14 weeks after conception, and that thumb sucking in utero is common. After birth, many infants continue to soothe themselves by sucking on their thumbs or fingers. A newborn's ability to get the hands up to his or her mouth and suck is seen as a positive ability of the infant to organize him or herself in a self-soothing way. This helps establish an infant's ability to independently cope with stress and frustration. Thus it would be an advantage to have a swaddle suit that overcomes the problems of improper swaddling and also provides an opportunity for non-nutritive sucking. This would improve the calming effect of the swaddling suit, since research that indicates that multiple simultaneous measures such as swaddling and sucking (along with rocking, white noise and other interventions) have an additive calming effect on crying infants: Karp H, Swaddling and excessive crying, Journal of Pediatrics, July 2007, e2. None of the aforementioned swaddling suits facilitates non-nutritive sucking. None of WO 2007/098558 (the Snuggo), the Ergococcoon or the Woombi provide access to the hands while the infant is swaddled. Movement of the infant's arms in all three of these swaddling suits is restricted to 180 degrees below the shoulder line so the hands are restrained near the body but below the shoulder line, out of reach of the mouth. U.S. Pat. No. 7,587,769 is a swaddling article including a blanket formed with opposed arm-receiving sleeves that attempts to facilitate non-nutritive sucking by securing a pacifier to the blanket, thus overcoming the problem of pacifiers falling out of an infant's mouth. The blanket incorporates a pacifier retaining structure to retain a pacifier relative to the blanket so that the pacifier is unable to fall away from the blanket. This keeps the pacifier positioned near the mouth when the blanket is wrapped around an infant so it is available for the infant to suck on at will. The pacifier retaining structure includes a flap of fabric secured to the upper edge of the swaddling blanket. The flap is drawn across the region of the baby's mouth. A disadvantage of the swaddling article of U.S. Pat. No.7,587,769 is that it relies on a pacifier to be secured to the blanket. Another disadvantage is that it essentially extends the blanket across the face (around the mouth region), which can be uncomfortable and covering the face during sleep increases the risk of SIDs. Yet another disadvantage is that the swaddle article is in the form of a modified blanket and so lacks the convenience and advantages of a swaddling suit for example, the risk remains that the swaddle may loosen through movement thus becoming less effective and also posing a suffocation risk. While research indicates that there are benefits associated with non-nutritive sucking (e.g. pacifier use), it also indicates that pacifier use may be associated with problems including: interference with breast feeding, dependence on the pacifier (so the baby cannot sleep without one), an increased risk of middle ear infections, and dental problems associated with prolonged use. Hence, despite the established benefits of pacifier use, many parents choose not to use pacifiers. Further, some infants simply do not take to pacifiers. In any event, so as to minimise interference with breastfeeding, the recommendation is to wait until nursing is going well (usually one month) before offering a pacifier. Thus pacifier use is not suitable for all infants and it would be an advantage to provide a means for non-nutritive sucking that does not rely on pacifier use. Reflexes are set motor responses to specific sensory stimuli. Newborns have a hand-to-mouth reflex that is a natural instinct to get their hands to their mouths. Research indicates that this ability to access the hands for sucking is important for self-soothing. The hand-to-mouth reflex (along with the startle reflex) is one of a number of primitive reflexes present from birth or earlier. Primitive reflexes are thought to have provided evolutionary advantages to humans. The somatosensory system is a complex system of receptors and processing centres that produce the senses including touch, motion perception (proprioception) and balance, and spatial perception of body parts (kinesthesia). The tactile or skin senses (that rely on skin sensors for touch and pressure) appear first during fetal development. The vestibular system, which is responsible for movement and balance perception, and the tactile (touch) sensors are highly developed in newborns. The hand-to-mouth reflex goes with two reflexes that are considered essential to appropriate feeding responses in newborns: the rooting (or search) reflex and the sucking reflex. Both of these reflexes are triggered by a touch (including pressure) stimulus. The rooting reflex occurs when the infant's cheek or corner of the mouth is touched or stroked. The infant's mouth opens to follow and “root” (search) in the direction of stroking or touch. Rooting helps the baby to become ready to suck. The suckling reflex is triggered by touching the mucous membranes on the inside of the mouth with any object. Both reflexes facilitate nursing. In the hand-to-mouth reflex, when an infant's cheek is stroked, his or her mouth roots and the arm flexes. After hand and mouth find each other, the infant may suck energetically on the hands. There is a need for a swaddling suit that does not suffer the disadvantages of a swaddling using a blanket and that effectively swaddles infants by sufficiently restraining movement of the limbs to suppress the startle reflex, yet still affords sufficient movement so that infants can get their hand(s) toward their mouth, so providing the opportunity for non-nutritive sucking without reliance on a pacifier. U.S. Pat. No. 4,611,353 describes a swaddling garment in which an infant's arms are gently bound in a bent-elbow, hands-up position to inhibit the ability to fling open the arms without restricting arm movement. Binding of the arms in this manner is described as useful for holding a premature infant. The BabySense Cuddlewrap is a blanket shaped to wrap an infant's arms tightly near to the body and face, again as a means for suppressing jerks of the arms and legs. However, neither the manufacturer of the BabySense Cuddlewrap nor the inventor of garment of U.S. Pat. No. 4,611,353 refer to the benefit of providing access to the hands for non-nutritive sucking while swaddled and neither swaddle addresses this need adequately. While the swaddle of U.S. Pat. No. 4,611,353 is referred to as a garment, the part of the garment that is responsible for binding the arms in the manner described is two flaps of sufficient length to wrap around the infant and overlap each other, secured in place either by strips of hook and loop fasteners or simply by relying on the length of the flaps. Thus binding of the arms is achieved by a length of fabric in a manner analogous to a blanket. Loosening of the binding is possible with movement/wriggling of the baby—particularly in the embodiment that relies on the length of the flaps to secure the wrapping around the infant or where the hook and loop fastening is not sufficient to restrain loosening of the flaps through wriggling movement of the infant. Therefore, the risks associated with use of swaddling blankets or cloths remain with both the BabySense Cuddlewrap and the swaddle of U.S. Pat. No. 4,611,353, including: 1. wrapping too tightly so as to suppress respiration; 2. overwrapping the infant in several layers of fabric so as to increase the risk of overheating (particularly as the preferred embodiment of U.S. Pat. No. 4,611,353 also includes a hood); 3. loosening of the swaddle around the upper body will result in excess fabric around the upper body, posing a suffocation risk to the infant; 4. the arms are only restrained so long as the swaddle remains tightly secured around the infant and loosening allows increasing movement of the arms; 5. the swaddle does not facilitate or maintain access to the hands, although access can initially be provided depending on how the hands are positioned when the infant is first swaddled. Thus both U.S. Pat. No. 4,611,353 and the BabySense Cuddlewrap share many of the disadvantages of swaddling using a blanket, and do not act to secure the hands in position near the face to provide the opportunity for non-nutritive sucking without reliance on a pacifier. It is an object of the present invention to provide a new or alternative swaddling suit that swaddles infants by restraining movement of the limbs and which overcomes the disadvantages of other swaddling suits by allowing movement of the hand towards the mouth and maintaining the hand in a position relative to the infant's face thereby facilitating non-nutritive sucking.
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5 Tips for Evaluating & Improving City Parks: Trust for Public Land Public parks are an essential component to a healthy and thriving city. Parks offer opportunities for fitness, relaxation and community building, giving children a place to play and adults a place to stay active. They incorporate green spaces, playgrounds, multi use trails, and open areas for sports and recreation to give city residents the chance to enjoy their natural surroundings. Why Parks Are Important in City Planning If you are involved in urban design and planning – as a public official, landscape architect or civil engineer – you know the importance of having green space in a city. When city parks are successful, they offer a clear return on investment, including: Promoting public health Boosting tourism and property value Rejuvenating local economies Creating more energy-efficient spaces Connecting neighbors to each other Exposing residents to nature Unfortunately, not every neighborhood has safe, green spaces for residents to enjoy. The Trust for Public Land, a nonprofit organization that works to conserve land for parks, gardens and other natural areas, reports that there is just 1 park for every 14,000 Americans. In neighborhoods that lack parks, children either play in streets and empty lots or stay inside and engage in more sedentary activities, increasing their risk for health problems such as obesity and diabetes. How to Evaluate City Parks The Trust for Public Land developed ParkScore as a system to analyze a city’s current access to parks and green space. ParkScore evaluates factors including acreage, playgrounds, recreational facilities, spending per resident and park accessibility within a 10-minute walk. Cities can earn a maximum score of 100. Of the 50 largest US cities, Minneapolis has the highest score at 81.0 and Fresno has the lowest at 27.5. The Trust for Public Land also outlines these seven factors of excellence for city parks: 1. A clear expression of purpose 2. An ongoing planning and community involvement process 3. Sufficient assets in land, staffing, and equipment to meet the system’s goals 4. Equitable access 5. User satisfaction 6. Safety from crime and physical hazards 7. Benefits for the city beyond the boundaries of the parks How can you use this information to enhance the green spaces in your city? 5 Tips for Improving Your City Parks 1. Use ParkScore and the seven factors of excellence as metrics. Make it a priority to build sustainable and thriving neighborhood parks in your city. Examine your ParkScore and compare your city with others around the country. Learn from best practices and case studies, then set your own city planning goals. 2. Identify the needs of your community. What do the people in your city – both children and adults – want in a neighborhood park? Do kids want a wide field for soccer, football and Frisbee? Would adults like long running and walking paths that are safe to use in all seasons? Survey stakeholders in your community to find out what they would use most, and explore what construction materials and other resources you would need to meet these goals. 3. Locate underserved areas to find where neighborhood parks are most needed. Which areas in your city aren’t within a 10-minute walk from a park? Consider how strategic city planning could resolve this problem. 4. Explore creative ideas to use your city’s available space. Even highly developed cities can use innovative urban design to develop more green spaces. Look at vacant factories, shipyards, empty lots, rail depots and other spaces not in use to see if they could be converted into city parks. Maintenance costs add up over time, so it’s important to build parks with a long-term strategic plan in mind. What construction materials will be a smart investment over the years? Which materials will stand the test of time and still work well decades from now? Elevated greenways, multi use trails, pedestrian bridges and other boardwalks built with PermaTrak’s precast concrete require no maintenance and are easy to install, durable, and design-flexible, making them a perfect fit for city parks. With more timber boardwalk alternates available, the debate around concrete boardwalks vs. timber boardwalks has become more prevalent. Engineers are faced with 6 key design differences between concrete and timber boardwalks...read more About This Blog The PermaTrak boardwalk blog articles are written for landscape architects, engineers, and agency or municipality professionals. We aim to provide educational resources for designing and building boardwalks, pedestrian bridges, trail and greenway systems.
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Q: how to filter an array using a binary representation of an integer argument? > > A binary representation of a number can be used to select elements from an array. For example, n: 88 = 23 + 24 + 26 (1011000) array: 8, 4, 9, 0, 3, 1, 2 indexes: 0 1 2 3 4 5 6 selected * * * result 0, 3, 2 so the result of filtering {8, 4, 9, 0, 3, 1, 2} using 88 would be {0, 3, 2} In the above, the elements that are selected are those whose indices are used as exponents in the binary representation of 88. In other words, a[3], a[4], and a[6] are selected for the result because 3, 4 and 6 are the powers of 2 that sum to 88. Write a method named filterArray that takes an array and a non-negative integer and returns the result of filtering the array using the binary representation of the integer. The returned array must big enough to contain the filtered elements and no bigger. So in the above example, the returned array has length of 3, not 7 (which is the size of the original array.) Futhermore, if the input array is not big enough to contain all the selected elements, then the method returns null. For example, if n=3 is used to filter the array a = {18}, the method should return null because 3=20+21 and hence requires that the array have at least 2 elements a[0] and a1, but there is no a1. If you are using Java or C#, the signature of the function is int[ ] filterArray(int[ ] a, int n) I have this question I am trying to solve and I wrote this code public static int[] filterArray(int[] a, int n) { int[] x = new int[a.length]; int j = 0; int count = 0; while (n > 0) { int digit = n % 2; n /= 2; x[j] = digit; j++; } System.out.println(Arrays.toString(a)); System.out.println(Arrays.toString(x)); for (int k = 0; k < x.length; k++) { if (x[k] == 1) count++; } System.out.println("count is " + count); int[] z = new int[count]; for (int i = 0; i < z.length; i++) { for (int k = 0; k < x.length; k++) { if(x[k] == 1) { z[i] = a[k]; } } } System.out.println(Arrays.toString(z)); return x; } When I try to test is with a test array of System.out.println(Arrays.toString(filterArray(new int[] { 0, 9, 12, 18, -6 }, 11))); It is giving me the following output [18, 18, 18] the correct output is [0, 9, 18] A: The problem is your nested loops: you're iterating over the entire input array for each element of the output array and keep overwriting the values with the last found element (step through your code with a debugger and you'll see that). To fix that, swap your loops and keep track of the "next" output index: int i = 0; for (int k = 0; k < x.length; k++) { if(x[k] == 1) { z[i] = a[k]; i++; //advance the output index } } That will make your code faster as well since now you don't have O(n2) complexity but just O(n).
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Species must overcome multiple barriers to successfully establish in a novel range[@b1]. One such barrier is associated with mutualistic interactions, which are predicted to limit invasion success because the new range may not contain effective mutualist partners required for initial establishment[@b2]. Legumes (*Fabaceae*) are a globally distributed and highly diverse family of flowering plants, many of which are dependent on symbiotic nitrogen-fixing bacteria for growth and reproduction[@b3]. Anthropogenic activity has introduced legumes into new regions and continents at an unprecedented global scale[@b4]. However, it remains untested whether legume dependency on symbiotic nitrogen fixation has facilitated or hindered establishment into novel ranges. Legume hosts acquire rhizobial symbionts horizontally via the environment. This could limit legume establishment following long distance dispersal by reducing access to compatible symbiont partners[@b5][@b6] or suitable environmental conditions for efficient nitrogen fixation[@b7]. On the other hand, symbiotic nitrogen fixation has been purported to facilitate legume colonization, especially in disturbed or degraded habitats[@b8][@b9], potentially favouring the establishment of symbiotic nitrogen-fixing legumes over non-symbiotic legumes. According to these contrasting hypotheses, symbiotic nitrogen fixation could either impede or promote plant establishment in new ranges. However, we currently lack a global macro-ecological analysis to support or refute the generality of either of these claims. Morphological and molecular evidence show that legumes (*Fabaceae*) form one large monophyletic group and that rhizobial symbiosis evolved from a single origin over 59 million years ago[@b10][@b11]. This origin was followed by multiple gains and losses of the ability to symbiotically fix nitrogen across multiple clades[@b10][@b12], allowing us to directly compare the relative prevalence of symbiotic and non-symbiotic legume species in non-native areas. Using an expert-annotated global legume distribution database[@b13] and the most comprehensive list of nitrogen-fixing trait data available[@b10], we evaluated differences in recent establishment in introduced areas between symbiotic and non-symbiotic legumes (see Methods). In total, our data set comprises 3,213 symbiotic species and 317 non-symbiotic species. Each species record consists of its symbiotic nitrogen-fixing status and a broad characterization of its global range distribution (as shown by a list of geographic polygons, referred to as 'regions\' hereafter, describing countries, islands or states in which the species is found), and the 'native\' or 'non-native\' designation for each geographic region (see Methods section). We found that non-symbiotic legumes have spread to a greater number of geographic areas compared to symbiotic species at a global scale, providing evidence that symbiosis with nitrogen-fixing bacteria has limited establishment of legumes into novel islands, regions and continents. Results ======= The role of symbiosis in introduction success --------------------------------------------- Within our dataset, 21.6% of all legume species occur in at least one non-native region (that is, polygon) and 15.8% occur in two or more non-native regions, confirming that many symbiotic and non-symbiotic legume species have successfully invaded or been introduced into new regions, continents and islands ([Fig. 1](#f1){ref-type="fig"}). Our analysis of all species in the dataset at the regional level (see Methods section) show that symbiotic legumes have a significantly lower probability of occurring in non-native regions ([Table 1](#t1){ref-type="table"}), which translates into 49.7% fewer non-native regions per species ([Fig. 2a](#f2){ref-type="fig"}). Furthermore, for successfully introduced species with at least one non-native range, we found that symbiotic legumes retain a lower probability of occurring in multiple non-native regions ([Table 1](#t1){ref-type="table"}), translating into 37.1% fewer numbers of non-native regions compared to non-symbiotic legumes ([Fig. 2b](#f2){ref-type="fig"}). We excluded the possibility that non-native symbiotic legume species simply occurred in fewer yet much larger countries ([Supplementary Note 1](#S1){ref-type="supplementary-material"}) by confirming that each non-symbiotic species had, on average, a larger total non-native range area ([Supplementary Table 1](#S1){ref-type="supplementary-material"}) and no difference in the average size of individual regions that comprise the total introduced range area ([Supplementary Table 1](#S1){ref-type="supplementary-material"}). For species occurring in more than one non-native region we also measured the degree of geographic dispersion between non-native regions and found no difference in the degree of geographic dispersion between either legume group ([Supplementary Table 1](#S1){ref-type="supplementary-material"}), showing that introduced symbiotic legumes do not have more or less geographically widespread non-native regions than non-symbiotic legumes. Together, our analyses show that the contrast in introduction success between symbiotic and non-symbiotic legumes was characterised by differences in the number of non-native regions. These results combined support the hypothesis that non-symbiotic legumes have a higher chance of establishing and subsequently spreading to a greater number of geographic areas ([Fig. 3](#f3){ref-type="fig"}). Accounting for potentially confounding species traits ----------------------------------------------------- We found that latitude of origin, size of a species\' native range, plant life form (woody or not woody), life-history (annual or perennial), number of human uses, and the interaction between symbiosis and number of human uses were all significant predictors of introduction success. Non-symbiotic legumes tended to occur more frequently at or near the equator in their native range ([Fig. 3](#f3){ref-type="fig"}; ref. [@b14]). However, our analysis show that latitudinal bias in introduction success favours legume species naturally occurring away from the equator ([Table 1](#t1){ref-type="table"}), indicating that biased dispersal related to latitudinal effects would favour symbiotic rather than non-symbiotic legumes. Total native area was a significant factor in predicting the prevalence of establishment in non-native regions, ([Table 1](#t1){ref-type="table"}), but we found no difference in total native range areas between symbiotic and non-symbiotic species ([Supplementary Fig. 4](#S1){ref-type="supplementary-material"}). While woodiness was the dominant life form in non-symbiotic legumes ([Supplementary Fig. 4](#S1){ref-type="supplementary-material"}), being woody did not always predict introduction success. Specifically, while woody plants had a higher probability of occurring in non-native regions among all species in the dataset, when the analysis was restricted to introduced species, woody plants had a significantly lower probability of being introduced into multiple non-native regions ([Table 1](#t1){ref-type="table"}). Furthermore, annual species were more likely to establish in non-native regions ([Table 1](#t1){ref-type="table"}), but only 0.8% of non-symbiotic species are annual ([Supplementary Fig. 4](#S1){ref-type="supplementary-material"}). In total, our analysis show that while total native area, latitude, plant life form and life-history are important (as other studies have also shown[@b15]), their effects do not eliminate the symbiosis trait as a key determinant of establishment in novel ranges. The geographic area of a region had no effect on the prevalence of non-native species within it ([Table 1](#t1){ref-type="table"}). This likely reflects limited variation in area between our regions ([Supplementary Fig. 6](#S1){ref-type="supplementary-material"}), combined with other factors being much more important for successful introduction such as the amount of trade a nation receives (this variation due to unknown factors would be reflected in the region-level random effect). The role of human use in successful introductions ------------------------------------------------- We found that ∼30% of species in our dataset had at least one human use, and that legume species with more uses are much more likely to establish in non-native regions ([Table 1](#t1){ref-type="table"}). Species with human uses may be more likely to establish due to more frequent intentional introduction attempts (i.e., higher human-mediated propagule pressure), which may mask or confound differential establishment patterns driven by the symbiosis trait itself. Our analysis accounts for this potential bias by including it as a covariate (along with its interaction with symbiosis), and then statistically evaluating the main effect of symbiosis at no (that is, zero) human uses (this is important because of the presence of the interaction[@b16]). The main effect of symbiosis ([Table 1](#t1){ref-type="table"}) thus evaluates any differences in non-native establishment patterns that are least likely to be impacted by human-mediated propagule pressure. After accounting for the number of human uses in this manner, we found that non-symbiotic legumes are still much more likely to establish in non-native regions ([Figs 2](#f2){ref-type="fig"} and [4](#f4){ref-type="fig"}; [Table 1](#t1){ref-type="table"}). We also found a significant interaction between symbiosis and the number of human uses, suggesting that human use does have an influence on the successful introduction of symbiotic versus non-symbiotic legumes. We predicted that if human uses were exacerbating the spread of non-symbiotic legumes over symbiotic legumes (above the disparity observed at no human uses) that we should observe a negative interaction in our main model. However, we found a positive interaction, indicating that the disparity between symbiotic and non-symbiotic legumes decrease, rather than increase ([Fig. 4](#f4){ref-type="fig"}). These results combined provide evidence that human-mediated propagule pressure is not generating the pattern that non-symbiotic legumes are more prevalent in non-native regions. Influence of phylogenetic history on introduction success --------------------------------------------------------- The ability to symbiotically fix nitrogen has been gained and lost multiple times across the legume phylogeny, although the trait is more concentrated in certain clades ([Supplementary Fig. 1](#S1){ref-type="supplementary-material"}). If the pattern of successful introductions across species also shows strong phylogenetic structure, it is possible that our results could reflect a lack of independence among the species we used in this study due to their shared evolutionary history with respect to other predictive yet unmeasured traits. However, the probability of having a non-native range has no phylogenetic signal (phylogenetic parameter alpha=31.27; [Supplementary Note 2](#S1){ref-type="supplementary-material"}). When we incorporated phylogenetic structure into our analysis, which included all covariates from our main analysis ([Supplementary Note 2](#S1){ref-type="supplementary-material"}), non-symbiotic legume species still had a significantly higher probability of establishing in non-native regions ([Supplementary Table 2](#S1){ref-type="supplementary-material"}), consistent with results of our main analysis. Overall, these analyses indicate that the increased ability of non-symbiotic legume species to establish in a greater number of non-native ranges was not driven by phylogenetic dependence and makes it unlikely that our results can be explained by another trait that is evolutionarily correlated with symbiosis and also influences introduction success. Discussion ========== In summary, our findings clearly support the argument that nitrogen-fixing legumes are highly dependent on the symbiosis and that this dependency is sufficiently large to generate dispersal or establishment barriers at a global scale across multiple legume species, regions and continents ([Fig. 3](#f3){ref-type="fig"}). Inadequate population density of compatible rhizobia or appropriate environmental conditions for effective nitrogen fixation in introduced ranges are viable explanations for our results. This explanation would suggest that symbiotic legume hosts and their compatible symbionts would frequently need to be introduced simultaneously or that introductions would favour legumes that are able to form associations with a broad diversity of rhizobia[@b17][@b18], which is consistent with empirical findings from previous studies examining introduced *Acacia* species[@b18][@b19][@b20]. Our results are also consistent with the explanation that an evolutionary investment in the mutualistic interaction with rhizobia has resulted in reduced competitive ability of symbiotic nitrogen-fixing legumes[@b21], relative to non-symbiotic legumes. This explanation would require that the fitness cost of harbouring the symbiosis trait is higher in non-native ranges relative to the native range. Changes in soil resource availability have been proposed as a mechanism to alter the cost-benefit ratio of plant nitrogen-fixation[@b21] and human activity is often associated with increased nutrient deposition[@b22]. However, experimental evidence has shown that invasive nitrogen-fixing plants have greater growth in fertile soils compared to invasive co-occurring non-fixing plants[@b23], suggesting that symbiotic nitrogen-fixation is a net fitness benefit in non-native ranges, rather than a cost. Our study also highlights the prominent effects of propagule pressure, mediated by increased intentional introductions associated with human use attributes of species. The number of human uses for a species was a powerful predictor of the prevalence of successful introduced ranges. This is consistent with a number of other studies which found human use to be important in predicting establishment of plant species outside their native range[@b24][@b25], including legumes[@b4][@b26][@b27]. Among highly useful species, we found that the difference in introduction success between symbiotic and non-symbiotic legumes lessens and eventually reverses ([Fig. 4](#f4){ref-type="fig"}). This suggests that if species are highly useful, any natural establishment barriers among symbiotic legumes (that is, lack of mutualist partners) may be overcome through increased human effort to intentionally introduce a species (for example, increased effort to inoculate new sites lacking rhizobia). It is possible that after human intervention has allowed a symbiotic legume species to overcome its establishment barriers, the benefits of nitrogen fixation then allow it to be more successful. However, the majority of species looked at in this study have no recorded human uses, so that the effect prevailing at low human uses is of particular importance for legume species as a whole. Transplant trials have shown that many legumes rely on soils that are pre-inoculated with compatible microbial symbionts to establish[@b28][@b29] and that soils are highly variable in the abundance[@b30][@b31][@b32] and inter-continental genetic structure[@b33] of compatible rhizobia. However, symbiotic nitrogen-fixation has also been implicated in facilitating the invasion of some of the most widespread and problematic legume species of the world[@b30], giving the appearance that compatible rhizobia are cosmopolitan in their distribution. Based on these isolated observations and studies, it has been difficult to establish a general pattern with respect to the role of symbiosis in limiting or facilitating legume establishment[@b34]. Though the size of our analysis and its global extent is unprecedented, we acknowledge that only a fraction of the estimated ∼19,000 legume species have been characterized for their symbiosis ability (∼20% species and ∼60% of legume genera[@b35]). Nevertheless, based on an examination of ∼3,500 legume species, our study reveals that symbiotic mutualism traits are important in predicting the introduction success of legumes across multiple continents and islands. Our study further highlights likely ecological costs associated with being a nitrogen-fixing species, and the potential for plant species distributions to be influenced by soil microbial biogeography at a global scale. Methods ======= Experimental design ------------------- The objective of our study was to investigate whether symbiosis with nitrogen-fixing legumes had any predictive power with respect to legume introductions globally. We compiled symbiotic nitrogen-fixation data and geographic distribution data matched to as many legume species as possible (see below). We measured introduction success by counting the number of non-native regions of occurrence for each available species. We then analysed the predictive power of the symbiosis trait on introduction success in the presence of other potentially confounding or correlated covariates that might be important in predicting legume introductions. Once we verified that the significance and direction of response for symbiosis remained after the inclusion of other covariates, we analysed the predictive power of symbiosis, incorporating phylogenetic structure into our analyses. Symbiotic nitrogen-fixation data -------------------------------- Nitrogen-fixation status was extracted for all available legume species (members of the family *Fabaceae*) from the publicly available database compiled by Werner *et al*[@b36]. This database scores each species as either 'symbiotic\' or not, and has been compiled from a number of experimental and observational studies examining the presence or absence of rhizobial infections on 5,427 legume species (see Werner *et al*.[@b36] for more details). For the species we used in this study, information on nitrogen-fixation status covers ∼20% of all known legume species (3,530 species out of ∼19,700) and ∼60% of all known legume genera (440 genera out of ∼750). Since we aimed to determine whether symbiosis is a potential barrier or facilitator of initial legume establishment, we evaluated the presence or absence of the ability to symbiotically fix nitrogen as specified in Werner *et al*.[@b36]; see the original source reference list on figshare[@b37] for all references related to every species used in this study. Global introduced status data ----------------------------- For each legume species found in the nitrogen fixation database, we searched the International Legume Database and Information Service (ILDIS)[@b13] and extracted geographic distribution information using a webscraper written in R[@b38]. The ILDIS geographic data was compiled by experts who synthesized regional floristic data from the primary literature. Because ILDIS data are a synthesis of recorded locations of living observations and herbarium records by flora experts, they likely encapsulate established species in a given region. In total, 3,973 legume species were found in ILDIS (species not found in ILDIS were discarded from the analyses) that matched the nitrogen-fixation trait database. Species distribution data in ILDIS is coded using the names of hierarchically structured geographic regions (i.e., continent, region, area, and country where available), and indicates whether each region is native, introduced, or unknown, thus capturing dispersal events at both regional and continental scales. We scraped geographic data at all available hierarchies and excluded areas where the introduced status was considered unknown. The geographic names in ILDIS were based on the World Geographical Scheme for Recording Plant Distributions developed by the Taxonomic Database Working Group (TDWG)[@b39]. We eliminated species records from our dataset just containing 'unknown\' regions, giving a total sample size of 3,530 species. The final dataset used in this study contained 317 non-fixing legumes out of 3,530 (9%), whereas the full Werner *et al*.[@b36] database contained 482 non-fixing legumes out of a total 5,427 total legumes (8.9%); therefore, our dataset showed no bias with respect to the proportion of non-fixers relative to all known data on legume nitrogen fixation. To convert the geographic names in the ILDIS database into usable geographic coordinate data, we downloaded a shapefile containing the standardized TDWG geographic regions as polygons[@b40], then matched these polygons to ILDIS geographic names. Where TDWG polygons and ILDIS geographic names could not be matched, we used the next available polygon in the geographic hierarchy (for example, if we could not find a polygon corresponding to an area name, we used the region name instead). Moving up to the next geographic level was only necessary for less than 10% of recorded regions and did not exceed one level. Once all geographic areas were matched to polygons, we only retained those at the lowest available hierarchical scale. Before analysis we merged any species range polygons that were touching each other and had the same introduction status, to prevent biases in the number of ranges due to finer subdivision within some areas. This way, all final polygons represent non-contiguous ranges. We checked the accuracy of the polygon occurrences by comparing our polygon data to occurrence records in the Global Biological Information Facility (GBIF)[@b41]. GBIF gives higher resolution point occurrence records, but for far fewer species (1,830 species) and invasive or introduced status is not recorded for each GBIF record. We found that, on average, ILDIS polygons for each species captured 93% of GBIF points (see [Supplementary Fig. 2](#S1){ref-type="supplementary-material"} for some example species maps). For points that fell outside ILDIS polygons, we calculated the geographic distance to the nearest ILDIS polygon and found that most points were geographically very close to an ILDIS polygon, with no obvious bias in the distribution of geographic distances between symbiotic and non-symbiotic legumes ([Supplementary Fig. 3](#S1){ref-type="supplementary-material"}). There was no obvious differences in the presence or number of 'unknown\' introduction status polygons between symbiotic and non-symbiotic species ([Supplementary Fig. 4](#S1){ref-type="supplementary-material"}), indicating that any ambiguities in polygon status was not different between our legume comparison groups. Together, these indicate that ILDIS geographic range data was reliable. Other species trait data ------------------------ We also scraped plant life-form (woody or not woody), life-history (annual or perennial), and information on human uses from ILDIS, as previous invasion studies have found these to be important factors in predicting legume invasion success[@b15]. We were able to obtain plant life form for 3,500 legume species and life-history for 3,462 legume species. We converted life form and history data into two binary traits by coding life form as a 1 for species that were woody (trees or shrubs), and as 0 for non-woody (herbs). Likewise, for life history, species that had an annual life history were assigned a value of 1, and perennial species assigned a 0. Life history and life form data was unavailable for ∼500 species, which would lead to a fairly large reduction in our sample size when including this data as covariates. To maintain full power in our models (see next section for model details), while still accounting for the potentially confounding effects of life form and life history, we imputed the missing values in these traits. We did this using a simple taxonomic imputation. If there were other species in the same genus as a missing species, its value was assigned to be the mean of the life form or life history values for that genus (for example, a value of 0.9 for life form would be assigned to a species in a genus with 90% woody species). If the data were missing for an entire genus, we used the mean of all species found in the same tribe in the same manner. Therefore, the life form and life history variables can be interpreted as the probability that a species is woody or annual respectively, based on their taxonomic group. 83 and 84.6% of missing species were filled at the genus level, for life form and life history respectively, and the remaining missing species at the tribe level. Some genera contained a mixture of either trait value, but 87.5 and 91.2% of genera could be coded greater than 0.75 or less than 0.25 (for example, more than 75% of the genus was one trait or the other) for life-form and life-history respectively. Most genera that contained species with missing data were entirely of one life form (73%) or life history (77%) and could be coded unambiguously as 0 or 1 based on their genus grouping. We repeated our main analysis with two other trait imputation methods (see [Supplementary Note 3](#S1){ref-type="supplementary-material"}) and our results did not change qualitatively, with all model coefficients changing only superficially, and no change in levels of significance for any factor, indicating that our results are robust to several methods of imputation. Therefore, only the results using the first method described above (that is, taxonomic mean imputation) are reported. Human use data was recorded in ILDIS by specifying whether a species was known to have a use in any of 11 different use categories (Chemical products, Domestic, Environmental, Fibre, Food and Drink, Forage, Medicine, Miscellaneous, Toxins, Weed or Wood). If none of these categories was specified in ILDIS, we assumed the species had no known uses. We calculated a human use covariate by counting the number of known human use categories for each species to create a value which could range from 0 to 9 (no species in our study had all 11 use categories), which we refer to here as 'number of human uses\'. Statistical analysis -------------------- We modelled the prevalence of successfully introduced species in regions across the world using a generalised linear mixed model (GLMM). Under the TDWG scheme, there are four nested levels of geographic range specification, from smallest to largest: the country, area, region, and continent level (though the country level does not necessarily always correspond to political countries). In our data, after translating from ILDIS to TDWG, geographic range was determined to different degrees of resolution, depending on the species. Some but not all species were specified at the TDWG area level, for example. To make all species comparable, we analysed introduced ranges on a single level. All non-native ranges were specified to at least the TDWG region level or below, so we used this as our focal geographic unit for the range during our analysis. Henceforth, we will refer to what TDWG calls region level simply as 'regions\'. There were 51 regions in total (see [Supplementary Fig. 6](#S1){ref-type="supplementary-material"} for a map of the regions used in this part of the analysis). Our response data therefore is made up of a vector of zeroes and ones *y*~*ij*~, which could be arranged into a matrix of *n*~species~ rows, and *n*~region~ columns *Y*~*ij*~ containing a one if species *i* is found non-natively in region *j* and a zero if it is not (e.g., the species is coded as one if at least one of its non-native polygons fell in the region). We were interested in testing whether symbiosis affects non-native prevalence across the globe, while controlling for several potentially biasing factors. Our model is the following: The non-native presence of a species *i* in region *j* is modelled as a realization of a binomial process on the probability of species *i* in region *j*, *P*~*ij*~: The probability of species *i* in region *j* is a function of the symbiosis status of species *i* (*SS*~*i*~; equals 1 if symbiotic, 0 if non-symbiotic), a number of potential covariates (*x*~*ik*~ and *x*~*jk*~), and random effects for species (SP\[*i*\]) and region (RE\[*j*\]): Where *α* is an intercept term, *β*~SS~ is the fixed effect coefficient determining the effect of symbiosis, *β*~*k*~ is the fixed effect coefficient determining the effect of species-level covariate *k*, *β*~*z*~ is the fixed effect coefficient determining the effect of region-level covariate *z*, and *V*~species~ and *V*~region~ are the variance parameters for the species and region random effects, respectively. We also initially included the TDWG continent level region as a higher level random effect (within which region was nested), however, we removed it in our final analysis as it explained almost no variation in the model (that is, variance parameter was very close to zero). This mixed effects model with crossed random effects has a number of advantages over a simpler species-level analysis. First, it allows the inclusion of both region-level as well as species-level covariates. Second, the random effect for region accounts for spatial non-independence within regions of the world. In a species-level only analysis, we would not be able to say if our results were driven just by one or a few regions across the globe, whereas with the full mixed model, our inferences are applicable globally. Species-level covariates (*x*~*k*~) included in the model were: the absolute latitude of the centroid of a species\' native range polygons, the total area of the species\' native range polygons, the species\' two binary life history traits (woody or not woody, and annual or perennial), and the number of human uses of the species according to ILDIS. We also included a symbiosis by number of human uses interaction, because we hypothesized that the number of human uses would reflect the probability of a species being deliberately introduced (as opposed to unintentionally), and this may affect the strength of any biological factors on introduction probability. We included one region level covariate (*x*~*z*~): the area of the introduced regions. This was to control for the possibility that larger areas may be more likely to have more introduced species simply due to a sampling effect. To fit the model, we used the lme4 package in R[@b42]. When fitting the model, all continuous covariates were mean centred (subtracted the mean such that zero corresponds to the mean) and scaled by the standard deviation, except for the number of human uses, for which zero is a biologically meaningful value, corresponding to the state at which deliberate introduction attempts should be lowest, and thus acting as the best reference point at which to evaluate other effects (see Frasier[@b16] for useful discussion). We ran two versions of the above model. The first model included all data on all species. Given the excess number of zeroes present in our analysis (that is, ∼78% species only occur natively), we ran a second model only on the species occurring in at least one non-native region to confirm similar results when zeroes were removed from the dataset. All response variables were analysed in R[@b38] and included the symbiosis trait, latitude of origin, total native area, plant life-form (woody or not woody), plant life-history (annual or perennial), number of human uses, the interaction between symbiosis and number of human uses, and the area of the introduced region as predictors. We calculated the correlation between all of our species-level model predictors ([Supplementary Fig. 5](#S1){ref-type="supplementary-material"}) and the highest correlation occurred between being woody and annual in our first (r=−0.49) and second (*r*=−0.59) model ([Supplementary Fig. 5](#S1){ref-type="supplementary-material"}). Testing the model effects ------------------------- We tested whether symbiosis and covariates were significant predictors of the prevalence of successful species introductions using parametric bootstrapping. We simulated 1,000 new response vectors (*y*~*ij*~) from the fitted model, using observed values of the fixed effect variables, and fixing species and region random effects at their estimated values. For each bootstrapped response vector we refit the same model to it and collected the fixed effect coefficients. We then calculated the 95% confidence intervals by determining the 0.025 and 0.975 quantiles of each coefficient\'s bootstrapped sample ([Table 1](#t1){ref-type="table"}). A fixed effect was classified as significant if its 95% confidence interval did not overlap zero. We also calculated 99 and 99.9% confidence intervals ([Table 1](#t1){ref-type="table"}). Visualising the results ----------------------- To translate the model results into a set of more intuitive measures for display, we again used parametric bootstrapping. To show the effect of symbiosis on the prevalence of successful introduced ranges, after controlling for all covariates, we simulated 1,000 response vectors from the fitted model, but this time setting all covariates to a value of zero (symbiosis remained at its observed values). This procedure removes the variation explained by the covariates in a way analogous to least square means in a standard statistical analysis. We took these 1,000 sampled response vectors and calculated several summary statistics for plotting. For each bootstrap sample, we calculated the mean number of introduced ranges for symbiotic and non-symbiotic species. We then plotted the mean and 95% confidence intervals of these values based on the bootstrap samples ([Fig. 2](#f2){ref-type="fig"}). Data availability ----------------- The full data set, including cleaned up ILDIS data, nitrogen-fixation data, and all covariates, is available from the authors on request. All data in their original form are available from public repositories (see Methods). Additional information ====================== **How to cite this article:** Simonsen, A. K. *et al*. Symbiosis limits establishment of legumes outside their native range at a global scale. *Nat. Commun.* **8,** 14790 doi: 10.1038/ncomms14790 (2017). **Publisher\'s note:** Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations. Supplementary Material {#S1} ====================== ###### Supplementary Information Supplementary Figures, Supplementary Tables, Supplementary Notes and Supplementary References We kindly thank the curators of the data sources used for this study who are fully listed and acknowledged in the Methods section. We also want to thank Mathew Hill and Kylie Ireland for manuscript comments. The authors declare no competing financial interests. **Author contributions** A.K.S. conceived of the study design. R.D. contributed data. A.K.S. and R.D. analysed the data. A.K.S. wrote the manuscript. All authors discussed the analyses, results and commented on the manuscript. ![A visual representation of the network of successful legume introductions.\ (**a**) Non-symbiotic and (**b**) symbiotic legume species. To facilitate visual interpretation of global network patterns, each species was assigned a single native point (coloured in blue), drawn randomly from its native range, and one or more non-native points (coloured in orange) drawn randomly from each of its non-contiguous non-native ranges. Non-contiguous ranges were defined by merging all polygons whose distance was less than 5 degrees Latitude-Longitude from each other. Connecting light lines between corresponding native and non-native ranges for each species indicate that legume species have successfully established into novel regions, continents and islands. Note: Lines do not necessarily represent actual dispersal pathways, as some non-native ranges may have been colonized from an intermediate non-native range, rather than directly from the native range.](ncomms14790-f1){#f1} ![Non-native ranges between symbiotic and non-symbiotic legumes species.\ (**a**) Mean number of introduced ranges across all legume species studied (including those with no introduced ranges) \[(*n*~total~=180,030=(*n*~species~=3,530) × (n~regions~=51)\]. (**b**) Mean number of introduced ranges for legume species recorded from at least one non-native region \[(*n*~total~=41,412=(*n*~species~=812) × (*n*~regions~=51)\]. A species\' introduced range is defined by a list of geographic regions of non-native occurrence. Points and error bars represent the mean and 95% confidence intervals from parametric bootstraps, controlling for all covariates (absolute native latitude, total native area, life form, life history, area of non-native region and number of human uses).](ncomms14790-f2){#f2} ![Global proportional distribution of symbiotic legume species.\ Regions are coloured according to the proportion of symbiotic legume species in (**a**) native and (**b**) non-native ranges. Lighter colours indicate higher proportions of non-symbiotic legume species. Non-symbiotic legume species tend to primarily occur near the equator in their native range. Non-symbiotic legume species currently account for a higher proportion of species within introduced ranges compared to their proportion within native ranges. The figure shows that the increased spread of non-symbiotic legumes spans multiple continents and islands across the world. Grey areas indicate terrestrial ecoregions where legumes are not known to occur[@b43]. Regions are defined using the Taxonomic Distribution Working Group system[@b39].](ncomms14790-f3){#f3} ![The interaction between symbiosis and human uses.\ The size of the symbiosis effect on successful introductions at different numbers of human uses, using the full dataset. Dots represent the difference in the predicted number of non-native ranges between non-symbiotic and symbiotic species, standardised by dividing by the predicted number of non-native ranges for non-symbiotic species. The standardisation controls for the differences in the predicted number of non-native ranges between different human use levels (determined by the main effect of number of human uses), and makes the interaction easier to visualize. Error bars represent the 95% confidence interval obtained through parametric bootstrapping. The size of the dots is proportional to the number of species in the dataset with that number of human uses, showing that most species had no uses recorded in the dataset (∼70%). The dotted vertical line represents the mean number of human uses across all species in the dataset (0.77). The x-axis is on a square root scale. Negative values mean the symbiotic species are predicted to have a lower prevalence of non-native ranges relative to non-symbiotic species. Apparent non-linearity is due to logit back-transformation.](ncomms14790-f4){#f4} ###### Introduction success as predicted by the symbiosis trait. **Factor** **All species** **Non-native species Only** ------------------------------------- ----------------------------------- ----------------------------- -------- ----------------------------------- -------- -------- Intercept −8.055 --- --- −3.125 --- --- Symbiosis? −0.523[†](#t1-fn3){ref-type="fn"} −0.960 −0.437 −0.587[†](#t1-fn3){ref-type="fn"} −0.832 −0.416 Latitude 0.142[†](#t1-fn3){ref-type="fn"} 0.094 0.210 0.026 −0.013 0.063 Total native area 0.194[†](#t1-fn3){ref-type="fn"} 0.119 0.211 −0.058[†](#t1-fn3){ref-type="fn"} −0.092 −0.038 Annual? 1.092[†](#t1-fn3){ref-type="fn"} 0.915 1.267 0.198[†](#t1-fn3){ref-type="fn"} 0.065 0.329 Woody? 0.353[‡](#t1-fn4){ref-type="fn"} 0.084 0.404 −0.476[†](#t1-fn3){ref-type="fn"} −0.634 −0.408 Number of human uses 0.964[†](#t1-fn3){ref-type="fn"} 0.865 0.981 0.323[†](#t1-fn3){ref-type="fn"} 0.282 0.370 Area of introduced region 0.010 −0.049 0.046 0.019 −0.046 0.051 Symbiosis by human uses interaction 0.152[†](#t1-fn3){ref-type="fn"} 0.104 0.223 0.080[†](#t1-fn3){ref-type="fn"} 0.042 0.129 CI, 95% confidence interval. Symbiosis is incorporated into the model as the presence or absence of the trait, with the inclusion of other factors found to predict introductions in our legume dataset. A negative coefficient indicates lower introduction success for symbiotic legumes compared with non-symbiotic legumes. We excluded non-significant interaction terms. 95% confidence intervals were obtained from parametric bootstrapping. Each response variable is modelled at the species by region level, and the model included a species and a region random effect to account for non-independence of observations within species or regions. The estimated variance for the species and region random effects respectively were 4.83 and 0.85 for the all species model, and 0.9 and 1.43 for the non-native species only model. ^†^99.9% CI does not overlap zero. ^‡^99% CI does not overlap zero. [^1]: These authors contributed equally to this work.
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General Multicarrier System A multicarrier system described herein indicates that one or more individual carriers are used as a group. FIGS. 1(A) and 1(B) show a signal transmission and reception method based upon a multiband radio frequency (RF). For efficient use of multiband (or multicarrier), a technique has been proposed in which one medium access control (MAC) entity handles multiple carriers (e.g., several frequency allocation (FA)). As shown in FIG. 1, one MAC layer in each of a transmitting end and a receiving end may manage several carriers for efficient multicarrier use. Here, for effective transmission and reception of the multicarrier, it is assumed that both the transmitting and receiving ends can transmit and receive multicarrier. Since frequency carriers (FCs) managed by one MAC layer do not have to be contiguous to one another, it may be flexible in view of resource management. That is, a contiguous aggregation and a non-contiguous aggregation are all available. Referring to FIGS. 1(a) and 1(b), PHY0, PHY1, . . . , PHY n−2, PHY n−1 denote multiband according to this technique, and each band may have a magnitude (bandwidth) of FA assigned for a specific service according to a predefined frequency policy. For example, PHY0 (RF carrier 0) may have a bandwidth of FA assigned for a typical FM radio broadcast, and PHY1 (RF carrier 1) may have a bandwidth of FA assigned for cellular phone communications. Each frequency band may have a different frequency bandwidth according to each frequency band characteristic. However, it may be assumed in the following description, for the sake of brief explanation, that each FA has A [MHz] magnitude. Also, each FA may be represented as a carrier frequency for using a baseband signal at each frequency band. Hereinafter, each FA is referred to as “carrier frequency band”or, if not ambiguous, simply as “carrier” representing each carrier frequency band. As shown in 3GPP LTE-A in recent time, to distinguish the carrier from a subcarrier used in a multicarrier technique, the carrier may be referred to as “component carrier.” In this regard, the “multiband” technique may be referred to as “multicarrier” technique or “carrier aggregation” technique. In order to send signals via multiband as shown in FIG. 1(a) and receive signals via the multiband as shown in FIG. 1(b), the transmitting and receiving ends are required to include RF modules, respectively, for transmission and reception of signals over the multiband. Also, in FIG. 1, the configuration of “MAC” may be decided by a base station regardless of downlink (DL) and uplink (UL). Briefly explaining, this technique indicates that one MAC entity (hereinafter, simply referred to as “MAC” if not obscure) manages/runs a plurality of RF carriers (radio frequencies) for signal transmission and reception. Also, the RF carriers managed by the one MAC may not have to be continuous to each other. Hence, in accordance with this technique, it is more flexible in view of resource management. In IEEE 802.16m system as one of wireless communication systems, the carriers may be divided into two carrier types from the perspective of a base station. For example, the carrier types may be divided into a fully configured carrier type (FCCT) and a partially configured carrier type (PCCT). The FCCT indicates a carrier by which every control information and data can be sent or received, and the PCCT indicates a carrier by which only downlink (DL) data can be sent or received. Here, the PCCT may be used for services, such as an enhanced multicast broadcast service (E-MBS), which usually provides DL data. From the perspective of a mobile terminal, assigned carriers may be divided into two types, for example, a primary carrier type and a secondary carrier type. Here, the mobile terminal may be allocated with one primary carrier and a plurality of sub-carriers from the base station. The primary carrier may be selected from the fully configured carriers. Most of essential control information related to the mobile terminal may be sent on the primary carrier. The subcarriers may be selected from the fully configured carriers or the partially configured carriers, and also additionally allocated in response to request of the mobile terminal or instruction of the base station. The mobile terminal may send and receive not only every control information but also control information related to the subcarriers over the primary carrier, and exchange (transceive) data with the base station over the subcarriers. Here, the subcarrier, as a fully configured carrier, allocated to a specific mobile terminal, may be set to a primary carrier of another mobile terminal. Multicarrier Switching Multicarrier switching indicates a multicarrier mode for a terminal to switch a physical layer connection from a primary carrier to a partially configured subcarrier or a fully configured subcarrier. Here, the carrier switching of the terminal may be performed based upon instruction (indication) from a base station in order to receive E-MBS service at a subcarrier. After being connected to the subcarrier for a specific time, the terminal may come back to the primary carrier. While the terminal is connected to the subcarrier for the specific time, the terminal does not have to maintain transmission or reception via the primary carrier. Basic Multicarrier (MC) Mode A basic multicarrier (MC) mode indicates a mode that a terminal operates using only one carrier. However, the terminal may support not only optimized scanning for carriers related to a multicarrier operation but also a primary carrier switching procedure. Carrier Switching Operation for E-MBS Service E-MBS service may be performed by a specific carrier (e.g., subcarrier) other than a primary carrier. In a connected state with a base station, an E-MBS terminal having only one transceiver (i.e., a terminal operating in a carrier switching mode) may perform carrier switching from a primary carrier to another carrier to receive E-MBS data burst, E-MBS configuration message and E-MBS MAP, and carrier switching from the another carrier to the primary carrier to receive a unicast service from the base station. The E-MBS terminal may perform a carrier switching operation based upon its E-MBS subscription information assigned from the base station to the terminal during a dynamic service addition (DSA) procedure. The E-MBS subscription information may be MSTIDs and FIDs, for example. In an actual E-MBS environment, basic (default) E-MBS channels may be assigned (allocated) to every terminals subscribed in the E-MBS service, and the number of default E-MBS channels may be much more than the number of specific E-MBS channels (e.g., premium channels). all the E-MBS terminals subscribe in all the default contents via default free channels. Additionally, some premium users may subscribe in premium contents. In other words, E-MBS terminals subscribed in the premium contents may stay longer in the E-MBS carrier than terminals merely subscribed in the default contents. FIG. 2 is a flowchart showing a carrier switching operation performed based upon terminal subscription information. As shown in FIG. 2, it is assumed that a terminal 1 merely subscribed in default contents and a terminal 2 subscribed in the default contents and a premium content 2. It is also assumed that E-MBS data bursts 1 and 3 are data for the default contents, E-MBS data burst 2 is data for a premium content 1, and E-MBS data bursts 4 and 5 are data for the premium content 2. Referring to FIG. 2, the terminal 1 may stay at a primary carrier while a base station sends E-MBS data bursts 2, 4 and 5 (S201), and the terminal 2 may stay at a primary carrier while the base station sends E-MBS data burst 2 (S202). That is, the base station may allocate unicast resources to terminals, which have subscribed in the premium contents having the lowest unicast scheduling efficiency. During free E-MBS service, a terminal may not need to perform a joining/leaving process at an upper layer. That is, in this case, when E-MBS terminal starts or ends E-MBS service reception, DSA/dynamic service deletion (DSD) process may not be performed. However, in the carrier switching mode, the base station must be known of whether a terminal is receiving the E-MBS service for efficient unicast scheduling. If the terminal is not receiving the E-MBS service, the base station may provide the unicast service to the terminal at the primary carrier at any time.
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Hydrogen is an important feedstock in the manufacture of ammonia, methanol, and a variety of other chemicals; but its largest market is the crude oil processing industry. In crude oil refineries, hydrogen is used in a number of processes including hydrodesulfurization where hydrogen is reacted with sulfur containing compounds over a catalyst to form hydrogen sulfide. Hydrogen sulfide itself is already produced in great quantities during the drilling and processing of natural gas and oil. A process that can economically extract hydrogen from low value feedstocks or wastes such as hydrogen sulfide would bring tremendous benefits to the petroleum sector as this sector consumes large amounts of hydrogen. Many processes exist for the production of hydrogen. The production of hydrogen is currently dominated by the steam reforming process where a relatively light hydrocarbon is reacted with steam inside a bed of reforming catalyst, usually nickel. Since steam reforming of hydrocarbon is endothermic, the energy to drive the reactions must be provided from an external source. In the steam reforming process, the hydrocarbon-containing stream must be free of sulfur or other contaminants such as carbon particles that can poison and deactivate the catalyst. Another hydrogen production method is partial oxidation. In a partial oxidation reaction, a hydrogen-containing feed is reacted with an oxidizer, such as oxygen or air, in substoichiometric proportion normally referred to as a rich mixture where the equivalence ratio spans from one 1 to the upper flammability limit of the fuel being utilized as the feedstock. The equivalence ratio, defined as the stoichiometric oxidizer to fuel ratio divided by the actual oxidizer to fuel ratio, is shown in equation R1. EquivalenceRatio = ( fuel Oxidizer ) actual / ( fuel Oxidizer ) stoichimetry R1 An equivalence ratio less than unity is considered lean, also referred to as fuel-lean, since a portion of the oxidizer is leftover after all of the fuel is consumed by the oxidation reaction. Where the fuel content of the mixture lies below the lower flammability limit of the fuel used as the feedstock, the fuel and oxidizer mixture is considered ultra-lean. Conversely, fuel and oxidizer mixtures of equivalence ratio greater than unity are considered rich, also referred to as fuel-rich, since a portion of the fuel is leftover after the oxidation reaction is complete. Mixtures of equivalence ratios greater than rich mixtures, normally taken to be higher than the upper flammability limit of the fuel being utilized as the feedstock, are considered ultra-rich. Ultra-rich mixtures do not normally produce self-sustained flames without the aid of external energy sources or preheating the mixture. Although the partial oxidation process does not need an external source of heat since it is exothermic, it is still less common than steam reforming since it is generally less efficient than steam reforming particularly at large scale. As a normally non-catalytic process, partial oxidation can utilize any hydrocarbon feeds. The steam reforming and partial oxidation processes can be combined into a single process normally referred to as an autothermal process. In the autothermal process, the energy for the reforming reactions is provided by oxidizing a small portion of the fuel inside the bed of a reforming catalyst. Due to its catalytic nature, the autothermal process falls under the same constraints as the steam reforming process in that the catalyst bed is susceptible to poisoning and deactivation by sulfur, carbon, and other poisons in the feed stream. The hydrocarbon stream must be desulfurized in a first step prior to entering the autothermal reactor. During reforming, whether by the steam reforming or autothermal process, water must be provided in excess of the stoichiometric quantity to prevent carbon formation. Additionally, excessive temperature must be prevented in the reactions to avoid sintering the reforming catalyst. Steam reforming, partial oxidation, and the autothermal process are well known methods in the industry that are practiced on industrial scales. The invention disclosed herein can be an economical process for producing hydrogen from hydrocarbons and various other hydrogen containing fuels. U.S. Pat. No. 6,517,771 to Li, incorporated herein by reference, disclosed a reverse flow inert porous media reactor for the purpose of heat-treating metals. Li limited the reactant stream to methane and oxygen or air, and the preheater to initiate the process is located inside the porous bed. Drayton et. al 27th, International Symposium on Combustion, 27, pp. 1361-1367, 1998, incorporated herein by reference, disclosed an application of the reverse flow reactor for fuel reforming, producing synthetic gas from methane in a reactor similar to Li's. None of the disclosed references above include an external energy source for the reverse flow reactor or are applied to the reformation of hydrogen sulfide. A number of studies in reverse flow inert porous media reactors are carried out in applications not intended for hydrogen production from hydrocarbons. Hoffman et al, Combustion and Flame, 111, pp. 32-46, 1997, incorporated herein by reference, operated a reverse flow reactor with ultra-lean air and methane mixtures for the purpose of heating fluids. Barcellos et. al. Clean Air 2003, Seventh International Conference on Energy for a Clean Environment; Lisbon, Portugal, Jul. 7-10, 2003, incorporated herein by reference, tested a reactor similar to Hoffman's for the production of saturated steam through heat exchangers protruding directly through the inert porous media and fitted at the extremities of the reactor. Production of hydrogen from both light and heavy hydrocarbons as well as other hydrogen containing wastes such as hydrogen sulfide is not addressed in the prior art. Hydrogen is a much more valuable commodity then sulfur. A process that can economically recover the hydrogen as well as other compounds could have significant impact on the petroleum and other industries. The reformation of hydrogen sulfide (H2S) to hydrogen and sulfur presents certain challenges not encountered in hydrocarbon reformation. For example, the low heat content of H2S precludes obtaining very high temperature in the partial oxidation regime. More importantly, H2S reforming requires the reaction to reach near equilibrium conditions at high temperature to obtain high yield. In the current invention, the intrinsic heat recuperating mechanism of the inert porous media matrix and the reactor's ability to create an isothermal high temperature volume render it a cost effective option for the reformation of H2S and other hydrocarbons by providing the necessary residence time and temperature without the requirement of an external energy source to be used continuously throughout the reactions. Specifically, all of the reforming reactions in these above-mentioned prior art references occur inside a hollow chamber. None of these references disclose an apparatus and process where the reaction zone may be located in any portion of a reactor chamber, where the reaction zone is allowed to freely propagate through the reactor chamber filled with a porous media matrix and where the reforming reactions occur directly in a heated inert porous media matrix, or packed bed. Therefore, there has developed a need for a reactor which can efficiently reform both hydrocarbon and hydrogen sulfide fuels to pure hydrogen while not requiring continuous external energy to produce a viable hydrogen yield.
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La Guajira Desert The La Guajira Desert is a desert located in northern Colombia and Venezuela, approximately north of Bogotá, covering most of the La Guajira Peninsula at the northernmost tip of South America. Most of the region is within Colombia's La Guajira Department, though a small portion is in Venezuelan territory. The area holds immense coal reserves which are exploited in a zone known as El Cerrejón. It is also home to the indigenous Wayuu people. The Wayuu are mostly herders but also master deep-sea divers, known for collecting pearls from the Caribbean Sea. The peninsula is populated chiefly by xeric scrubland, which is home to a large variety of flora and fauna. The National Natural Park of Macuira, established in 1977, is a tropical oasis located in the La Guajira Desert. The park covers in La Guajira’s only mountain chain and ranges in altitude from sea level to . It has a warm climate that averages about . References External links Category:Deserts of Colombia Category:Deserts of Venezuela Category:Geography of La Guajira Department
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Text entry is the first step of most uses of computers and there will always be a need to enter text faster. While many users of computers are familiar with keyboard operations, this cannot be assumed of the expanding new classes of users and this has created interest in alternative techniques for text entry, such as voice processing and handwriting recognition. But the problem of speed remains unresolved by these alternative techniques. Handwriting is slower than typing. A skilled typist can be expected to enter around 40 to 70 words per minute, but no voice recognition technique appears close to reaching it while this typing speed remains below the more than 100 words per minute of normal speech. Finally, the speed of speech is itself below the speed of reading--well beyond 200 words per minute--and we are known to recognize certain elements of text at far higher speeds, measured in thousands of words per minute. So the limitations of the speed of text entry contribute to the frustration of users of computers when there may be more than a factor of ten between the time it takes to form an idea and keying it into a computer. Many high-level users therefore consider the use of computers as too slow and, in particular, as slowing down the thought process. Several techniques have been tried in the past to accelerate text entry. These present techniques fall into the so-called categories of word-completion and macros. Word-completion Word-completion allows the user to type the initial letters of a word and let the computer system do the completion. A good example of word-completion was offered by the Spell key of the formula editor of a commercial spreadsheet called Javelin, released in 1984. When a Javelin user types a few letters and presses the Spell key, Javelin either completes the name or gives a list of possible names that match what was typed so far: If there is only one name that matches, completion is done automatically and the name is inserted; if two or more names match what was typed so far, Javelin displays a menu of possible choices. Selection of one of the menu choices is then done using cursors or a mouse, or by adding letters and pressing Spell again. Similar word-completion techniques have been offered in many other commercial software products, such as word-processors and spelling checkers, for at least the past ten years. An early example was the spelling checker included with Microsoft Word, a word processor released around 1983. The major drawback of word completion techniques comes from the fact that the root of a word (its first letters) is usually not a very good way to discriminate among several alternative words. For example, there are several hundred words starting with the root "con", and therefore any meaningful choice will require at least a fourth letter. Even with a fourth letter, there are more than a hundred words that start with "cont" or with "cons" and more than fifty that start with "const". So in practice, the root has to be sufficiently long to reduce the number of possible choices to ten or less, a number small enough to allow easy selection. Consequently, word completion fails to achieve a significant reduction in the number of keystrokes. Several techniques have been proposed to overcome these limitations. For example, U.S. Pat. No. 4760528 offers a system of abbreviation based on the uses of abbreviated prefixes and suffixes. Similarly, U.S. Pat. No. 4893238 offers an abbreviation technique based on syllables. Neither these, nor other similar techniques based on strict abbreviation rules, have been very successful in practice. Both patents claim to achieve a reduction in the number of keystrokes entered that is in the range of 1.3 to 1.4. But most potential users consider this reduction to be insufficient to justify learning a set of strict abbreviation rule. To achieve a higher reduction payoff requires other techniques and, in particular, it requires using abbreviations for phrases, not just for words, a domain addressed mostly with macros in the past. Macros Macros are an even older concept, first published in 1958 by Christopher Stratchey. With macros, a user can define abbreviations for certain (usually long) phrases or words, type the abbreviation and request its expansion with a special key. For example, the abbreviation "dj" may be defined for "Dow Jones Industrial Average" and then typing the two letters "dj" followed by the special key has the effect of expanding the abbreviation, that is, of replacing it by the corresponding text. Commercial products offering this kind of macro capability appeared very early on microcomputers. Prokey, released in 1983, is an early example of such products. Similar macro capabilities were also incorporated in early versions of word-processors such as Microsoft Word (1983) and XyWrite. The names used for these facilities vary widely with the products and so do the special keys used for requesting expansion. Prokey allowed the user to select which key to use for expansion. A number of recent products use a single space as the key for expansion. For example, this is done in the Windows version of Microsoft Word (1994), with the so-called Autocorrect feature: having defined the abbreviation "asap", it may be expanded into "as soon as possible" when a space is typed after the final letter of "asap". A similar facility is offered in XyWrite and in WordPerfect version 6.1. The above examples would suggest that macros have the potential to provide reduction factors higher than the 2 or 3 that is the minimum required to reach the speed of slow or moderate speech. But in practice the use of macros is severely limited by the difficulty of learning, remembering, and applying systematically such macros. So the facility tends to be used for a few favorite phrases--usually less than a hundred--, which means that its overall effect on input speed is only marginal. Both word-completion and macros fall short of offering a viable solution for fast text entry.
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Know EducationNow... Waiter or Waitress If you have charming personality and people skills then you can surely become waiter or waitress. Waiters and waitresses, also called servers, are responsible for ensuring that customers have a satisfying dining experience. The specific duties of servers vary considerably with the establishment in which they work. Prepare itemized checks and hand them to customers and sometimes take payment Clean and set up dining areas, refill condiments, roll silverware, and stock service areas Skills of Waiter or Waitress Communication skills: Waiters and waitresses must listen carefully to customers’ specific requests, and relay the information they get from the customers to the kitchen staff, so that orders are prepared to the customers’ satisfaction.Customer and personal-service skills: Waiters and waitresses spend most of their work time serving customers. They should be friendly and polite and be able to develop a natural rapport with customers.Good memory: Waiters and waitresses must keep customers’ orders straight. They also should be able to recall the faces, names, and food and drink preferences of frequent customers.People skills: Waiters and waitresses must be courteous, tactful, and attentive as they deal with customers in all circumstances. Physical stamina: Waiters and waitresses must be able to spend hours on their feet carrying heavy trays, dishes, and glassware.Team oriented: Busy dining hours can be hectic and fast paced, workers must be able to work well as a team to ensure that customers feel welcome and receive prompt service.Well-groomed and neat appearance: Waiters and waitresses are the front line of customer service in food service and drinking establishments, a neat appearance is often important.
3.15625
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Assessment of lead exposure of children from K-XRF measurements of shed teeth. Lead is accumulated and immobilized for long periods of time in teeth. Thus the Pb concentration of a tooth can be used as an indicator of the cumulative Pb intake of a child. Shed and extracted teeth were collected from children in Beijing, China and some industrial regions in the Middle Urals in Russia. The Pb levels in the teeth were measured in Philadelphia, PA using an X-ray fluorescence (XRF) technique. Since Pb deposits in the tooth during the entire period that it is in the child, the measured tooth Pb level was divided by the age of the child when the tooth was shed and expressed in terms of (microgram/g-yr). 10% (n = 100) of the teeth from Beijing, China had Pb levels exceeding 5.5 and 3% above 9 micrograms/g-yr. For comparison, in the 1970s when urban environmental Pb levels were elevated, the tooth Pb levels in Philadelphia children were similar, i.e. 10% (n = 298) of the teeth had Pb levels exceeding 7.5 and 6% were above 9 micrograms/g-yr. Children in a more rural setting, Bennington, VT, had no detectable tooth Pb (n = 200). The Pb levels in the teeth from the Urals were much higher; 50% (n = 134) of the teeth had Pb levels exceeding 7.5 and 10% exceeding 17.8 micrograms/g-yr. The tooth Pb levels observed in the teeth from Beijing, and more so from the Urals, indicate that these children are residing in Pb polluted environments. Further studies are required to determine the extent of the Pb pollution and to explore the possibility that there are associated Pb-related health deficits.
3.03125
3
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Miranda warnings are essential On March 1, 1966, the case of Miranda v. Arizona was argued in the Supreme Court, and was decided on June 13, 1966. The issue was that prior to the time of arrest and any interrogation of a person suspected of a crime, he/she must be told that he/she has: “the right to remain silent, the right to legal counsel, and the right to be told that anything he/she says can be used in court against” him/her. Also, if the accused person confesses to the authorities, the prosecution must prove to the judge that the defendant was informed of them and knowingly waived those rights, before the confession can be introduced in the defendant’s criminal trial. The warnings are known as Miranda Rights. Although there are crusades against Miranda rights suggesting that it significantly harmed law enforcement efforts in this country. The Miranda rights have its advantages and should remain its continuum because of ample amount of false convictions and to stop abuse of power. Many argue that the cost of Miranda rights outweighs the benefits. Advocates of letting Miranda go, main arguments are over the number of lost confessions. To them it’s the belief that fewer people will confess if police warn them of their right to silence. Advocates would say that this procedure allows dangerous criminals back into the street. But, based on small percentages, it has been argued that Miranda rights have had only a minimal effect on law enforcement. This warning statement has been in place for years and has been met with extreme success. “It revolutionized criminal interrogations and was part of a larger revolution in the nature of both the Supreme Court and the federal system generally.” This decision took power out of the hands of law officials and placed it in the hands of judges. Before confessions were being obtained by coercion and police brutality. “What has proven to be a problem is the exclusionary rule feature of Miranda. That is the feature that throws out perfectly voluntary confession” Paul Cassell. It’s odd that this controversy has even arisen, because the Miranda Rights works for both sides. It gives the police a clear set of rules to follow. It makes it easier to admit confessions at trial, as long as the police obey the rules. It is fair to defendants because it informs them of their rights. It protects the basic fifth amendment right against self- incrimination. Miranda rights in the twentieth century has reduced police misconduct, preserved our independence, avoid false confessions and just overall is fair. It is the belief that these rights are of the utmost importance to every American citizen. We must decide on the constitutionality of these rights as critics of the constitution as well as people who may be affected by our own decisions. They must do a more thorough job so as to avoid unnecessary pain and disruption to lives of people who may be falsely accused and to be absolutely sure that they have the right person in custody. Not being aware of your rights is like being thrown into the driver’s seat of a car having no idea as to which pedal is the accelerator and which is the brake. The problem with this way of thinking is that these people are not just suspects in a crime; they are people and should be treated as such. Miranda warnings are a safety net. Here, the court ruled that suspects have the right to remain silent and that prosecutors may not use statements made by suspects in police custody, unless they have been informed of their rights first. These advisements have kept innocent people out of prison and therefore not only saved the lives and futures of those people and their families but also saved this country a significant amount of money that can be put to use elsewhere. There are laws that 90% of the country is unaware of. The Supreme Court is now in the process of hearing arguments, and reviewing cases to decide if the Miranda rights are really constitutional, and therefore, enforceable. Some believe that it is not required to recite this warning when a suspect is arrested, rather it is required when and if the police decide to interrogate the suspect. It is the privilege of that suspect to either wave these rights or to remain silent and request that a lawyer be present at all times. The consequences were seen in Smith v. Illinois in which Smith was arrested for armed robbery, he was taken to an interrogation room and read his rights under Miranda v. Arizona. When officials asked whether he understood his right to a lawyer and to have a lawyer present during the questioning, he replied: “Uh, yeah. I’d like to do that.” However, rather than stop the interrogation to meet Smiths request, the interrogating officers continued the interrogation; ultimately, he made incriminating statements. Smith’s motion to suppress the statements was denied, and he was convicted of armed robbery. His conviction was affirmed by both the Illinois Appellate Court and the Illinois Supreme Court, which held that his responses to continued police questioning made his initial request for a lawyer ambiguous and that the officers therefore were not required to terminate their questioning. Once Smith clearly stated he did want a lawyer all other questions shouldn’t have been asked afterward. This case brings up a strong point that not enough suspects use their right to cut off questioning after it has begun. This in fact is an important Miranda decision. Despite the fact that some people argue against it, in many others view It serves its purpose and we should also be reminded that the Miranda rights prevents self-incrimination in violation of the Fifth Amendment to the U. S. Constitution Plagiarism Warning: Essays from FreeOnlineResearchPapers.com are for example ONLY. Do NOT submit papers from FreeOnlineResearchPapers.com as your own. If you choose to use information obtained from our essays, it is your responsibility to cite it. Free Online Research Papers is made possible by people like you submitting and commenting on research papers, research articles, book reviews, poetry, and creative writing pieces.
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Put that sandwich down, now. As if the link between carbohydrates and the muffin-top spilling over your waistband wasn't bad enough, new research indicates that a high-carbohydrate diet may also influence your cancer risk and the growth of tumours. Scientists at Canada's British Columbia Cancer Research Centre found that mice fed on a high-protein, low-carbohydrate diet had slower tumour cell growth than those fed a typical Western diet high in carbohydrates. While the experiments were conducted with mice, the findings appear to be strong enough to be applied to humans. High-carb diet ... delicious but deadly? "On the Western diet, half of the mice had tumours by middle age. On the low-carb diet, none of the mice had the tumours," said Dr Gerry Krystal, who authored the study along with colleague Dr Vincent Ho. The mice used were predisposed to breast cancer, and had a life expectancy of two years.
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Resource recovery operations on Earth require an economic feasibility with a financial return on the invested capital. The cost of transporting payloads to and from the moon is a barrier to economic development of the moon. Rocket propelled space vehicles transporting cargo outside the proximity of the Earth in airless space do not require the same vehicle hardware to push up through the atmosphere or land on the moon, but discarding the vehicle hardware on each mission like Apollo is still expensive. The space exploration initiative announced by President Bush and implemented by NASA has the opportunity to mature the transportation cycles beyond the Earth and the moon. The requirements and cost for each of these six lunar transportation cycles is different and the requirements for manned versus unmanned missions differs greatly. If one breaks out these different cycle or leg transportation requirements for each portion of a lunar trip, then six distinct transportation cycles emerge. As each cycle matures, it becomes more effective and efficient Commerce competitive forces help accelerate this maturing process and the evolution into a cost competitive transportation environment. The transportation cycles emerging are Earth to low Earth orbit or LEO, LEO to Lunar orbit “LO,” LO to the lunar surface, the lunar surface back to LO, LO to LEO and the re-entry from LEO to the Earth's surface. Placing a transportation node between each of the separate cycles would accelerate the maturing of the transportation process and facilitate introducing commerce. In a mature transportation cycles on Earth, we find that changing the requirements for a portion of a trip, like from water to land results in the change of a vehicle and results in a harbor emerging. Why not fly and eliminate the harbor? Well, people fly, eliminate the harbor and pay the extra cost, but most cargo goes a different less expensive route through the harbor. The airport becomes the transportation node for humans and the harbor is for cargo with very different costs related to transportation. Aircraft manufacturers want all humans and cargo to fly, but when paying for the transportation, the cost competitive aspects become important. In a remote site like the moon, the ratio of humans to cargo is significantly skewed. In looking at similar remote locations on Earth the ratio is less than 1% human and 99% cargo. To combine the manned and unmanned portions as we did in Apollo makes space transportation expensive, in part, because the safety and reliability of manned space flight is expensive. Such manned vehicles may be similar to the Saturn vehicle of the Apollo project, which landed the first man on the moon more than 30 years ago. The next series of exploration trips to the moon might consider separating unmanned cargo from humans in some manner consistent with safety. Rendezvousing, docking and transferring payloads between space vehicles was performed more than forty years ago in the Apollo program, and more recently between shuttles and the International Space Station. The Apollo program used a form of transportation node, for example, the astronauts had to transfer cargo from the lunar lander to the command module in lunar orbit. The command module in lunar orbit was a node in the transportation system and saved mass from being transported to and from the moon's surface. Today these transportation node techniques and procedures can be refined and used, for example, between each of the six transportation cycles and two of the nodes already exist, the Spaceports on Earth and the International Space Station. Travel between them has become partly commercial and will become competitive. In such conventional systems, the actual transfer of cargo is performed by people after docking of the vehicles and opening of a hatch, However, the automatic transfer of cargo between two vehicles in space, such as unmanned space vehicles, is a more complex operation, but possible by combining innovation with conventional systems. The enhancement of the transportation process to be more effective and more affordable can also happen. U.S. Patent Application Publication No. 2002/0079407 to Lounge et al. entitled, “Underway replenishment system for space vehicles” discloses a replenishment system used to deliver payloads and supplies to an orbiting receiving space vehicle using a tether. The 2002/0079407 application does not enhance the payload movement. The 2002/0079407 application discloses a method of transferring payloads between a delivering space vehicle and a receiving space vehicle, but falls short of a transportation node. U.S. Pat. No. 4,790,499, to Taylor, et at, describes docking with an orbital object using a tether. Docking with an object at the end of a cable is less likely to damage the orbital facility because both objects can move in rendezvous and docking operations. The '499 patent discloses a passive operations with no mention of active “seeker” tether tip operations.
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1. Technical Field The present invention relates generally to semiconductor memories and more specifically to controlling of wordline signals. 2. Background Art Microprocessors are used in many applications including personal computers and other electronic systems. A goal of any microprocessor is to process information quickly. One problem has been the communication rate between a microprocessor and main memory. The instructions to be executed by the microprocessor and the data on which operations implemented by the instructions are to be performed are stored at addresses within main memory. To access instructions and data, the microprocessor transmits addresses to main memory. The main memory decodes the address and makes the contents at the requested address available for reading and/or writing. The time required for the microprocessor to transmit an address to main memory and receive the respective contents therefrom can significantly constrain system performance. One technique, which is used to increase the speed with which the microprocessor processes information, is to provide the microprocessor with an architecture, which includes a fast local memory called a cache memory A cache memory is a small, fast memory that keeps copies of recently used data or instructions. When these items are reused, they can be accessed from the cache memory instead of main memory. Instead of operating at slower main memory access speeds, the microprocessor can operate at faster cache memory access speeds most of the time. In order to further increase performance, microprocessors have come to include more than one cache memory on the same semiconductor substrate as the microprocessor. The most commonly used cache memories use static random access memory (SRAM) circuitry, which provide high densities using wordlines and bitlines to access SRAM memory cells. However, in order to place as much memory on the microprocessor die as possible, SRAM circuitry requires minimal cell and read/write circuit architectures. To support minimal architectures, a memory cell is accessed by enabling a row wordline wire and enabling a selected column-gating transistor to read the value from the memory cell. The use of memory circuits in battery-operated and other low-voltage devices make it desirable to operate the memory circuits at lowest voltage possible. Typically, when read or write operations are done in memory arrays, the wordline is set high with the power applied while the information stored in the memory cells is read by being transferred onto bitlines or information on the bitlines is written by being stored in the memory cells. For read operations, bitlines are then read by a sense-amplifier, or sense-amp. Sense-amps are common to all memories whether the memories are dynamic, static, Flash, or other types of memories. For write operations, information on the bitlines change the held charge in the memory cell. While the wordline is kept on, power is being consumed. The wordline remains on during and after the desired operation, whether it is a read or a write, to ensure the operation is complete; i.e., power is consumed even when no longer required. Reading reliable results from memory circuits operating at a low-power supply voltage is complicated by the large capacitance of the wordlines and the threshold drop produced by the gating transistor. Low-power supply voltages reduce memory speed, and at very low voltages, the reliability of the information drops. To address the reliability problem, memory circuits, which have a bootstrapped boost voltage applied to the wordlines, have been developed. The row wordline is charged to a voltage that is higher than the power supply line. In addition, the row wordline is charged prior to accessing the memory location by switching on the column-gating transistor. Boost circuits provide reliable memory operation at low voltages. One of the problems with boost circuits is that at high voltages, the access circuitry is over-stressed. This limits the upper end of the power supply operating range of a memory device. Another problem is that boosting increases the power consumption of a memory circuit. At high supply voltages, the power dissipation can exceed tolerable levels and the memory circuitry is subject to failures due to overheating. Power saving has been a persistent need. Because low-power consumption is becoming even more important, it is desirable to provide a method and apparatus for operating a memory device in a manner that saves power. Furthermore, it is desirable to achieve reliable read and write operations at low voltages. With the urgency of increasing speed and saving power, solutions to these problems have been long sought but have long eluded those skilled in the art. The present invention provides a memory system, and method of operation therefor, having memory cells for containing data, bitlines for writing data in and reading data from the memory cells, and wordlines connected to the memory cells for causing the bitlines to write data in the memory cells in response to wordline signals. A decoder is connected to the wordlines for receiving and decoding address information in response to a clock signal and an address signal to select a wordline for a write to a memory cell. Latch circuitry is connected to the decoder and the wordlines. The latch circuitry is responsive to the clock signal for providing the wordline signal to the selected wordline for the write to the memory cell and for removing the wordline signal from the selected wordline when the write to the memory cell is complete. The memory system conserves power while permitting reliable read and write operations at low voltages. Certain embodiments of the invention have other advantages in addition to or in place of those mentioned above. The advantages will become apparent to those skilled in the art from a reading of the following detailed description when taken with reference to the accompanying drawings.
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Vacuum plasma generators can be an integral component of an alternating voltage gas discharge excitation arrangement that couples to a gas discharge device for treating a workpiece. Vacuum plasma generators can have different power classifications and different output signal forms. In vacuum glass coating, for example, medium frequency (MF) vacuum plasma generators are used that have an MF output signal with power levels of between 30 and 300 kW. The MF output signal is mostly a sinusoidal signal having frequencies of between 10 kHz and 200 kHz. The output voltages may be from several 100 V to above 1000 V. In order to ignite plasma in the gas discharge device, the output voltages of vacuum plasma generators are often much higher than during normal operation. In the plasma, brief and also longer-lasting spark-overs, so-called arcs, may occur, and such arcs are undesirable. An arc is generally identified by a break-up or a drop in the voltage at the vacuum plasma generator and an increase in the current at the vacuum plasma generator, for example, at the output of the vacuum plasma generator or at another location in the vacuum plasma generator. If an arc of this type is identified, it is extinguished or prevented from reaching a maximum level. For example, in DE 41 27 505 C2, the output of the alternating current generator is caused to short circuit when an arc is identified, which is a suitable method for low-power MF generators. The higher the power levels become, the higher the voltages and currents also become and a switch for short circuiting would have to be able to short circuit such higher currents. Components of such a switch are usually larger and more expensive to fabricate. In some cases, components of a short circuiting switch would be connected in series and/or in parallel in order to be able to switch off the high voltages and currents. When arcs occur, the MF generator should supply as little residual energy as possible into the gas discharge device. For example, in MF generators for Flat Panel Display (FPD) production, an arc may lead to pixel errors, and a single pixel error can have a significant influence on the quality of a large surface-area (for example, for 19″ thin film transistor monitors) and consequently can cause a comparatively high level of damage. In some designs, when an arc is identified, control to the vacuum plasma generator or to parts of the vacuum plasma generator is switched off so that no further energy flows into an output oscillating circuit of the generator. This procedure may not be sufficient for FPD production since there can still be too much residual energy in the output oscillating circuit of the generator, in the inductors of an output transformer that may be provided in the generator, and in the supply lines to the generator.
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Head wounds The back of the skull shows dramatic injuries. One consists of a hole near the spine, where a large piece of bone has been sliced away by a heavy bladed weapon such as a halberd. This, along with a smaller wound opposite, may well have been a fatal injury. A smaller dent which cracked the inside of the skull, is thought to have been caused by a dagger. There are a further five wounds on the skull, all inflicted around the time of death.
3.25
3
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--- author: - 'Kevin J. Walsh' - Alessandro Morbidelli title: 'The Effect of an Early Planetesimal-Driven Migration of the Giant Planets on Terrestrial Planet Formation' --- Introduction ============ The formation of the terrestrial planets is expected to have occurred from a disk of planetesimals in two steps. In the first step, Moon to Mars-size “planetary embryos” formed by runaway and oligarchic accretion (Greenberg et al. 1978; Wetherill & Stewart 1993; Kokubo & Ida 1998). In the second step, the terrestrial planets formed by high-velocity collisions among the planetary embryos (Chambers & Wetherill 1998; Agnor et al. 1999; Chambers 2001; Raymond et al. 2004, 2005, 2006, 2007; O’Brien et al. 2006; Kenyon & Bromley 2006). The most comprehensive effort to date in modeling terrestrial planet formation (Raymond et al. 2009) focused on 5 constraints of the terrestrial planets: 1. the orbits, particularly the small eccentricities, 2. the masses, with the small mass of Mars the most difficult to match, 3. formation timescales, 4. bulk structure of the asteroid belt and 5. the water content of Earth. Despite success with some of these constraints in each simulation, no simulation satisfied all the constraints simultaneously. For the simulations with fully formed Jupiter and Saturn on nearly circular orbits, the constraint consistently missed is the small mass of Mars. A Mars of the correct size is only obtained in simulations where the giant planets are on orbits with current semimajor axes but much larger eccentricities. This scenario, however, raises the problem of not allowing any water delivery to Earth from material in the outer asteroid belt region. The size of Mars has been a consistent problem for previous works with giant planets assumed on current orbits and disks of planetesimals and embryos stretching from $\sim$0.5–4.0 AU (Chambers & Wetherill 1998; O’Brien et al. 2006), or even only up to 1.5 or 2.0 AU (Kokubo et al. 2006; Chambers 2001). However, Hansen (2009) had great success creating analogs of Mars in simulations which begin with a narrow annulus of planetary embryos between 0.7 and 1.0 AU. In these simulations both Mercury and Mars are formed from material that is scattered out of the original annulus by the growing Earth and Venus analogs. In addition, the orbits of the Earth and Venus analogs have eccentricities and inclinations similar to those observed today and the accretion timescales are in agreement, although on the low side, with the ages of the Earth-Moon system deduced from the $^{182}$Hf - $^{182}$W chronometer. This model points to the need for a truncated planetesimal disk at, or near, the beginning of the process of terrestrial planet formation. The origin of this truncation remains to be understood. Similarly, it remains to be clarified how the truncation of the disk of planetesimals at 1 AU can be compatible with the existence of asteroids in the 2-4 AU region. Nagasawa et al. (2005) and Thommes et al. (2008) effectively produced a cut in the planetesimal distribution at  1.5 AU by assuming that the giant planets were originally on their current orbits and that secular resonances swept through the asteroid belt during gas-dissipation. However, the assumption that the giant planets orbits had their current semimajor axes when the gas was still present is no longer supported. When embedded in a gas disk, planets migrate relative to each other until a resonance configuration is achieved (Peale & Lee 2002; Kley et al. 2009; Ferraz-Mello et al. 2003; Masset & Snellgrove 2001; Morbidelli & Crida 2007; Pierens & Nelson 2008). Thus it is believed that the giant planets were in resonance with each other when the gas disk disappeared (Morbidelli et al. 2007; Thommes et al. 2008; Batygin & Brown 2010) which causes problems in understanding the consequences of the Thommes et al. (2008) model. Moreover, the Nagasawa et al. (2005) and Thommes et al. (2008) simulations produce the terrestrial planets too quickly ($\sim 10$ Myr), compared to the timing of moon formation indicated by the $^{182}$Hf - $^{182}$W chronometer ($>30$ Myr and most likely $>50$ Myr; Kleine et al. 2009) and they completely deplete the asteroid belt by the combination of resonance sweeping and gas-drag (see also Morishima et al. 2010, for a discussion). The resonant configuration of the planets in a gas disk is extremely different from the orbital configuration observed today. Planetesimal-driven migration is believed to be the mechanism by which the giant planets acquired their current orbits after the gas-disk dissipation. In fact, work by Fernandez & Ip (1984) found that Uranus and Neptune have to migrate outward through the exchange of angular momentum with planetesimals that, largely, they scatter inward. Similarly, Saturn suffers the same fate of outward migration, though Jupiter migrates inward as it ejects the planetesimals from the solar system. The timescale for planetesimal-driven migration of the giant planets depends on the distribution of the planetesimals in the planet-crossing region. It is typically 10 My, with 5 My as the lower bound (Morbidelli et al. 2010). Close encounters between pairs of giant planets might also have contributed in increasing the orbital separations among the giant planets themselves (Thommes et al. 1999; Tsiganis et al. 2005; Morbidelli et al. 2007; Brasser et al. 2009; Batygin & Brown 2010). Beyond the consequences for the scattered planetesimals, the migration of the giant planets affects the evolution of the solar system on a much larger scale, through the sweeping of planetary resonances through the asteroid belt region. The chronology of giant planet migration is important for the general evolution of the solar system, including the formation of the terrestrial planets. It has been recently proposed (Levison et al. 2001; Gomes et al. 2005; Strom et al. 2005) that the migration of the giant planets is directly linked in time with the so-called “Late Heavy Bombardment” (LHB) of the terrestrial planets (Tera et al. 1974; Ryder 2000, 2002; Kring & Cohen 2002). If this is true, then the migration of the giant planets should have occurred well after the formation of the terrestrial planets. In fact, the radioactive chronometers show that the terrestrial planets were completely formed 100 Myr after the condensation of the oldest solids of the solar system (the so-called calcium alluminum inclusions, which solidified 4.568 Gyr ago; Bouvier et al. 2007; Burkhardt et al. 2008), whereas the LHB occurred 3.9–3.8 Gyr ago. Thus the terrestrial planets should have formed when the giant planets were still on their pre-LHB orbits: resonant and quasi-circular. However, the simulations of Raymond et al. (2009) fail to produce good terrestrial planet analogs when using these pre-LHB orbits. The alternative possibility is that giant planet-migration occurred as soon as the gas-disk disappeared. In this case, it cannot be a cause of the LHB (and an alternative explanation for the LHB needs to be found; see for instance Chambers 2007). However, in this case giant planet migration would occur while the terrestrial planets are forming, and this could change the outcome of the terrestrial planet formation process. In particular, it is well known that, as Jupiter and Saturn migrate, the strong $\nu_6$ secular resonance sweeps through the asteroid belt down to $\sim 2$ AU (Gomes 1997). The $\nu_6$ resonance occurs when the precession rate of the longitude of perihelion of the orbit of an asteroid is equal to the mean precession rate of the longitude of perihelion of Saturn, and it affects the asteroids’ eccentrcities. If the giant planet migration occurs on a timescale of 5–10 Myr, typical of planetesimal-driven migration, then the $\nu_6$ resonance severely depletes the asteroid belt region (Levison et al. 2001; Morbidelli et al. 2010). This can effectively truncate the disk of planetesimals and planetary embryos, leaving it with an outer edge at about 1.5 AU. Although the location of this edge is not as close to the sun as assumed in Hansen (2009) (1 AU), it might nevertheless help in forming a Mars analog, i.e. signficantly less massive than the Earth. An equally important constraint is the resulting orbital distribution of planetesimals in the asteroid belt region, between 2–4 AU. After that region has been depleted of planetesimals and embryos by the sweeping resonances, what remains will survive without major alteration and should compare favorably with todays large asteroids. Studies of late giant planet migration start with an excited asteroid belt, where inclinations already vary from 0–20$^{\circ}$ (Morbidelli et al. 2010), and cannot match the inclination distribution of the inner asteroid belt with 5 Myr or longer migration timescales. The early migration presented here is different because it occurs immediately after the dissipation of the gas disk so that the planetesimal orbits are dynamically cold, with inclincations less than 1$^{\circ}$. Thus, in principle, an early giant planet migration could lead to a different result. Also, the embryos will be present, another difference with late migration scenarios. The purpose of this paper is to investigate, for the first time, the effect that an [*early*]{} migration of the giant planets could have had on the formation of the terrestrial planets and on the final structure of the asteroid belt. In Section 2 we discuss our methods and in Section 3 we present our results. The conclusions and a discussion on the current state of our understanding of terrestrial planet formation will follow in Section 4. Methods ======= We assume in our simulations that the nebular gas has dissipated, Jupiter and Saturn have fully formed; in the terrestrial planet and asteroid belt region, in the range 0.5-4.0 AU, the planetesimal disk has already formed planetary embyros accounting for half of its total mass. The lifetime of the circumstellar gas disk is observed to be 3–6 Myr, and both Jupiter and Saturn are expected to be fully formed by this time (Haisch et al. 2001). The timescales for oligarchic growth is similar, with lunar to Mars sized embryos growing on million year timescales (Kokubo & Ida 1998,2000). The numerical simulations are done using SyMBA, a symplectic $N$-body integrator modified to handle close encounters (Duncan et al. 1998). In our model, the planetary embryos interact with each other; the planetesimals interact with the embryos but not with themselves; all particles interact with the giant planets and, except when specified (explained further below), the giant planets feel the gravity of embryos and planetesimals. Collisions between two bodies result in a merger conserving linear momentum. It has been demonstrated by Kokubo & Genda (2010) that this a priori assumption of simple accretion does not significantly affect the results. The SyMBA code has already been used extensively in terrestrial planet formation simulations (Agnor et al. 1999; Levison & Agnor 2003; O’Brien et al. 2006; McNeil et al. 2005). Protoplanetary disk ------------------- The initial protoplanetary disks are taken directly from O’Brien et al. (2006), which themselves were based on those of Chambers (2001). The O’Brien et al. (2006) study produced some of the best matches for terrestrial planets and by using similar intial conditions allows a direct comparison. The initial conditions are based on a “minimum mass” solar nebula, with a steep surface denstiy profile. The solid mass is shared between many small planetesimals and a small number of large bodies, the embryos, as suggested by runaway/oligarchic growth simulations (Kokubo & Ida 1998, Kokubo & Ida 2000). In theory, it is possible that, by the time the gas disappears from the disk (which cooresponds to time zero in our simulations) the planetary embryos in the terrestrial planet region could have grown larger than the mass of Mars. However, the current mass of Mars seemingly excludes this possibility, and argues for masses to have been martian or sub-martian in mass. The surface density profile is $\Sigma(r) = \Sigma_{0}(\frac{r}{1 \mathrm{AU}})^{-3/2}$, where $\Sigma_{0}$ = 8 g cm$^{-2}$. The distribution of material drops linearly between 0.7 and 0.3 AU. Half of the mass is in the large bodies, of which there were either 25 embryos, each of 0.0933 Earth masses ($M_\oplus$) or 50 embryos of 0.0467 $M_\oplus$. The small bodies are 1/40 as massive as the large embyros, or 1/20 as massive as the small embryos. For all test cases the embryos are spaced between 4–10 mutual hill radii at the beginning of the simulations. In some tests, the smaller planetesimals with an initial semimajor axis larger than 2.0 were cloned into two particles with identical semi-major axis, half the mass in each, and different random eccentricities and inclinations (noted as ’Double Asteroids’ in Table 1.). The initial eccentricities and inclinations were selected randomly in the range of 0-0.01 and 0-0.5 degrees respectively. Thus the initial mass of the disk consisted of 2.6 $M_\oplus$ located inside of 2 AU and a total mass of 4.7 $M_\oplus$. Giant planets and migration --------------------------- In all tests Jupiter and Saturn were started on orbits closer to each other than at the present time, i.e. with semimajor axes of 5.4 and 8.7 AU, respectively. These initial orbits are just beyond their mutual 1:2 mean motion resonance, i.e. the corrseponding ratio of orbital periods of Saturn and Jupiter is slightly larger than 2. Even if the giant planets should have started from a resonant configuration - probably the 2:3 resonance (Masset & Snellgrove 2001; Pierens & Nelson 2008) - it is known that secular resonance sweeping through the asteroid belt is important only when the planets’ orbital period ratio is larger than 2 (Gomes 1997; Brasser et al. 2009). Thus, our choice of the initial orbits of Jupiter and Saturn is appropriate for the purposes of this study. Each planet was forced to migrate by imposing a change to their orbital velocities that evolves with time $t$ as: $$v(t) = v_0 + \Delta v [1 - \exp(-t/\tau)]$$ appropriate $\Delta v$ to achieve the required change in semimajor axis, and $\tau=5$ Myr. The latter is the minimum timescale at which planetesimal-driven migration can occur, simply due to the lifetime of planetesimals in the giant planet crossing region, as discussed extensively in Morbidelli et al. (2010). Longer timescales are possible, but previous work has shown that fast timescales affect the asteroid belt region less, and since terrestrial planet formation timescales are in the 10’s of millions of years, more rapid migration has a greater chance of affecting the accretion of Mars. Thus, we think that restricting ourselves to the 5 My timescale is sufficient, as this timescale is the most favorable for these purposes. ![Example of idealized migration for a system with only Jupiter and Saturn, ending with orbits very close to the current ones. Panel (a) shows the semimajor axis of Jupiter, (b) the eccentricity of Jupiter, (c) the semimajor axis of Saturn and (d) the eccentricity of Saturn, all plotted as a function of time in years.[]{data-label="migration"}](Figs/IdealMigration.ps){width="9.0cm"} If the motion of the giant planets was not affected by the other bodies in the system, the evolution of the eccentricities and inclinations would not change much during migration (Brasser et al., 2009, and Fig. 1). Thus it is relatively simple to find initial conditions that lead to the final orbital configurations with eccentricities and inclinations with mean values and amplitude of oscillations similar to current one. In fact, as shown in Brasser et al. (2009), the initial values $(e_J,e_S)=(0.012,0.035)$ and $(i_J,i_S)=(0.23^\circ,1.19^\circ)$, after migration, lead to eccentricities and inclinations whose mean values and amplitudes of oscillation closely resemble those characterizing the current secular dynamics of the giant planets (see Fig. \[migration\]). In our case, however, as the giant planets migrate, they scatter planetesimals and planetary embryos, and their orbits are affected in response. Thus, the final orbits are not exactly like those of Fig. \[migration\]. Typically, for instance, the eccentricities and inclinations of the planets are damped, and their relative migration is slightly more pronounced than it was intended to be. Thus, we tried to modify the initial eccentricities of Jupiter and Saturn and the values of $\Delta v$ in order to achieve final orbits as similar as possible to those of Fig. \[migration\]. However, while the effect of planetesimals on the planets is statistically the same from simulation to simulation, (and so can be accounted for by modifying the initial conditions of the planets), the effects of embryos are dominated by single stochastic events. Thus, it is not possible to find planetary initial conditions that lead systematically to good final orbits. In some cases the final orbits are reasonably close to those of the current system, but in many cases they are not. In total we performed 30 simulations. We discarded the simulations with unsuccessful final orbits, and kept only those (9/30) that lead to orbits resembling the current ones. These successful runs are called hereafter “normal migration simulations”. Our criterion for discriminating good from bad final orbits was determined after the 15 Myr of migration, and the semimajor axis, eccentricity and oscillation in eccentricity ($\Delta e$) were the factors examined. Jupiter’s orbit must have had $|a - a_j| < 0.05$, $|e - e_j| < 0.0156$, and $|\Delta e - \Delta e_j| < 0.0164$, while Saturn’s orbit required $|a - a_s| < 0.075$, $|e - e_s| < 0.0252$, and $\Delta e - \Delta e_s| < 0.0256$. We complemented our normal migration simulations with what we call hereafter ’perfect migration’ cases. In these simulations, the planetesimals and embryos do not have any direct effect on the giant planets, even during close encounters. However, their indirect effects cannot be suppressed (specifically the H$_{\mathrm{sun}}$ term from eq. 32b. in Duncan et al. 1998) , but in principle they are weaker. Thus the migration of the giant planets, starting with the initial conditions from Brasser et al. 2009 (as in Fig. \[migration\]), met the above criteria in 3 out of 4 simulations. The giant planets had the full gravitational affect on the planetesimals and embryos throughout these simulations, and the mutual effects between planetesimals and embryos remained unchanged. Results ======= We present the results of 12 simulations of terrestrial planet formation each covering 150 Myr. Of these runs, 9 are normal migration simulations and 3 ’perfect migration’ simulations (all simulations are listed in Table 1. and refered to by run name, “Test31” etc., throughout). These two sets of simulations had qualitative and quantitative similarities and are thus discussed at the same time and combined in the figures. First, the resulting planets are compared with the current terrestrial planets, followed by a look at the consequences the migration has on the structure of the asteroid belt. ![The final mass ($M_\oplus$) for each planet produced in our simulations is plotted as a function of the planet’s semimajor axis. The horizontal error bars show the locations of the perihelion and aphelion of the cooresponding orbit. The open squares refer to the planets produced in the normal migration simulations, the open circles to the planets produced in the run with twice as many half-sized embryos, and the open triangles to those produced in the ‘perfect migration’ simulations; the solid squares represent the real terrestrial planets. []{data-label="RandomMvS"}](Figs/MassSemi.ps){width="8.4cm"} The planets ----------- Results for these simulations are summarized in Fig. \[RandomMvS\], where the final masses and semimajor axes of our synthetic planets are compared to those of the real terrestrial planets (see also Table \[runtable\]). The trend is similar to that found in previous works (see for instance Chambers et al. 2001), where the masses and locations of Earth and Venus are nearly matched by a number of different simulations, but most planets just exterior to Earth, near $a$ $\sim$1.5 AU are at least 3 times more massive than Mars. However, a handful of planets close to 1.8 AU were of similar mass to Mars. Of note, Test31 had two $\sim$Mars-mass bodies, at 1.2 and 2.4 AU, with an Earth mass planet at 1.52 AU. Test54, the only one of four simulations starting with the smaller embryos with successful migration, produced a sub-Mars mass body at 1.89 AU, just at the edge of the current day asteroid belt. The Ran4 simulation produced a body within 50% of Mars’ mass at 1.71 AU, though it had a high eccentricity above 0.13 and was a member of a 3 planet system. In general, planets produced at around 1.5 AU were $\sim$ 5 times more massive than Mars, and Mars-mass bodies were typically only found beyond 1.7 AU. The total number of planets produced in each simulation is not systematically consistent with the real terrestrial planet system. Only two simulations produce 4 planets, where we define a “planet” as any embryo-sized or larger body with a semimajor axis less than 2.0 AU. Most simulations had 3 planets at the end, while one produced 5 planets. A common metric for measuring the distribution of mass among multiple planets is the radial mass concentration statistic (RMC), defined as $$RMC = max\bigg(\frac{\sum M_j}{\sum M_j[\log_{10}(a/a_j)]^2}\bigg) ,$$ where $M_j$ and $a_j$ are the mass and semimajor axis of planet $j$ (Chambers, 2001). The bracketed function is calculated for different $a$ in the region where the terrestrial planets form. The RMC is infinite for a single planet system, and decreases as mass is spread among multiple planets over a range of semimajor axes. The current value of RMC for the solar system is 89.9. For all but one simulation the RMC value is below the current solar systems value, largely due to the large mass concentrated in a Mars-analog orbit (we did not include the two embryos stranded in the asteroid belt region in these calculations, one in Test31 and one in TestPM24). The single simulation with a larger RMC value did not have a Mars analog, and thus the mass was contained in a smaller semimajor axis range. The terrestrial planets have low eccentricities and inclinations, Earth and Venus both have $e < 0.02$ and $i < 3^\circ$, properties which has proved difficult to match in accretion simulations. O’Brien et al. (2006) and Morishima et al. (2008) reproduced low eccentricities and inclinations largely due to remaining planetesimals which damp the orbital excitation of the planets. A metric used as a diagnostic of the degree of success of the simulations in reproducing the dynamical excitation of the terrestrial planets is the angular momentum deficit (AMD; Laskar 1997): $$AMD = \frac{\sum_j M_j \sqrt{a_j}\left(1-\cos(i_j)\sqrt{1-e_j^2}\right)}{\sum_j M_j \sqrt{a_j}} ,$$ where $M_j$ and $a_j$ are again the mass and semimajor axis and $i_j$ and $e_j$ are the inclination and eccentricity of planet $j$. The AMD of the current solar system is 0.0014. The AMD for our simulations ranged from 0.0011 to 0.0113. The plantesimal disk used in these simulation is based on that from O’Brien (2006), and is therefore not surprising that some AMDs are consistent with the solar system value. Simulation PM22 is the one with the largest final AMD, because it produced an Earth-analog with a 10$^\circ$ inclination. ![Evolution of the system over time, showing the clearing of the asteroid belt region with inclination plotted as a function of semimajor axis. The open boxes are planetesimals on orbits within the current asteroid belt region, the crosses are planetesimals elsewhere, and the open circles are embryos or planets scaled in relation to their diameters. The simulation is Test31. []{data-label="31"}](Figs/Test31Evol.ps){width="8.4cm"} ![Same as Fig. \[31\], but for simulation Test54, which started from 50 embryos of 0.0467 $M_\oplus$ instead of 25 embryos twice as massive. []{data-label="54"}](Figs/Test54Evol.ps){width="8.4cm"} Figures \[31\] and \[54\] show snapshots of two systems evolving over time. Of interest is the radial clearing caused by the movement of the giant planets and the sweeping of their resonances, particularly the $\nu_6$ resonance. This clearing progresses from the outer edge of the disk towards the sun, following the migration of the $\nu_6$ resonance, and stops at $\sim 2$ AU, which is the final location of this resonance when the giant planets reach their current orbits. Thus, the region of $a > 2.0$ is almost entirely cleared of material in 10 Myr, with only handfuls of planetesimals surviving and a single embryo. At 3 Myr, only $a > 2.5$ AU is largely cleared. ![Mass growth of the Mars analogs for all simulations plotted as a function of time. The most massive Mars analogs exceed the mass of Mars (0.11 $M_\oplus$) in only 2–3 Myr, and then in the next 10–20 Myr continue to grow to their final sizes, ending many times more massive than Mars. The two lines starting from $\sim 0.05$ $M_\oplus$ are for two planets of simulation ’Test54’, the only successful normal simulation that started with half-Mars mass embryos. The bold line shows the mass growth of the planet ending at $\sim 1.2$ AU; the thin line the planet ending at $\sim 1.9$ AU. []{data-label="marsgrowth"}](Figs/MarsGrowth2.ps){width="8.4cm"} As seen in Figure \[marsgrowth\] the accretion of embryos for the Mars analogs (where a Mars analog is defined as the largest body between 1.2–2.0 AU) begins immediately with $\sim$2 Mars-mass typically being reached in only 2 Myr (note that Figure \[marsgrowth\] shows 12 growth curves, as there are two planets displayed for Test54). Nine of the 11 Mars analogs have reached 0.2 $M_\oplus$ by 3 Myr. At 10 Myr 6 of the 11 have reached 0.3 $M_\oplus$, and by 30 Myr 10 of 11 are above 0.3 $M_\oplus$, or $\sim$3 $M_ \mathrm{Mars}$. One might wonder if our inability to produce a small Mars analog is due to the fact that, in all but one of the presented simulations (Test54 is the exception), the planetary embryos are initially $\sim$ one Mars mass. This is not regarded as a problem for the following reasons. First, the Mars analogs with semimajor axes near that of Mars, near 1.5 AU, typically accreted 4 or 5 embryos; thus they consistently accreted much more mass than Mars, and are not simply the result of a chance accretion between two Mars mass embryos. Second, only two of the 11 Mars analogs did not accrete another embryo, in Test54 and Ran4, but both had semimajor axes larger than 1.7 AU, well beyond the current orbit of Mars. Third, our single successful normal migration simulation that started with half-Mars mass embryos also produced an Earth mass planet at 1.2 AU. This planet was already two-mars masses in 5 Myr (notice that in the same simulation one embryo escaped all collisions with other embryos and therefore remained well below the mass of Mars - see Figure \[marsgrowth\]– but this object ended up at 1.9 AU, well beyond the real position of Mars). Finally, previous works (Chambers 2001; Raymond et al. 2009; Morishima et al. 2010 to quote a few) which started with embryos significantly less massive than Mars met the same Mars-mass problem found here. The similarities between our work and previous in terms of the mass distribution of the synthetic planets as a function of semimajor axis suggest that the giant planet migration does not affect significantly the terrestrial planet accretion process. Thus it is unlikely that small changes in the adopted evolution pattern of the giant planets could lead to significantly different results. Therefore the initial conditions do not appear to be at fault for the failure to match the mass of Mars. The reason for which the Mars analog consistently grows too massive is twofold. First, they grow fast (in a few million years, as shown in Figure \[marsgrowth\]), compared with the timescale required to effectively truncate the disk at $\sim 2$ AU (10 Myr, as shown in Figures \[31\] and \[54\]). Second, the truncation of the disk caused by the sweeping of the $\nu_6$ resonance is not sunward enough: the final edge is approximately at 2 AU, whereas an edge at $\sim 1$ AU is needed (Hansen 2009; Kokubo et al. 2006; Chambers 2001). Figure \[allSims\] shows the final incination vs. semimajor axis distributions of all our simulations (respectively, ’normal’ and ’perfect’ ones). The sizes of the symbols representing the planets are proportional to the cubic roots of their masses. Again, the problem of the mass of Mars stands out. ![Endstates of all simulations with the inclination plotted as a function of the semimajor axis with asteroids as open squares, non-asteroid planetesimals as crosses and embryos/planets as open circles scaled by their mass to the 1/3 power. []{data-label="allSims"}](Figs/allSims.ps){width="8.4cm"} The asteroid belt ----------------- In the previous section we have shown that the an early sweeping of secular resonances through the asteroid belt is not useful to solve the small-Mars problem. Here we address the question of other observational constraints. For this purpose, in this section we turn to the asteroid belt, whose orbital distribution is very sensitive to the effects of resonance sweeping (Gomes 1997; Nagasawa et al. 2000; Minton & Malhotra 2009; Morbidelli et al. 2010). Morbidelli et al. (2010) have shown that the properties of the asteroid belt after the slow migration of the giant planets are largely incompatible with the current structure of the asteroid belt. However, they assumed that the migration of the giant planets occurred late, after the completion of the process of terrestrial planet accretion and after the primordial depletion/dynamical excitation of the asteroid belt. Thus, that work does not exclude the possibility of an early migration. In fact, the outcome of an early migration could be very different from that of a late migration for two reasons: first, the initial orbits of the plantesimals are quasi-circular and co-planar in the early migration case whereas they are dynamically excited in the late migration case, which is an important difference; second, planetary embryos reside in, or cross, the asteroid belt region during the early time of terrestrial planet formation, and this process has the potential of erasing some of the currently unobserved signatures of resonace sweeping. ![(Top) The inclination of current day asteroids with absolute magnitude H $<$ 9.7, corresponding to D $\gtrsim$ 50 km, plotted as a function of their semimajor axis. The long-dashed lines show the location of the major mean motion resonances with Jupiter and the short-dashed curves the location of the $\nu_{6}$ and $\nu_{16}$ secular resonances. (Bottom) Surviving planetesimals from the 12 simulations, showing a strong depletion of low inclination bodies in the inner part of the asteroid belt region.[]{data-label="Asteroids"}](Figs/Asteroids.ps){width="8.4cm"} To compare the planetesimal distribution obtained in our simulations with the “real” asteroid population, we focus on asteroids larger than $\sim$50 km in diameter, as in previous works (Petit et al. 2001; Minton & Malhotra 2009; Morbidelli et al. 2010). These bodies are a reliable tracer of the structure of the asteroid belt that resulted from the primordial sculpting process(es), as they are too large to have their orbits altered significantly by the thermal Yarkovsky effect or by collisions (see Fig. \[Asteroids\],). Moreover, their orbital distribution (see top panel of Fig \[Asteroids\]) is not affected by observational biases, because all bodies of this size are known (Jedicke et al. 2002). The final distribution of the planetesimals residing in the asteroid belt in our 12 simulations is shown in the bottom panel of Fig \[Asteroids\]. As can be seen, the difference in orbital distribution between the real belt and that resulting from the giant planet migration process is striking. A simple metric used in Morbidelli et al. (2010) to quantify the difference in orbital distributions between the real and the synthetic belts is the ratio of asteroids above and below the location of the $\nu_6$ secular resonance with semimajor axis below 2.8 AU. The current day value for asteroids with a diameter above 50 km is 0.07. Combining together all the surviving planetesimals from all our 12 simulations results in a 67/13 ratio, in stark contrast to the current value. Thus, our result is qualitatively similar to that of Morbidelli et al. (2010), even though our resulting ratio is much larger than that obtained in that work (close to 1/1). The reason for the large ratio obtained in migration simulations, as discussed in Morbidelli et al. (2010), is that the migration of the giant planets forces the $\nu_6$ and $\nu_{16}$ secular resonances to move Sun-ward. More precisely, if the orbital separation of Jupiter and Saturn increased by more than $1$ AU (as predicted by all models and enacted in our simulations), the $\nu_6$ resonance sweeps the entire asteroid belt as it moves inwards from 4.5 AU to 2 AU; meanwhile the $\nu_{16}$ resonance sweeps the belt inside of 2.8 AU to its current location at 1.9 AU (Gomes et al. 1997). In the inner asteroid belt, the $\nu_{16}$ resonance sweeps first and the $\nu_6$ resonance sweeps second. The $\nu_{16}$ resonance occurs when the precession rate of the longitude of the node of the orbit of an asteroid is equal to the precession rate of the node of the orbit of Jupiter, and it affects the asteroid’s orbital inclination. Given the characteristic shape of the $\nu_6$ resonance location in the $(a,i)$ plane (see Fig \[Asteroids\]), the asteroids that acquire large enough inclination when they are swept by the $\nu_{16}$ resonance, avoid being swept by $\nu_6$; thus, their eccentricities are not affected and they remain stable. Conversely, the asteroids that remain at low-to-moderate inclinations after the $\nu_{16}$ sweeping are then swept by the $\nu_6$ resonance and their eccentricities become large enough to start crossing the terrestrial planet region. These bodies are ultimately removed by the interaction with the (growing) terrestrial planets. This process favors the survival of high-inclination asteroids (above the current location of the $\nu_6$ resonance) over low-inclination asteroids and explains the large ratio between these two populations obtained in the resonance sweeping simulations. This ratio is larger in our simulations than in those of Morbidelli et al. (2010), because the initial orbits of planetesimals and embryos in our case have small inclinations and eccentricities. Consequently, the secular resonance sweeping can only increase eccentricities and inclinations. Conversely, in the Morbidelli et al. (2010) simulations, the initial orbits covered a wide range of eccentricities and inclinations. Large eccentricities or inclinations can be [*decreased*]{} by the secular resonance sweeping. Thus, more objects could remain at low-to-moderate inclinations after the $\nu_{16}$ sweeping and fewer objects were removed by the $\nu_{6}$ sweeping than in our case. We conclude from our simulations that the migration of the giant planets with an $e$-folding time of 5 Myr (or longer, as the effects of secular resonance sweeping increases with increasing migration timescale) is inconsistent with the current structure of the asteroid belt, even if it occurred early. In fact, our simulations provide evidence that the planetary embryos crossing the asteroid belt during the process of formation of the terrestrial planets are not able to re-shuffle the asteroid orbital distribution and erase the dramatic scars produced by secular resonance sweeping. Discussion and Conclusions ========================== This paper has investigated the effects of [*early*]{} giant planet migration on the inner disk of planetesimals and planetary embryos. In the context of solar system formation, “early” is immediately following the disappearence of the gas disk, which is identified as time-zero in our simulations. The giant planets are migrated towards their current orbits with a 5 Myr $e$-folding time which is appropriate if the migration is caused by planetesimals scattering. We have shown that the sweeping of secular resonances, driven by giant planet migration, truncates the mass distribution of the inner disk, providing it with an effective outer edge at about 2 AU after about 10 Myr. This edge is too far from the Sun and forms too late to assist in the formation of a small Mars analog. In fact, Chambers (2001) already showed similar results starting from a disk of objects with semi-major axes $0.3<a<2.0$ AU, the terrestrial planet accretion process leads to the formation of planets that are systematically 3-5 times too massive at $\sim 1.5$ AU. For completeness, we have continued our simulations well beyond the migration timescale of the giant planets to follow the accretion of planets in the inner solar system, and we have confirmed Chambers (2001) result. Hansen (2009) showed that obtaining planets at $\sim 1.5$ AU that have systematically one Mars mass requires that the disk of solid material in the inner solar system had an outer edge at about 1 AU. The inability of secular resonance sweeping during giant planets migration to create such an edge suggests that a different mechanism needs to be found. Moreover, our study adds to the continuing inability of models with a slow migration of the giant planets, $\tau \gtrsim 5$ Myr, to leave an asteroid belt with a reasonable inclination distribution. Morbidelli et al. (2010) argued that the only possibility for the orbits of Jupiter and Saturn to move away from each other on a timescale shorter than 1 Myr is that an ice giant planet (presumably Uranus or Neptune) is first scattered inwards by Saturn and is subsequently scattered outwards by Jupiter, so that the two giant planets recoil in opposite directions. They dubbed this a “jumping-Jupiter” evolution and showed that in this case the final orbital distribution of the asteroid belt is consistent with that observed. Again, Morbidelli et al. (2010) worked in the framework of a “late” displacement of the orbits of the giant planets. Our results in this paper suggest that a jumping-Jupiter evolution would also be needed in the framework of an “early” displacement of the orbits of the giant planets. At this point, it is interesting to speculate what the effects of an “early” jumping-Jupiter evolution would be on the terrestrial planet formation process. In essence, an early jumping-Jupiter evolution would bring the giant planets to current orbits at a very early time. So, the outcome of the terrestrial planet formation process would resemble that of the simulations of Raymond et al. (2009) with giant planets initially with their current orbital configuration, labelled ’EJS’ in that work. In these simulations, though, (see their Fig. 10), the Mars analog is, again, systematically too big. It is questionable whether a jumping-Jupiter evolution could bring the giant planets onto orbits with current semimajor axes but larger eccentricities, as required in the most successful simulations of Raymond et al. (2009), labelled ’EEJS’. However, even though jumping-Jupiter evolutions satisfying this requirement were found, it is important to note that all of the outcomes of the EEJS simulations of Raymond et al. (2009). While producing a small Mars in several cases, the EEJS simulations failed in general to bring enough water to the terrestrial planets, formed the Earth too early compared to the nominal timescale of 50 Myr and left the terrestrial planets on orbits too dynamically excited. For all these reasons an early jumping-Jupiter evolution is not a promising venue to pursue for a successful model of terrestrial planet formation. In conclusion, our work substantiates the problem of the small mass of Mars and suggests that understanding terrestrial planet formation requires a paradigm shift in our view of the early evolution of the solar system. Acknowledgments {#acknowledgments .unnumbered} --------------- The authors would like to thank an anonymous reviewer for a careful reading of the manuscript. KJW acknowledges both the Poincaré Postdoctoral fellowship at the Observatoire de Côte d’Azur. This work is part of the Helmholtz Alliance’s ’Planetary evolution and Life’, which KJW and AM thank for financial support. Computations were carried out on the CRIMSON Beowulf cluster at OCA. 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Search Navigation Subnavigation Noncommunicable diseases Noncommunicable diseases (NCDs) are a group of diseases that affect individuals over an extended period of time causing socio-economic burden to the nation. The major NCDs share four behavioral risk factors- unhealthy diet, lack of physical activity, and use of tobacco and alcohol. Factors contributing to the rise of NCDs also include ageing, rapid unplanned urbanization and globalization. In 2008, NCDs accounted for 5.2 million deaths in India. A rising trend in the burden of NCDs is expected in the years ahead. There are primarily four type of noncommunicable diseases: cancer, chronic respiratory disease, stroke and diabetes, which are responsible for a majority of morbidity and mortality in the country. Mental health and injuries also have a considerable burden. In South-East Asia, including India, NCDs affect relatively younger population as compared to the western countries, thus causing severe economic burden to the nation. In order to reduce the growing burden of NCDs, it is important not only to address the diseases but also their key underlying risk factors, namely tobacco use, unhealthy diet, harmful use of alcohol and physical inactivity. A range of interventions have been identified that constitute as ‘best buys’. Best-buys for addressing the NCD risk factors Preventive strategies focus on the common underlying behavioral risk factors for NCDs including tobacco and harmful alcohol use, physical inactivity and unhealthy diet. These will help in controlling the metabolic risk factors like raised blood pressure, blood sugar and cholesterol, and obesity. Tobacco control Implementing the key elements of the WHO Framework Convention on Tobacco Control have been found cost-effective. These include increasing taxes, comprehensive legislations creating smoke-free indoor workplaces and public places, health information and warnings about the effects of tobacco, and bans on advertising, promotion and sponsorship. Harmful alcohol use Reduction in the harmful use of alcohol not only prevents cancers and cardiovascular diseases, but also prevents conditions like liver cirrhosis, depression and road traffic injuries. Enhanced taxation of alcohol beverages and comprehensive bans on their advertising/ marketing have proved to be beneficial. Unhealthy diet Excessive salt intake is related to raised blood pressure. Reducing salt content in foods is an effective strategy. The use of added salt should be discouraged. In India, we need to address both, homemade and processed food. Population based approaches include reaching out through mass media campaigns. Use of polyunsaturated fats as cooking medium, along with avoiding transfats is also recommended. Physical inactivity Indoor air pollution The dependence on solid fuels (coal, wood, animal dung, crop wastes) and traditional stoves for cooking and heating leads to high levels of indoor air pollution. This increases the risk of childhood pneumonia, chronic lung disease and lung cancers. In addition to tobacco control, reducing indoors air pollution is the most important strategy for preventing chronic lung disease, particularly in non-smokers. Best-buys for tackling major NCDs Cardiovascular disease (CVD) and diabetes Counselling and multi-drug therapy (including blood sugar control for diabetes mellitus) for people with risk of developing heart attacks and strokes will reduce the morbidity and mortality due to these conditions. A regimen of aspirin, statin and blood pressure-lowering agents will significantly reduce vascular events in people with cardiovascular risk and is considered a best buy. Preventive measures, such as tobacco cessation and adopting a healthy life style, augment the therapeutic benefits. Administration of aspirin to people who develop a myocardial infarction is another best buy. Cancer Hepatitis B immunization beginning at birth can prevent liver cancer. Presently a regimen of three doses- first at birth (only possible in case of institutional deliveries), at six weeks, 10 weeks and 14 weeks along with diphtheria, pertussis, tetanus(DPT) have been included into the Universal Immunization Programme (UIP). Screening and treatment of pre-cancerous lesions is effective for preventing cervical cancer. Pain relief and palliative care is a low cost, yet essential, intervention when judged against societal norms and standards, keeping in mind the human rights perspective. Chronic respiratory disease Chronic respiratory disease, including asthma and chronic obstructive pulmonary disease are major contributors towards morbidity and mortality in the country. Treatment of persistent asthma with inhaled corticosteroids and beta-2 agonists like salbutamol are very low cost interventions and feasible to deliver in primary care, but their cost-effectiveness is limited by their modest impact on disease burden. However, as already mentioned above, tobacco cessation and alleviation of indoor air pollution are the key strategies for preventing chronic respiratory disease.
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Cells move. They do it to help embryos develop, fashioning organs and tissues. White blood cells chase bacteria and viruses, preventing us from getting sick. Cancer cells spread via the blood. Cell movement is an essential process that underlies health and disease. Yet despite many years of intensive study, a good understanding of the mechanics of this important phenomenon has remained out of biologists' grasp. In an effort to "glue" together large groups of scientists to tackle such pressing problems confronting biomedical scientists today, the National Institute of General Medical Sciences has provided an $8 million "glue grant" (for the first year of funding) to a consortium of basic scientists who will work to unlock the mysteries of cell movement. NIGMS anticipates spending a projected total of $38 million on the project over the course of five years. "For some research, the intellectual and material resources available to individual laboratories, or even to small groupings of labs, are simply not enough to adequately attack the problem. Glue grants provide an opportunity to marshal the resources needed," said Dr. Marvin Cassman, director of NIGMS. The "Cell Migration Consortium" project brings together a large group of scientists from leading academic medical centers across the country. Leading the project are two scientists from the University of Virginia School of Medicine, Dr. Alan F. "Rick" Horwitz and Dr. J. Thomas Parsons. "Understanding the mechanism of how cell migration occurs is critical to our understanding of diseases like cancer, arthritis and osteoporosis, as well as wound repair, embryonic development and tissue engineering," said Horwitz, professor of cell biology at U.Va. and the project's principal investigator. "For example, most people who have cancer don't die from primary tumors but from tumor spread — that's a migration problem. And a significant number of congenital brain defects are migration problems." One of the Consortium's goals is to generate new understanding about the basic mechanisms involved in cell migration. A key part of the plan is to generate new and sophisticated imaging strategies to visualize the fundamental signaling pathways that regulate cell migration — technologies that are sorely needed by the scientific community currently investigating cell movement. Another objective of the Consortium is to catalyze the translation of new discoveries in cell migration to the development of novel therapeutic drugs and treatments. The Consortium will be truly multifaceted — consisting of biologists, chemists, biophysicists, optical physicists, mathematicians, computer scientists, geneticists and engineers. The arrangement should foster a multi-pronged attack on the study of cell migration that will interface with the larger community of cell migration researchers. "The days of the lone investigator are rapidly waning in disciplines like cell biology," said Horwitz. "We have to cooperate rather than compete if we are to answer some of the most complex and challenging scientific questions." Using state-of-the-art Internet and interactive video technologies, Consortium researchers will share and discuss data as it is collected, Parsons explained. A Consortium Web site (www.cellmigration.org) will make possible the timely sharing of findings, ideas, and information. The Web site will be publicly accessible to scientists everywhere. NIGMS originally conceived of the large-scale glue grants following consultations with leaders in the scientific community who emphasized the importance of confronting intractable biological problems with the expertise and input of large, multifaceted groups of scientists. The first glue grant was awarded last year to Dr. Alfred G. Gilman, a pharmacologist at the University of Texas Southwestern Medical Center, who won the Nobel Prize in 1994 for work on signaling molecules called G proteins. Joining forces with U.Va. scientists are consortium members from several institutions, including the University of North Carolina at Chapel Hill; the Massachusetts Institute of Technology; the Burnham Institute; The Scripps Research Institute; Northwestern University; Harvard University; The Johns Hopkins University; Florida State University; the University of California, Davis; the University of Connecticut Health Center; and the University of Illinois. Please mention support for this work from the National Institute of General Medical Sciences (NIGMS), a component of the National Institutes of Health that supports basic biomedical research. Please fax clips to (301) 402-0224. Contacts: For comment on the glue grant program, call Alison Davis in the NIGMS Office of Communications and Public Liaison at (908) 735-7207 to arrange an interview with NIGMS director Dr. Marvin Cassman. For comment on the Cell Migration Consortium, call Marguerite Beck in the U.Va. Health System Media Relations office at (434) 924-5679 to arrange an interview with consortium leader Dr. Alan F. "Rick" Horwitz.
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William Douglas, 6th Earl of Morton William Douglas, 6th Earl of Morton (c. 1540 – 1606) was the son of Sir Robert Douglas of Lochleven and Margaret Erskine, a former mistress of James V of Scotland. Career Connections Sir William's half-brother from his mother's liaison with the king was James Stewart, Earl of Moray, Regent of Scotland from 1567 until his assassination in January 1570. Sir William's cousin was another Regent of Scotland James Douglas, 4th Earl of Morton, and was closely associated with him in his career, the two men being occasionally confused in the histories. William's father was killed at the battle of Pinkie in September 1547. William suffered from breathing difficulties all his life. His wife was Agnes Leslie, daughter of George Leslie, 4th Earl of Rothes, by whom he had eleven children. The Leslies were active in Scottish Reformation. Lochleven's prisoner William Douglas was the owner of the island Loch Leven Castle, where Mary, Queen of Scots had met John Knox in April 1563. Since 1546, he and his mother had built the "Newhouse of Lochleven" on the shore of Loch Leven where Kinross House now stands. The "Newhouse" eventually replaced the island castle as the centre of the estate. In June 1567, Queen Mary was imprisoned in the island castle following her surrender at the Battle of Carberry Hill. On 24 July she was forced to sign abdication papers at Lochleven in favor of her infant son James VI. William Douglas had a legal paper drawn up on 28 July 1567, which stated that he was not present when the Queen signed her "demission" of the crown and did not know of it, and that he offered to convey her to Stirling Castle for her son's coronation which was the following day, which offer she refused. Mary also signed that paper. However, in 1581 Mary wrote that William was one of her few remaining enemies in Scotland, and should have witnessed that she was compelled to assent to her resignation. The Scottish government directed by his half-brother paid William Douglas £1,289-12d for keeping the Queen. William's wife, Lady Agnes Leslie, became the Queen's chief female companion during her ten and a half months of imprisonment, accompanying her throughout the day and often sleeping in her bedchamber. Queen Mary had an opportunity of greater liberty following the birth of Agnes's child when she was recovering from her pregnancy. She chose to escape on 2 May 1568 from Lochleven with the aid of Sir William's brother George and a young orphaned cousin named William Douglas who also lived at the castle and may or may not have been the earl's illegitimate son. When Sir William learned of his royal captive's escape, he was so distressed that he attempted to stab himself with his own dagger. Ruthven Raid and Earl of Morton The title Earl of Morton was declared forfeit in 1581 when Regent Morton, the 4th earl, was attainted; and the title was granted to John Maxwell, 7th Lord Maxwell, a grandson of the 3rd earl. While Regent Morton was on trial in January 1581, William and other leading members of the family were not allowed to come to Edinburgh, and in March he was ordered to live north of Cromarty. A year later he joined in the Raid of Ruthven, and when this faction was defeated he was exiled in France at La Rochelle, returning in 1586. The 17th century historian David Hume of Godscroft relates that Agnes Leslie wrote to her husband saying she would prevent their son Robert from joining him at the Lords Enterprisers attempt to take Stirling Castle in 1584, saying it was a foolish work that would ruin them. William replied that their course was honourable, and intended for the good of the church, and he trusted in providence. Robert and their son-in-law Laurence Oliphant were banished to France despite their mother's efforts, and were lost at sea in a battle with "Hollanders" or pirates. In 1586, the attainder on the Morton earldom was reversed and the title returned to the 4th earl's family. By the 4th earl's will, on the death of Archibald Douglas, 8th Earl of Angus in 1588, William Douglas succeeded to the earldom of Morton, which brought him additional lands and houses including Dalkeith Palace, Aberdour Castle, Auchterhouse and Drochil Castle. In May 1590 he hosted the Danish Admiral Peder Munk at the Newhouse of Lochleven. Munk had been at Falkland Palace to accept the property as part of the dowry of Anne of Denmark. William wrote a short history of the Scottish reformation and reigns of Mary and James VI briefly mentioning the Siege of Leith, the Battle of Carberry Hill, the murder of David Rizzio, and the Ruthven Raid. Marriage and children On 26 November 1554 he married Lady Agnes Leslie, Countess of Morton (born after 1541-died ca. 1606), the daughter of George Leslie, 4th Earl of Rothes and as a direct descendant of King James II in her maternal line. The contract for their marriage was signed on 19 August 1554. The couple made their home at Lochleven Castle, which was a fortress situated on an island in the middle of the loch, and where his widowed mother also resided. Sir William and Agnes together had eleven children: Christian Douglas, married firstly Laurence, Master of Oliphant, (lost at sea in March 1585) by whom she had issue; she married secondly Alexander Home, 1st Earl of Home. Robert Douglas, Master of Morton, (lost at sea in March 1585), married Jean Lyon of Glamis, by whom he had two sons, including William Douglas, 7th Earl of Morton. First it was rumoured that Laurence Oliphant and Robert had been killed by pirates or drowned, then it was thought they were slaves in Algiers. In 1601, Robert Oliphant went to Algiers to look for his kinsman, carrying a letter of introduction to Sultan Mehmed III written by Queen Elizabeth, who also recommended her ambassador John Wroth help the search. James Douglas, Commendator of Melrose, married firstly Mary Kerr, by whom he had issue; secondly Helen Scott, by whom he had issue; and thirdly Jean Anstruther, by whom he had issue. Sir Archibald Douglas of Kilmour (died 1649), married Barbara Forbes (born 31 January 1560), by whom he had one son. Sir George Douglas of Kirkness (died December 1609), married Margaret Forrester. Euphemia Douglas, married Sir Thomas Lyon of Auldbar, Master of Glamis. Agnes Douglas, Countess of Argyll (1574- 3 May 1607), on 24 July 1592 married as his first wife Archibald Campbell, 7th Earl of Argyll, the son of Colin Campbell, 6th Earl of Argyll and Agnes Keith, by whom she had one son and two daughters. Elizabeth Douglas, married Francis Hay, 9th Earl of Erroll, by whom she had issue. Jean Douglas. Mary Douglas, married Sir Walter Ogilvy, 1st Lord Ogilvy of Deskford, by whom she had issue. Margaret Douglas, married Sir John Wemyss of Wemyss. Agnes's seven daughters were said to have been so beautiful that they were known as "the pearls of Lochleven". In 1586, the earldom of Morton which had been forfeited in 1581 following the execution and attainder of the 4th Earl of Morton for being one of Henry Stuart, Lord Darnley's murderers, returned to the Douglas family. In 1588, upon the death of Archibald Douglas, 5th Earl of Morton, Sir William became the 6th Earl of Morton. From that time onward Agnes was styled the Countess of Morton. Sir William received the charter for the earldom on 20 July 1589. William died sometime around the year 1606, which was the same year his wife died. Notes References External links Category:Earls of Morton William Douglas, 6th Earl of Morton Category:1606 deaths Category:Year of birth uncertain
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Antimony (Sb) is an element belonging to Group 15 of the Periodic Table and behaves similar to arsenic (As). Sb and its compounds are recognized as priority pollutants by the United States Environmental Protection Agency[@b1] and European Union[@b2]. In recent years, the serious Sb pollution resulting from increased exploitation and industrial emission has aroused growing concern[@b3][@b4][@b5]. Among various oxidation states (−3, 0, 3, and 5), antimonite \[Sb(III)\] and antimonate \[Sb(V)\] are the most common forms[@b6]. Because microbial redox reactions can be used as a strategy for biochemical detoxification and can further affect the mobility, toxicity, and bioavailability of Sb in the environment[@b7][@b8], a better comprehension of the microbe-Sb interactions is important for the bioremediation of Sb-contaminated environments and to understand the Sb biogeochemical cycle. In generally, Sb(III) is more toxic than Sb(V)[@b5][@b9], thus, examining the mechanisms driving bacterial oxidation from Sb(III) to Sb(V) could be of significant value in this regard. The understanding of microbial Sb transformation remains deficient compared to that of As[@b10]. It has been reported that the glycerol transporter GlpF and its homolog Fps1p are responsible for Sb(III) uptake, reflecting the structural similarities between Sb(OH)~3~ and glycerol[@b11][@b12][@b13], while the As(III) efflux proteins ArsB and Acr3 can also function as Sb(III) efflux pumps[@b14][@b15]. Nevertheless, the pathway of Sb(V) entrance has not been found yet. In addition, the genes and enzymes involved in microbial Sb(V) reduction and Sb(III) methylation have not been identified, although these phenomena are environmentally widespread[@b9]. In contrast with bacterial As(III) oxidation, which has been clarified for several decades, the mechanism of bacterial Sb(III) oxidation is of relatively recent interest. At present, about 60 Sb(III)-oxidizing bacteria, widely existing in various genera (e.g., *Pseudomonas, Comamonas, Agrobacterium* and *Acinetobacter*), have been reported[@b16]. Recently, we found that the As(III) oxidase AioAB is also function as an Sb(III) oxidase in *Agrobacterium tumefaciens* 5A[@b17], and subsequently we found a novel Sb(III) oxidase AnoA belonging to the short-chain dehydrogenase/reductase family of enzymes in *A. tumefaciens* GW4[@b18]. Compared with *A. tumefaciens* 5A[@b17], strain GW4 has considerably higher Sb(III) resistance and Sb(III) oxidation efficiency[@b18]. However, deletion of each gene only partially influenced the Sb(III) oxidation efficiency of *A. tumefaciens* strains, indicating other unknown mechanisms. Chemically, Sb(III) can be oxidized through several oxidants, such as H~2~O~2~, iodate, nature minerals (e.g., Fe and Mn oxyhydroxides) and humic acid under oxic conditions[@b19][@b20][@b21][@b22]. In bacterial cells, the aberrant electron flow under stress conditions from the electron transport chain or cellular redox enzymes to O~2~ results in the production of reactive oxygen species (ROS)[@b23]. The harmful ROS \[e.g., superoxide (O~2~^**·**−^), hydroxyl (OH^**·**^) and H~2~O~2~\] can induce DNA damage and the oxidative deterioration of lipids and proteins[@b24][@b25][@b26]. Thus, bacteria have evolved defense mechanisms against the oxidative stress. Superoxide dismutase (Sod), which catalyzes the dismutation of O~2~^**·**−^ to H~2~O~2~ and O~2~, plays an important role in defense against ROS. The generated H~2~O~2~ is subsequently consumed by catalases and peroxidases[@b23][@b27]. In a recent work, we deleted the catalase gene *katA* in *A. tumefaciens* GW4 and observed that the Sb(III) oxidation efficiency of the mutant strain was significantly increased, and the phenotype of the complementary strain was recovered[@b16]. Moreover, the transcription of *katA* was induced by both H~2~O~2~ and Sb(III)[@b16]. Therefore, we proposed that the increased Sb(III) oxidation efficiency in the mutant strain might reflect the accumulation of H~2~O~2~ in bacterial cells. Nevertheless, there is no direct evidence of a correlation between H~2~O~2~ and Sb(III) oxidation. In the present study, we performed gene knock-out/complementation of *katA, anoA, aioA* and *anoA/aioA* and in combination with the analyses of Sb(III) oxidation, cellular H~2~O~2~ content and resistance of Sb(III) and H~2~O~2~ in *A. tumefaciens* GW4[@b28]. We provide the first evidence that besides the biotic factors (AnoA and AioAB), the Sb(III) induced cellular H~2~O~2~ also catalyzes bacterial Sb(III) oxidation as an abiotic oxidant. The present study documented the abiotic Sb(III) oxidation and clarified the relationship between Sb(III) resistance and bacterial oxidative stress. The results represent an important step toward unraveling the co-metabolism of bacterial Sb(III) oxidation. Results ======= Genomic information of *aioA, anoA* and *katA* in *A. tumefaciens* GW4 ---------------------------------------------------------------------- *A. tumefaciens* GW4 is an Sb(III)-oxidizing strain, and its genome sequence was previously published (Accession No. AWGV00000000)[@b18]. To investigate the abiotic factors of Sb(III) oxidation, two types of cellular oxidative stress-related genes were analyzed. The catalase gene *katA*, responsible to degrade H~2~O~2~ to H~2~O and O~2~[@b27], showed a 91% sequence identity with *katA* in *A. tumefaciens* C58[@b29]. We also analyzed the superoxide dismutase Sod, which could convert O~2~^**·**−^ to H~2~O~2~ and O~2~. The BlastN results showed that *katA* is a single-copy gene in the genome of strain GW4, while *sod* has two copies (*sod1* and *sod2*). Thus, subsequent gene knock-out and complementation studies associated with the abiotic factors of Sb(III) oxidation were mainly focused on the *katA* gene. The arrangement of *katA* and its surrounding genes are shown in [Fig. 1A](#f1){ref-type="fig"}. For biotic Sb(III) oxidation, the oxidoreductase gene *anoA* ([Fig. 1B](#f1){ref-type="fig"}), identified as a novel Sb(III) oxidase, is conserved in the genomes of *Agrobacterium, Sinorhizobium* and *Rhizobium* strains[@b18]. Although several genes were annotated as "short chain dehydrogenase", "oxidoreductase", or "putative oxidoreductase" in the genome of strain GW4, the BlastN analyses indicated that the sequences of these genes showed no similarities with that of *anoA*. Moreover, BlastP analyses showed that the protein sequence of AnoA showed only \~30% similarity with those of other oxidoreductases. In addition, draft genome sequencing revealed that an arsenic gene island located in contig 215 contains the As(III) oxidase genes *aioAB* ([Fig. 1C](#f1){ref-type="fig"}), and *aioA* encodes the large subunit of As(III) oxidase[@b30]. Sb(III) induces the transcription of *katA, sod1, sod2* and *anoA*, but not *aioA* ---------------------------------------------------------------------------------- To investigate the biotic and abiotic factors associated with Sb(III) oxidation in *A. tumefaciens* GW4, the transcription levels of genes *katA, sod1, sod2, anoA* and *aioA* were examined. The catalase KatA and superoxide dismutase Sod are involved in the bacterial oxidative stress response, and the Sb(III) oxidase AnoA and As(III) oxidase AioAB were both reported to catalyze Sb(III) oxidation *in vitro*[@b16][@b17][@b18]. The quantitative reverse transcriptase PCR assays indicated that the transcription levels of both *katA* and *anoA* were increased with the addition of Sb(III), consistent with the results of our previous studies[@b16][@b17][@b18]. In addition, the transcription of *sod1* and *sod2* were also induced by Sb(III). The transcription level of *sod1* was much lower than *sod2*, suggesting that *sod2* might play a more important role in dismutation of O~2~^**·**−^. However, the transcription level of *aioA* was not induced by Sb(III) ([Fig. 1D](#f1){ref-type="fig"}), consistent with the previous observations in *A. tumefaciens* 5A[@b17]. Gene knock-out and complementation analyses showed effects of *katA, anoA* and *aioA* on Sb(III) oxidation ---------------------------------------------------------------------------------------------------------- Previously, we showed that the disruption of H~2~O~2~ degradation gene *katA* increased Sb(III) oxidation efficiency in strain GW4[@b16]. The successful deletion and complementation of *katA* were confirmed by diagnostic PCR shown in [Fig. S1](#S1){ref-type="supplementary-material"}. Strains GW4-Δ*aioA*, GW4-Δ*anoA* and their complemented strains were obtained from previous studies[@b17][@b18]. Strains GW4-Δ*aioA*/*anoA* and GW4-Δ*aioA*/*anoA-*C were obtained from this study and diagnostic PCR and DNA sequencing were used to confirm the successful deletion and complementation (data not shown). Based on our previous studies[@b16] and the growth tests in this study, all of the strains showed consistent growth profiles in CDM medium containing 50 μM Sb(III) ([Fig. 2](#f2){ref-type="fig"}), indicating that the Sb(III) oxidation was not affected by the growth of the strains under 50 μM Sb(III). Based on our previous results[@b16], we calculated that the Sb(III) oxidation efficiency of strain GW4-Δ*katA* (\~52%) was increased by \~80% compared with the wild-type strain GW4 (\~29%). The catalase KatA is responsible for cellular H~2~O~2~ consumption[@b27], thus we proposed that the high efficient Sb(III) oxidation in strain GW4-Δ*katA* might be associated with the cellular H~2~O~2~ content. Moreover, the GW4-Δ*anoA* showed a \~30% decrease in the Sb(III) oxidation efficiency ([Fig. 2B](#f2){ref-type="fig"}), which is similar to our previous study[@b18]. In contrast, deletion of *aioA* had no effect on the Sb(III) oxidation efficiency during the log phase, while the Sb(III) oxidation efficiency was slightly increased during the stationary phase ([Fig. 2D](#f2){ref-type="fig"}). It has been suggested that in the stationary phase of bacterial growth, other Sb(III) oxidation mechanism(s) might exist and function more efficiently in the absence of *aioA*. The simultaneous deletion of *aioA* and *anoA* resulted in a phenotype of Sb(III) oxidation efficiency between GW4-Δ*aioA* and GW4-Δ*anoA* (\~19% decreased) ([Fig. 2F](#f2){ref-type="fig"}), and all of the complemented strains showed a Sb(III) oxidation efficiency similar to that of the wild-type strain GW4 ([Fig. 2](#f2){ref-type="fig"}). The *katA, anoA* and *aioA* influence each other and further affect Sb(III) oxidation ------------------------------------------------------------------------------------- To elucidate how *katA, anoA* and *aioA* influence each other and further affect Sb(III) oxidation, we detected the transcription level of these genes in each *A. tumefaciens* strain. Bacterial cells were cultivated in CDM medium, and samples were collected after 0.5 h of induction with 50 μM Sb(III). In strain GW4-Δ*katA*, the transcription levels of *aioA* and *anoA* were not increased ([Fig. 3A](#f3){ref-type="fig"}), suggesting that the reduced consumption of H~2~O~2~ might be responsible for the efficient Sb(III) oxidation. In addition, the transcription levels of *aioA* and *katA* in strain GW4-Δ*anoA* showed no significant difference with the wild-type strain, consistent with the phenotype of decreased Sb(III) oxidation efficiency ([Fig. 3B](#f3){ref-type="fig"}). In contrast, the transcription levels of *anoA* and *katA* were up-regulated in strain GW4-Δ*aioA* (p \< 0.01), indicating that the AnoA- and H~2~O~2~-catalyzed Sb(III) oxidation was enhanced relative than the wild-type strain ([Fig. 3C](#f3){ref-type="fig"}). Therefore, the deletion of *aioA* increased the Sb(III) oxidation efficiency in strain GW4. In strain GW4-Δ*aioA*/*anoA*, although the transcription level of the *katA* was increased (p \< 0.01), the loss function of AnoA could not be compensated ([Fig. 3D](#f3){ref-type="fig"}). Expectedly, all of the complemented strains recovered the phenotype back to the wild-type strain GW4 ([Fig. 3](#f3){ref-type="fig"}). The *katA, anoA* and *aioA* are involved in Sb(III) resistance -------------------------------------------------------------- Subsequent efforts focused on the Sb(III) resistance of the *A. tumefaciens* strains. After 48 h incubation in CDM medium without Sb(III) supplementation, all of the strains exhibited a similar amount of viable cell counts ([Fig. 4A](#f4){ref-type="fig"}). Moreover, there was no significant difference between the viable cell counts of the strains cultured with or without 50 μM Sb(III), indicating that 50 μM Sb(III) has no effect on bacterial growth. However, the deletion of *katA* significantly inhibited the growth of strain GW4 with the addition of 100 or 200 μM Sb(III) (p \< 0.05 and p \< 0.01, respectively), suggesting that the reduced H~2~O~2~ consumption might associated with bacterial Sb(III) resistance. In addition, the growth of strains GW4-Δ*anoA*, GW4-Δ*aioA* and GW4-Δ*aioA*/*anoA* were also obviously constrained (p \< 0.05) relative to strain GW4 in the presence of 100 or 200 μM Sb(III), and the phenotypes of the complemented strains were recovered to the wild-type strain ([Fig. 4A](#f4){ref-type="fig"}). These results indicated that both biotic and abiotic factors of Sb(III) oxidation were essential for bacterial Sb(III) resistance. The *katA* is involved in H~2~O~2~ resistance --------------------------------------------- Plate counting assays were also performed to evaluate the antibacterial activities of H~2~O~2~ against *A. tumefaciens* strains using the same culture conditions with Sb(III) resistance. H~2~O~2~ is a substantial component of cellular oxidative stress with a toxic effect on different types of macromolecules[@b31][@b32]. The growth of strain GW4 was not affected by 50, 100 and 200 μM H~2~O~2~, suggesting that the oxidative stress response in strain GW4 is efficient for the detoxification of such concentrations of H~2~O~2~. For strains GW4-Δ*aioA*, GW4-Δ*anoA* and GW4-Δ*aioA*/*anoA* and their complemented strains, the viable cell counts were consistent with wild-type strain GW4, indicating that the deletion of biotic factors in strain GW4 did not affect bacterial H~2~O~2~ resistance ([Fig. 4B](#f4){ref-type="fig"}). However, the growth of GW4-Δ*katA* was significantly inhibited by 50, 100 and 200 μM H~2~O~2~ (p \< 0.01), because such concentrations of H~2~O~2~ could not be efficiently consumed without decomposition through KatA. The phenotype of the complemented strain GW4-Δ*katA*-C was recovered ([Fig. 4B](#f4){ref-type="fig"}). The results demonstrated that *katA* is essential for bacterial H~2~O~2~ resistance. Correlation between H~2~O~2~ content and Sb(III) oxidation both *in vivo* and *in vitro* ---------------------------------------------------------------------------------------- To understand the relationship between the cellular H~2~O~2~ content and Sb(III) oxidation, we examined the H~2~O~2~ content in *A. tumefaciens* strains with or without the induction of 50 μM Sb(III). The results indicated the following: i) The generation of cellular H~2~O~2~ was induced by Sb(III), ii) The cellular H~2~O~2~ content was consistent with the transcription level of genes associated with abiotic Sb(III) oxidation, and iii) The content of H~2~O~2~ was proportional to the bacterial Sb(III) oxidation efficiency. The strain with a higher H~2~O~2~ content showed a faster Sb(III) oxidation efficiency ([Figs 2](#f2){ref-type="fig"} and [5A](#f5){ref-type="fig"}). In addition, we measured the dynamic changes in the cellular H~2~O~2~ content and Sb(V) generation in strains GW4, GW4-Δ*katA* and GW4-Δ*katA*-C from 24 to 48 h cultivation with the addition of 50 μM Sb(III). A significant decrease in the residual H~2~O~2~ content was observed with incubation time, while the Sb(V) concentration correspondingly increased ([Fig. 5B,C](#f5){ref-type="fig"}), indicating that the consumed H~2~O~2~ might catalyze bacterial Sb(III) oxidation. Moreover, the H~2~O~2~ content and the increased Sb(V) concentration were significantly linearly correlated, with a correlation coefficient of 0.93 ([Fig. 5D](#f5){ref-type="fig"}). The dynamic changes in the H~2~O~2~ content and Sb(V) generation were also measured in CDM medium with the addition of 50 μM Sb(III) and different concentrations of H~2~O~2~. [Figure 5E](#f5){ref-type="fig"} showed that Sb(III) was transformed to Sb(V) with the addition of H~2~O~2~, indicating that H~2~O~2~ could oxidize Sb(III) to Sb(V) *in vitro*. In addition, there is a correlation between the H~2~O~2~ and Sb(V) contents *in vitro* (R^2^ = 0.94) ([Fig. 5F](#f5){ref-type="fig"}). Based on the *in vivo* and *in vitro* analyses, we proposed that H~2~O~2~ is responsible for bacterial Sb(III) oxidation as an abiotic oxidant in strain GW4. Comparison of Sb(III) oxidation between *A. tumefaciens* GW4 and *A. tumefaciens* 5A ------------------------------------------------------------------------------------ Previous studies have shown that *A. tumefaciens* 5A, which has a *16S rRNA* homology of 99% compared with *A. tumefaciens* GW4, also oxidizes Sb(III) to Sb(V)[@b17][@b33]. AioAB is responsible for Sb(III) oxidation in strain 5A, as the deletion of *aioA* decreased the Sb(III) oxidation efficiency, in contrast with the phenotype of strain GW4-Δ*aioA*[@b17]. To clarify the different effects of *aioA* on Sb(III) oxidation between strain GW4 and 5A, we also investigated the *aioA* mutant in strain 5A under the same culture conditions of strain GW4. The growth of strains GW4 and 5A were not affected by disruption of *aioA* in CDM medium supplemented with 50 μM Sb(III) ([Fig. S2A,B](#S1){ref-type="supplementary-material"}). However, the Sb(III) oxidation efficiency was increased in strain GW4-Δ*aioA* ([Fig. S2C](#S1){ref-type="supplementary-material"}), and the transcription of *anoA* and *katA* and the cellular H~2~O~2~ content were increased when *aioA* was deleted ([Figs S3A and S4A](#S1){ref-type="supplementary-material"}). In contrast, the Sb(III) oxidation efficiency was decreased in strain 5A-Δ*aioA* ([Fig. S2D](#S1){ref-type="supplementary-material"}), and no increased transcription of *katA* was observed, moreover, the transcription level of *anoA* was only slightly increased ([Fig. S3B](#S1){ref-type="supplementary-material"}). Although Sb(III) also stimulated the generation of H~2~O~2~, this process was not affected by the disruption of *aioA* in strain 5A ([Fig. S4B](#S1){ref-type="supplementary-material"}). Discussion ========== Currently, studies have shown that bacterial Sb(III) oxidation is catalyzed through AioAB or AnoA with a certain percentage of contribution[@b17][@b18], indicating the existence of other new bacterial Sb(III) oxidation mechanisms. The present study documents a non-enzymatic basis for microbial Sb(III) oxidation, according to the following observations: i) The transcription of *katA, sod1, sod2* and the cellular H~2~O~2~ content were induced by Sb(III); ii) the Sb(III) oxidation efficiency was consistent with the cellular H~2~O~2~ content in *A. tumefaciens* strains; and iii) The cellular H~2~O~2~ content in the *katA* mutant was remarkably linearly correlated with the Sb(V) concentration. Thus, we concluded that the cellular H~2~O~2~ acts as an abiotic factor in bacterial Sb(III) oxidation. The cellular H~2~O~2~ mediated bacterial Sb(III) oxidation is an smart detoxification process of Sb(III)-oxidizing bacteria through the "using poison against poison" strategy, which could transform the toxic Sb(III) to the much less toxic Sb(V) and consume the toxic cellular H~2~O~2~ simultaneously. In addition, the Sb(III) resistance mechanism associated with bacterial oxidative stress has not been well clarified so far. It has been reported that H~2~O~2~ induces the death of *E. coli*, primarily reflecting DNA damage via the Fenton reaction[@b34][@b35][@b36]. Recently, the bacterial oxidative stress was found to associate with Sb(III) oxidation in *Pseudomonas stutzeri* TS44[@b37]. In this study, the deletion of *katA* significantly decreased H~2~O~2~ resistance, reflecting the disruption of the release of the oxidative stress response in strain GW4. A large number of literatures have shown that heavy metals (e.g. Cr, Cd)[@b38][@b39], transition metals (e.g. Fe, Cu)[@b23] and metalloid (As)[@b40] could induce bacterial oxidative stress response due to their toxic effects. As a most common toxic heavy metal, the production of H~2~O~2~ could be the primary response of bacterial to Sb(III). It appears that the *katA* mutant is more tolerant to Sb(III) than H~2~O~2~ because Sb(III) oxidation consumed the cellular H~2~O~2~ even the *katA* was disrupted. In the presence of 50 μM Sb(III), the amount of H~2~O~2~ was consumed by Sb(III) oxidation and the cellular H~2~O~2~ was not toxic enough to inhibit bacterial growth. However, in the presence of high concentrations (e.g. 100 or 200 μM) of Sb(III), the high amount of H~2~O~2~ induced by Sb(III) in the *katA* mutant has a higher toxic effect on bacterial cells, even though the Sb(III) oxidation also consumed some of the H~2~O~2~. Thus, the Sb(III) resistant level in strain GW4-Δ*katA* was still lower than the wild-type strain GW4. To understand bacterial Sb(III) oxidation and the contribution of each cellular oxidative factor comprehensively, we also investigated the effects of biotic factors on Sb(III) oxidation in *A. tumefaciens* GW4. The deletion of *anoA* led to a \~ 30% decrease in the Sb(III) oxidation efficiency and the abiotic Sb(III) oxidation was not enhanced, indicating that the decreased Sb(III) oxidation efficiency reflected the contribution of AnoA. However, the deletion of *aioA* increased Sb(III) oxidation efficiency, reflecting the increased expression of AnoA and the generation of more H~2~O~2~. Thus, the contribution of AioAB to Sb(III) oxidation in strain GW4 was not obvious, however, AioAB is indeed related to Sb(III) oxidation, since it affects the expressions of AnoA and KatA. In addition, the results of a kinetic analysis in our previous study indicated that AnoA tends to catalyze the Sb(III) oxidation more efficiently than As(III) oxidation, while AioAB is prone to catalyze As(III) oxidation[@b16]. These results suggested that the effect of AnoA on Sb(III) oxidation may higher than that of AioAB. The contribution of H~2~O~2~-catalyzed abiotic Sb(III) oxidation may higher than that of enzymatic catalysis in strain GW4 since the disruption of KatA significantly increased Sb(III) oxidation efficiency[@b16]. The results of a previous study demonstrated that AioAB was responsible for bacterial Sb(III) oxidation in *A. tumefaciens* 5A, suggesting that the effect of *aioA* on Sb(III) oxidation between strain 5A and GW4 was different. In strain 5A, AioAB has a substantial contribution to Sb(III) oxidation efficiency (approximately 25%)[@b17]. However, it appears that AioAB has no positive effect on Sb(III) oxidation in strain GW4, potentially reflecting the different characteristics between these two strains. The Sb(III) MIC of strain 5A is 0.3 mM, while strain GW4 is a highly Sb(III) resistance bacterium with a 8 mM MIC of Sb(III) (data not shown). In addition, strain 5A had a longer lag phase than that of strain GW4 with the addition of 50 μM Sb(III), indicating that Sb(III) might has a more toxic effect on strain 5A. Nonetheless, we cannot exclude the possibility that AioA might catalyze Sb(III) oxidation along with AnoA in strain GW4 because complex regulatory mechanism(s) might be involved in the compensation of the Sb(III) oxidation efficiency in the *aioA* mutant, which needs to be further studied. In nature, H~2~O~2~ is a strong oxidant and it can oxidize not only Sb(III), but also other metalloids, such as As(III). However, the efficiency of bacterial As(III) oxidation catalyzed by H~2~O~2~ is not as obvious as Sb(III) oxidation and the abiotic As(III) oxidation could be hardly observed *in vivo* (data not shown). So far, bacterial As(III) oxidation has been found to be an enzymatic reaction which is primarily catalyzed through AioAB in most As(III)-oxidizing bacteria[@b41]. However, the mechanism of bacterial Sb(III) oxidation is a co-metabolism process catalyzed by AioAB, AnoA and H~2~O~2~, which is different from bacterial As(III) oxidation (at least in *A. tumefaciens* GW4). Although previous studies have shown that AnoA could also oxidize As(III) *in vitro*[@b16], the expression of *anoA* was not induced by As(III)[@b18], and the deletion of *anoA* did not affect the As(III) oxidation efficiency in strain GW4 (data not shown). Thus, the effect of AnoA on bacterial As(III) oxidation was hardly observed. In addition, H~2~O~2~ is an important and effective oxidant responsible for Sb(III) oxidation in alkaline aqueous environments[@b42][@b43], and the Sb(III) oxidation rate is much faster than that of As(III)[@b44][@b45][@b46]. In the present study, the pH of the cultures increased from the initial 6.5 to approximately 8.0 following exposure to Sb(III), indicating that the culture conditions are suitable for H~2~O~2~ to catalyze Sb(III) oxidation ([Fig. S3E,F](#S1){ref-type="supplementary-material"}). However, the culture pH decreased with the increasing incubation time during As(III) oxidation of strain GW4 (data not shown), and this pH might not be suitable for abiotic oxidation mediated through H~2~O~2~. Therefore, the abiotic oxidation is more effective on Sb(III) in strain GW4. Based on the observations of the present study, we proposed that microbial Sb(III) oxidation is a co-metabolism process in strain GW4 ([Fig. 6](#f6){ref-type="fig"}): (i) AioAB might be responsible for Sb(III) oxidation in the periplasm[@b17]; (ii) AnoA catalyzes cytoplasmic Sb(III) oxidation with NADP^+^ as a co-factor[@b18]; (iii) Sb(III) induces the bacterial oxidative stress response, leading to the production of ROS[@b37] and H~2~O~2~; iv) the disruption of AioAB increases the expression of AnoA; (v) the disruption of AioAB increases the cellular H~2~O~2~ content and expression of KatA; (vi) the induced H~2~O~2~ oxidizes Sb(III) to Sb(V); and (vii) the redundant H~2~O~2~ is partially consumed by KatA. In summary, the present study provides novel evidences that microbial antimonite oxidation contains both abiotic and biotic mechanisms and elucidates the contribution of each oxidative factor. We show that Sb(III) causes oxidative stress to bacterial cells and further induces the generation of cellular H~2~O~2~. Sb(III) oxidation is a detoxification process by transforming the toxic Sb(III) to the much less toxic Sb(V). Meanwhile, since the cellular H~2~O~2~ is consumed by Sb(III) oxidation process, the Sb(III) oxidation also contributes to against the toxic H~2~O~2~. Such co-mechanism may be widely exist in other Sb(III)-oxidizing microorganisms. The relationship among the biotic and abiotic factors may be further studied by changing Sb(III) concentration, environmental and nutritious conditions. Materials and Methods ===================== Strains and genomic analysis ---------------------------- Bacterial strains and plasmids used in the present study are listed in [Table S1](#S1){ref-type="supplementary-material"}. *A. tumefaciens* strains were grown in a chemically defined medium (CDM)[@b47] containing 0 or 50 μM K~2~Sb~2~(C~4~H~2~O~6~)~2~ \[Sb(III)\] with aeration through shaking at 28 °C. *E. coli* strains were cultured at 37 °C in Luria-Bertani (LB) medium. When required, ampicillin (Amp, 100 mg/mL), kanamycin (Kan, 50 mg/mL), tetracycline (Tet, 5 mg/mL), gentamicin (Gen, 50 mg/mL) or chloromycetin (Cm, 50 mg/mL) were added. The genomic analyses of *aioA, anoA, katA* and *sod* were conducted through blastn and blastp in the genome of *A. tumefaciens* GW4 on the NCBI website (<http://www.ncbi.nlm.nih.gov>). Constructions *A. tumefaciens* GW4 mutant strains and complemented strains -------------------------------------------------------------------------- An in-frame deletion in *katA* was constructed in strain GW4 using crossover PCR[@b48]. The primers used for construction of the deletion are listed in [Table S2](#S1){ref-type="supplementary-material"}. The PCR products were double digested with *BamH*I and *Xba*I and subsequently cloned into pJQ200SK digested with the same restriction enzymes. The final construct pJQ-*katA* was mobilized into strain GW4 via conjugation with *E. coli* S17-1. Single-crossover mutants were identified on LB agar plates containing 100 μg/mL Amp and 50 μg/mL Gen, which were subsequently screened on CDM agar containing 20% sucrose[@b49]. Sucrose^R^ and Gen^Sen^ transconjugants were screened using PCR and DNA sequencing to verify the *katA* deletion. For GW4-Δ*aioA*/*anoA*, an in-frame deletion in *anoA* was constructed in the mutant strain GW4-Δ*aioA* using the method described above. The GW4-Δ*aioA* and GW4-Δ*anoA* mutants and their complementary strains were obtained from previous works[@b17][@b18]. The construction of GW4-Δ*katA* complementation was accomplished using plasmid pCPP30. The complete *katA* coding region was PCR-cloned into *BamH*I - *Pst*I double-digested pCPP30. The resulting plasmid pCPP30-*katA* was subsequently mobilized into strain GW4-Δ*katA* via *E. coli* S17-1. Tet^R^ and Amp^R^ transconjugants were screened on LB agar plates, yielding the complementary strain GW4-Δ*katA*-C. The complementation of GW4-Δ*aioA*/*anoA* was performed using two plasmids, pCPP30 and pCT-Zori[@b50]. The *aioAB* genes along with the upstream RpoN binding site and the complete *anoA* coding region were PCR-cloned into *BamH*I - *Pst*I double-digested pCT-Zori and pCPP30, respectively. The resulting plasmid pCT-Zori-*aioAB* and pCPP30-*anoA* were simultaneously mobilized into strain GW4-Δ*aioA*/*anoA* via *E. coli* S17-1. Subsequently, Tet^R^, Cm^R^ and Amp^R^ transconjugants were screened on LB agar plates. The complementary strains were verified through PCR and DNA sequencing. Quantitative RT-PCR analysis ---------------------------- To investigate the expression of the genes associated with Sb(III) oxidation in *A. tumefaciens* strains, overnight cultures of these strains were each inoculated into 100 mL of CDM at 28 °C with 120 rpm shaking. When the OD~600~ reached 0.2--0.3, 0 or 50 μM Sb(III) was added to the cultures. After 0.5 h of induction, the bacterial cells were harvested for total RNA extraction using Trizol reagent (Invitrogen) and treated with RNase-free DNase I (Takara) according to the manufacturer's instructions (Invitrogen, Grand Island, NY, USA). The quality and quantity of the RNA were monitored using a spectrophotometer (NanoDrop 2000, Thermo). Reverse transcription was performed using the RevertAid First Strand cDNA Synthesis Kit (Thermo) with 300 ng total RNA for each sample[@b51]. Subsequently, the obtained cDNA was diluted 10-fold and used as a template for further analysis. Quantitative RT-PCR was carried out by ABI VIIA7 in 0.1 mL Fast Optical 96-well Reaction Plate (ABI) using SYBR^®^ Green Real-time PCR Master Mix (Toyobo) and the primers listed in [Table S2](#S1){ref-type="supplementary-material"}. To eliminate error, three technical and biological replicates were established for each reaction. The *A. tumefaciens* GW4 16S rRNA gene was used as an internal control and the expression data of the genes were normalized to 16S rRNA without Sb(III) using the formula 2^−(ΔCT−CT,16SrRNA,zero\ Sb)^, which was modified from the 2^−ΔΔCT^ method[@b52][@b53][@b54]. Growth, Sb(III) oxidation and sensitivity assays ------------------------------------------------ *A. tumefaciens* strains were each inoculated into 5 mL of CDM with the addition of 50 μM Sb(III) and incubated at 28 °C with shaking at 120 rpm. When the OD~600~ reached 0.5--0.6, the strains were each inoculated into 100 mL of CDM in the presence of 50 μM Sb(III). Culture samples were collected every 8 h for measuring OD~600~ by spectrophotometry (DU800, Beckman). In addition, the samples were centrifuged (13,400 × g) and subsequently filtered (0.22 μm filter) to monitor the Sb(III)/Sb(V) concentrations through HPLC-HG-AFS (Beijing Titan Instruments Co., Ltd., China) according to Li *et al*.[@b55]. To determine the Sb(III) and H~2~O~2~ resistance of *A. tumefaciens* strains, the viable plate counting method was employed. The strains were each inoculated into 100 mL of CDM medium with the addition of different concentrations of Sb(III) or H~2~O~2~ (0 μM, 50 μM, 100 μM and 200 μM) respectively, and incubated at 28 °C with shaking at 120 rpm. After cultivation for 48 h, the samples were collected for gradient dilution and spread onto solid LB medium, respectively. The plates were incubated at 28 °C and counted after 2--3 days until colonies formed. H~2~O~2~ content and Sb(III) oxidation assays --------------------------------------------- To assess the H~2~O~2~ contents, *A. tumefaciens* strains were cultured as described above. After incubation for 0.5 h with 50 μM Sb(III), the bacterial cells (2 mL) were harvested through centrifugation (13,400 × g for 5 min at 4 °C) and washed twice with 50 mmol/L K~3~PO~4~ (pH 7.8). Subsequently, the cells were resuspended in 1 mL K~3~PO~4~ (pH 7.8) and sonicated on ice. The supernatants were obtained through centrifugation (13 400 × g, 10 min, 4 °C) to remove cell debris and subsequently mixed with 50 μL amplex red (AR) (Chemical Co., St. Louis, MO, USA) and 50 μL horseradish peroxidase (HRP) (F. Hoffmann-La Roche Ltd, Shanghai, China)[@b56]. After incubation at 37 °C for 15 min, fluorescence (530 ex/587 em) was measured using an EnVision^®^ Multimode Plate Reader (Perkin Elmer). To determine the dynamic variations in the H~2~O~2~ and Sb(V) contents *in vivo*, strains GW4, GW4-Δ*katA* and GW4-Δ*katA*-C were each inoculated into 100 mL of CDM medium supplemented with 50 μM Sb(III) and incubated at 28 °C for 48 h with shaking at 120 rpm. At designated times, the culture samples were collected to assess the H~2~O~2~ contents and monitor the Sb(V) contents as described above. For *in vitro* dynamic changes in the H~2~O~2~ and Sb(V) contents, at designated times, the measurement of Sb(V) concentrations was performed in CDM medium with the addition of 50 μM Sb(III) and different concentrations of H~2~O~2~ (5 μM, 10 μM, 15 μM and 20 μM). Additional Information ====================== **How to cite this article**: Li, J. *et al*. Abiotic and biotic factors responsible for antimonite oxidation in *Agrobacterium tumefaciens* GW4. *Sci. Rep.* **7**, 43225; doi: 10.1038/srep43225 (2017). **Publisher\'s note:** Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations. Supplementary Material {#S1} ====================== ###### Supplementary Information This work was financially supported through a grant from the National Natural Science Foundation of China (31470226) to G.W. The authors declare no competing financial interests. **Author Contributions** J.L. designed and performed the experiments and drafted the manuscript. B.Y., M.S., K.Y., W.G. and Q.W. performed the experiments. G.W. designed the study and revised the manuscript. All authors read and approved the final manuscript. ![Physical map of *katA, anoA* and *aioA* (**A--C**) and gene transcription of *katA, sod1, sod2, anoA* and *aioA* in *A. tumefaciens* GW4 (**D**). (**A--C**) Gene clusters of *katA, anoA* and *aioA.* (**D**) Quantitative reverse transcriptase-PCR analysis. Total RNA was isolated from strain GW4 cultured in CDM medium with 0.5 h induction of 0 or 50 μM Sb(III). The *16S rRNA* gene was used as a reference. Data are shown as the mean of three replicates, with the error bars representing ± SD. \*\*Represents p \< 0.01; \*represents p \< 0.05.](srep43225-f1){#f1} ![Growth and Sb(III) oxidation curves of *A. tumefaciens* strains.\ (**A**,**C**,**E**) The growth curves of *A. tumefaciens* strains in CDM medium containing 50 μM Sb(III). Panels A, C, E share the same data of strain GW4. (**B**,**D**,**F**) Sb(III) oxidation profiles of the same strains. Panels B, D, F share the same data of strain GW4. The culture conditions were the same as previous described (Li *et al*.[@b15]). Cell growth was measured based on culture optical density, and Sb(V) concentrations in the culture fluids were measured using HPLC-HG-AFS. Error bars correspond to the standard deviations of the means from three independent experiments. The Sb(III) oxidation efficiency was calculated at 48 h according to the formula: \[Sb(V) concentration/Total Sb concentration\]\*100%.](srep43225-f2){#f2} ![Quantitative reverse transcriptase-PCR analysis of the genes associated with Sb(III) oxidation in *A. tumefaciens* strains.\ (**A--D**) Total RNA was each isolated from strains GW4, GW4-Δ*katA,* GW4-Δ*katA-*C, GW4-Δ*anoA*, GW4-Δ*anoA*-C, GW4-Δ*aioA*, GW4-Δ*aioA-*C, GW4-Δ*aioA/anoA* and GW4-Δ*aioA/anoA-*C cultured with 50 μM Sb(III). Panels A-D share the same data of strain GW4. The 16S rRNA gene was used as a reference. Data are shown as the mean of three replicates, with the error bars representing ± SD. \*\*Represents p \< 0.01; \*represents p \< 0.05.](srep43225-f3){#f3} ![Sb(III) (**A**) and H~2~O~2~ (**B**) resistance of *A. tumefaciens* strains. Bacterial cells were inoculated into 100 mL of CDM medium with the addition of different concentrations of Sb(III) or H~2~O~2~ (0, 50, 100 and 200 μM). After 24 h of incubation, the samples were collected for viable plate counting. Data are shown as the mean of three replicates, with the error bars represents ± SD. \*\*Represents p \< 0.01; \*represents p \< 0.05.](srep43225-f4){#f4} ![The cellular H~2~O~2~ content is correlated with bacterial Sb(III) oxidation.\ (**A**) The H~2~O~2~ content and relevant Sb(V) concentration of *A. tumefaciens* strains after 2 h of incubation with or without 50 μM Sb(III). (**B**) H~2~O~2~ content and (**C**) Sb(V) concentration in strains GW4, GW4-Δ*katA* and GW4-Δ*katA*-C from 24 to 48 h of cultivation in CDM medium with the addition of 50 μM Sb(III). (**D**) Correlation between the H~2~O~2~ content and Sb(V) concentration in strain GW4-Δ*katA*. (**E**) Dynamic changes in the H~2~O~2~ and Sb(V) contents in CDM medium with 50 μM Sb(III) and different concentrations of H~2~O~2~ and without the inoculation of *A. tumefaciens* strains. (**F**) Correlation between H~2~O~2~ and Sb(V) contents *in vitro*. Data are shown as the mean of three replicates, with the error bars represents ± SD. \*\*Represents p \< 0.01; \*represents p \< 0.05.](srep43225-f5){#f5} ![A proposed model of bacterial Sb(III) oxidation based on the present study and literatures.\ (1) Sb(III) oxidation might be catalyzed through As(III) oxidase AioAB[@b17]; (2) Sb(III) oxidase AnoA was shown to oxidize Sb(III) to Sb(V) in cytoplasm with NADP^+^ as a cofactor[@b18]; (3) Sb(III) induced the cellular production of ROS (O~2~^−^) and H~2~O~2~; (4--5) Deletion of *aioA* in *A. tumefaciens* GW4 resulted in the increased expression of AnoA and KatA and cellular H~2~O~2~ content; (6) H~2~O~2~ oxidizes Sb(III) oxidation as an abiotic factor; (7) The residual H~2~O~2~ was partially consumed through KatA.](srep43225-f6){#f6} [^1]: Present address: Department of Land Resources and Environmental Sciences, Montana State University, Bozeman, MT 59717, USA.
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Buruli ulcer. A disabling infection. Buruli ulcers result from an initial skin infection that often leads to extensive tissue necrosis. The causative agent is Mycobacterium ulcerans, a bacterium prevalent in humid, rural tropical areas. Several thousand people are infected each year, especially in Africa, where Buruli ulcers are a source of major disability. A combination of oral rifampicin and injectable streptomycin is effective. Surgical treatment and functional rehabilitation are often necessary. Diagnostic tests suitable for use in primary care settings are needed, along with well-tolerated, effective oral treatments.
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A. Technical Field The present subject matter is directed to items that are usable to help educate children in learning activities. More specifically, the present subject matter is directed to the field of educational devices for teaching people about wave action and the dynamics of liquids. B. Description of Related Art Duck races are a popular pastime. It is not uncommon to see hundreds or thousands of people converge on a river to put ducks, which are almost universally yellow, into a river to see whose duck reaches the finish line first. Often, there is an entry fee and the proceeds may go to the winner or be given to a charity. It is fun for all, but the outcome is determined solely by luck. It is an object of the present subject matter to provide a water raceway device designed for racing ducks or other floating objects, where skill is a factor in the outcome of the race. It is a further object of the present subject matter to provide a water raceway device where the floating objects are conveyed down a first sluice primarily by the action of waves and are conveyed down a second sluice primarily under the force of currents. It is a further object of the present subject matter to provide an insert that can be positioned in a tub to convert the tub into a device for racing floating objects. It is a further object of the present subject matter to provide an educational experience that is so much fun that participants may not realize that they are learning about fluid dynamics and currents and waves. It remains desirable to provide improvements in water raceway devices
3.03125
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On Dreams On Dreams (Ancient Greek: Περὶ ἐνυπνίων; Latin: De insomniis) is one of the short treatises that make up Aristotle's Parva Naturalia. The short text is divided into three chapters. In the first, Aristotle tries to determine whether dreams "pertain to the faculty of thought or to that of sense-perception." In the second chapter, he considers the circumstances of sleep and how the sense organs operate. Finally, in the third chapter he explains how dreams are caused, proposing that it is the residual movements of the sensory organs that allow them to arise. Content Aristotle explains that during sleep there is an absence of external sensory stimulation. While sleeping with our eyes closed, the eyes are unable to see, and so in this respect we perceive nothing while asleep. He compares hallucinations to dreams, saying "...the faculty by which, in waking hours, we are subject to illusion when affected by disease, is identical with that which produces illusory effects in sleep." When awake and perceiving, to see or hear something incorrectly only occurs when one actually sees or hears something, thinking it to be something else. But in sleep, if it is still true that one does not see, hear, or experience sense perception in the normal way, then the faculty of sense, he reasons, must be affected in some different way. Ultimately, Aristotle concludes that dreaming is due to residual movements of the sensory organs. Some dreams, he says, may even be caused by indigestion: We must suppose that, like the little eddies which are formed in rivers, so the movements are each a continuous process, often remaining like what they were when first started, but often, too, broken, into other forms by collisions with obstacles. This gives the reason why no dreams occur in sleep after meals, or to sleepers who are extremely young, e.g., to infants. The movement in such cases is excessive, owing to the heat generated from the food. Hence, just as in a liquid, if one vehemently disturbs it, sometimes no reflected image appears, while at other times one appears, indeed, but utterly distorted, so as to seem quite unlike its original; while, when once the motion has ceased, the reflected images are clear and plain; in the same manner during sleep the images, or residuary images are clear and plain; in the same manner during sleep the images, or residuary movements, which are based upon the sensory impressions, become sometimes quite obliterated by the above described motion when too violent; while at other times the sights are indeed seen, but confused and weird, and the dreams are incoherent, like those of persons who are atrabilious, or feverish, or intoxicated with wine. For all such affections, being spirituous, cause much commotion and disturbance. Aristotle also describes the phenomenon of lucid dreaming, whereby the dreamer becomes aware that he is dreaming. Legacy The 17th century English philosopher Thomas Hobbes generally adopted Aristotle's view that dreams arise from continued movements of the sensory organs during sleep, writing that "dreames are caused by the distemper of some inward parts of the Body." He thought this explanation would further help in understanding different types of dreams, for example, "lying cold breedeth Dreams of Feare, and raiseth the thought and Image of some fearfull object." The neurologist Sigmund Freud cited Aristotle in his 1899 work, The Interpretation of Dreams, as the first to recognize that dreams "do not arise from supernatural manifestations but follow the laws of the human spirit." He held Aristotle's definition of dreams to be "the mental activity of the sleeper in so far as he is asleep." References Notes Sources External links On Dreams, translated by J. I. Beare HTML Greek text: Mikros apoplous Category:Works by Aristotle Category:Philosophical literature
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Monkey made to eat by just using its brain power London, May 29 (ANI): Scientists at the University of Pittsburgh School of Medicine have announced that a monkey in their experiments has been successful in moving a robotic arm to feed itself marshmallows and chunks of fruit by using signals from its brain. The researchers revealed that the monkey performed this task as its arms were restrained for the restrained. Explaining the significance of their study, the researchers said that it might benefit development of prosthetics for people with spinal cord injuries, and those with locked-in conditions like Lou Gehrigs disease or amyotrophic lateral sclerosis. Our immediate goal is to make a prosthetic device for people with total paralysis. Ultimately, our goal is to better understand brain complexity, Nature magazine quoted Dr. Andrew Schwartz, senior author and professor of neurobiology at the University of Pittsburgh School of Medicine, as saying. Now we are beginning to understand how the brain works using brain-machine interface technology. The more we understand about the brain, the better well be able to treat a wide range of brain disorders, everything from Parkinsons disease and paralysis to, eventually, Alzheimers disease and perhaps even mental illness, added Dr. Schwartz. The researcher revealed that the technology is based on computer software that interprets signals picked up by probes the width of a human hair. He revealed that the probes were inserted into neuronal pathways in the monkeys motor cortex, a brain region where voluntary movement originates as electrical impulses, during the study. Dr. Schwatz said that the software programmed with a mathematic algorithm evaluated the neurons collective activity, and then sent it to the arm, he added. As a result, he added, the arm carried out the actions the monkey intended to perform with its own limb. He said that the movements were fluid and natural, and that the monkey was found to regard the robotic device as part of its own body. The monkey learns by first observing the movement, which activates his brain cells as if he were doing it. Its a lot like sports training, where trainers have athletes first imagine that they are performing the movements they desire, he added. (ANI)
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As semiconductor technology continues to inch closer to practical limitations in terms of increases in clock speed, architects are increasingly focusing on parallelism in processor architectures to obtain performance improvements. At the integrated circuit device, or chip level, multiple processing cores are often disposed on the same chip, functioning in much the same manner as separate processor chips, or to some extent, as completely separate computers. In addition, even within cores, parallelism is employed through the use of multiple execution units that are specialized to handle certain types of operations. Pipelining is also employed in many instances so that certain operations that may take multiple clock cycles to perform are broken up into stages, enabling other operations to be started prior to completion of earlier operations. Multithreading is also employed to enable multiple instruction streams to be processed in parallel, enabling more overall work to performed in any given clock cycle. The net result of applying the aforementioned techniques is an ability to provide multithreaded processing environment with a pool of hardware threads distributed among one or more processing cores in one or more processor chips and in one or more computers, and capable of processing a plurality of instruction streams in parallel. It is expected that as technology increases, processor architectures will be able to support hundreds or thousands of hardware threads, and when multiple processors are combined into high performance computing systems such as supercomputers and massively parallel computers, a potential exists to support millions of hardware threads. However, effective parallel processing requires that the software applications that run in a multithreaded processing environment take suitable advantage of multithreading capabilities. Software developers are typically more comfortable with developing single threaded applications since they typically follow the sequences of steps needed to perform desired tasks. Support for multithreading is often not as intuitive, and often requires consideration for minimizing conflicts and dependencies to minimize the frequency that threads may spend waiting for other threads to complete work that they need before they can complete their own work. For example, if one thread needs to calculate an average of some set of values that are being calculated by other threads, that thread will not be able to perform its operation until all of the other threads calculate their respective values. Threads that perform completely independent tasks, on the other hand, typically do not suffer from dependency concerns, so much of the effort associated with developing for multithreaded applications is devoted to breaking tasks up into relatively independent threads so that inter-thread dependencies are minimized. Given the difficulties associated with developing multithreaded applications, a significant need has existed in the art for techniques for simplifying the development of multithreaded applications. For example, significant efforts have been made to programmatically convert single threaded application code into multithreaded application code during compilation, e.g., using an optimizing compiler. With one methodology, for example, fine grained parallelism is employed to convert in-order code in an instruction stream into multiple, small out-of-order code segments, and instructions are inserted into the instruction streams to pass data between the code segments in the form of variables. One type of instruction is a “put” instruction, which sends a variable to another thread, and another type of instruction is a “get” instruction, which retrieves a variable from another thread. Through the use of these instructions, synchronization between code segments executing on multiple threads can be maintained by stalling a code segment that has issued a get statement for a particular variable until another code segment has issued a corresponding put instruction for that variable. While the use of put and get instructions can effectively maintain synchronization between dependent code segments executing on different hardware threads, any time that a thread is stalled waiting for a variable from another thread represents lost productivity, so it is desirable to minimize the latency associated with communicating variables between threads. Therefore, a significant need exists in the art for a manner of efficiently communicating data between multiple threads in a multithreaded processing environment to minimize latencies for inter-thread dependencies.
3.15625
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SLAVERY IN FOCUS January 16, 2013 The history of slavery is outside my immediate compass since I do not watch contemporary films. My ancestors (I imagine) were either indigenous inhabitants of the islands on the North West coast of the Eurasian landmass,or conceivably they might have been part of the extraordinary migration of boat people from the mainland, who might then have been captured by the Feudal System, which underpinned the conflict there over rights in the 17th Century. I have some experience of wage slavery, of course, and it bears repetition that modern corporations are not fundamentally democratic, which in the very least is deeply contradictory. Perhaps this observation might not be coincidental. History is often reduced to a mythical narrative. I have been criticized, probably correctly, for dabbling in this activity. Some myths, even if contradicted by very apparent evidence, both then and now, such as the Egalitarian Myth may be on balance be positive. However, it is more important to recognize the humanity of all people, and therefor their human potentials. Imara Jones at Colorlines, via Alternet, identifies her list of ten top things everybody should know about the economic history of slavery in the US: 1) Slavery laid the foundation for the modern international economic system. The massive infrastructure required to move 8 to 10 million Africans halfway around the world built entire cities in England and France, such as Liverpool, Manchester and Bordeaux. It was key to London’s emergence as a global capital of commerce, and spurred New York’s rise as a center of finance. The industry to construct, fund, staff, and administer the thousands of ships which made close to 50,000 individual voyages was alone a herculean task. The international financial and distribution networks required to coordinate, maintain and profit from slavery set the framework for the modern global economy. 2) Africans’ economic skills were a leading reason for their enslavement. Africans possessed unique expertise which Europeans required to make their colonial ventures successful. Africans knew how to grow and cultivate crops in tropical and semi-tropical climates. African rice growers, for instance, were captured in order to bring their agricultural knowledge to America’s sea islands and those of the Caribbean. Many West African civilizations possessed goldsmiths and expert metal workers on a grand scale. These slaves were snatched to work in Spanish and Portuguese gold and silver mines throughout Central and South America. Contrary to the myth of unskilled labor, large numbers of Africans were anything but. 3) African know-how transformed slave economies into some of the wealthiest on the planet. The fruits of the slave trade funded the growth of global empires. The greatest source of wealth for imperial France was the “white gold” of sugar produced by Africans in Haiti. More riches flowed to Britain from the slave economy of Jamaica than all of the original American 13 colonies combined. Those resources underwrote the Industrial Revolution and vast improvements in Western Europe’s economic infrastructure. 4) Until it was destroyed by the Civil War, slavery made the American South the richest and most powerful region in America. Slavery was a national enterprise, but the economic and political center of gravity during the U.S.’s first incarnation as a slave republic was the South. This was true even during the colonial era. Virginia was its richest colony and George Washington was one of its wealthiest people because of his slaves. The majority of the new country’s presidents and Supreme Court justices were Southerners. However, the invention of the cotton gin took the South’s national economic dominance and transformed it into a global phenomenon. British demand for American cotton, as I have written before, made the southern stretch of the Mississippi River the Silicon Valley of its era. The single largest concentration of America’s millionaires was gathered in plantations along the Mississippi’s banks. The first and only president of the Confederacy—Jefferson Davis—was a Mississippi, millionaire slave holder. 5) Defense of slavery, more than taxes, was pivotal to America’s declaration of independence. The South had long resisted Northern calls to leave the British Empire. That’s because the South sold most of its slave-produced products to Britain and relied on the British Navy to protect the slave trade. But a court case in England changed all of that. In 1775, a British court ruled that slaves could not be held in the United Kingdom against their will. Fearing that the ruling would apply to the American colonies, the Southern planters swung behind the Northern push for greater autonomy. In 1776, one year later, America left its former colonial master. The issue of slavery was so powerful that it changed the course of history. 6) The brutalization and psychological torture of slaves was designed to ensure that plantations stayed in the black financially. Slave revolts and acts of sabotage were relatively common on Southern plantations. As economic enterprises, the disruption in production was bad for business. Over time a system of oppression emerged to keep things humming along. This centered on singling out slaves for public torture who had either participated in acts of defiance or who tended towards noncompliance. In fact, the most recalcitrant slaves were sent to institutions, such as the “Sugar House” in Charleston, S.C., where cruelty was used to elicit cooperation. Slavery’s most inhumane aspects were just another tool to guarantee the bottom line. 7) The economic success of former slaves during Reconstruction led to the rise of the Ku Klux Klan. In less than 10 years after the end of slavery, blacks created thriving communities and had gained political power—including governorships and Senate seats—across the South. Former slaves, such Atlanta’s Alonzo Herndon, had even become millionaires in the post-war period. But the move towards black economic empowerment had upset the old economic order. Former planters organized themselves into White Citizens Councils and created an armed wing—the Ku Klux Klan—to undermine black economic institutions and to force blacks into sharecropping on unfair terms. Isabel Wilkerson’s Pulitzer Prize-winning book, “The Warmth of Other Suns”, details the targeting of black individuals, as well as entire black communities, for acts of terror whose purpose was to enforce economic apartheid. 8) The desire to maintain economic oppression is why the South was one of the most anti-tax regions of the nation. Before the Civil War, the South routinely blocked national infrastructure protects. These plans, focused on Northern and Western states, would have moved non-slave goods to market quickly and cheaply. The South worried that such investments would increase the power of the free-labor economy and hurt their own, which was based on slavery. Moreover, the South was vehemently opposed to taxes even to improve the lives of non-slaveholding white citizens. The first public school in the North, Boston Latin, opened its doors in the mid-1600s. The first public school in the South opened 200 years later. Maintenance of slavery was the South’s top priority to the detriment of everything else. 9) Many firms on Wall Street made fortunes from funding the slave trade. Investment in slavery was one of the most profitable economic activities throughout most of New York’s 350 year history. Much of the financing for the slave economy flowed through New York banks. Marquee names such as JP Morgan Chase and New York Life all profited greatly from slavery. Lehman Brothers, one of Wall Street’s largest firms until 2008, got its start in the slave economy of Alabama. Slavery was so important to the city that New York was one the most pro-slavery urban municipalities in the North. 10) The wealth gap between whites and blacks, the result of slavery, has yet to be closed. The total value of slaves, or “property” as they were then known, could exceed $12 million in today’s dollars on the largest plantations. With land, machinery, crops and buildings added in, the wealth of southern agricultural enterprises was truly astronomical. Yet when slavery ended, the people that generated the wealth received nothing. The contention that outright theft, rather than the workings of the price system in a free market, was the primary engine of economic wealth in the West will have some ideologues frothing. But if the “market” was so great, why was slavery necessary and why was it maintained. Whatever else it may be slavery is a system of economic and social violence. The History of Slavery in the US provides an overview from the 17th Century to Reconstruction, including reference to Frederick Douglass, Harriet Tubman and James Brown: Related articles The real reason the Second Amendment was ratified, and why it says “State” instead of “Country” (the Framers knew the difference – see the 10th Amendment), was to preserve the slave patrol militias in the southern states, which was necessary to get Virginia’s vote. Founders Patrick Henry, George Mason, and James Madison were totally clear on that . . . and we all should be too. So this contention seems credible, and so it is very significant given the current fervour among many gun ownership advocates. Related With just one click, your heavy garage doors will open, without you having to touch the door. It often comes in two varieties one with dual flexible sides and one that has a hard side and a flexible side that looks a lot like wood molding. Just as you did before, watch for any glowing items, since you’ll want to be able to build a new lock grinder in a moment.
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