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from keras import Model | |
from keras.layers import Input | |
from keras.layers import Multiply | |
from keras.layers import Dense, Dropout, Activation, Flatten | |
from keras.layers import Convolution1D, AveragePooling1D | |
import pandas as pd | |
import numpy as np | |
import keras | |
import requests | |
from functools import reduce | |
from operator import add | |
from Bio.SeqRecord import SeqRecord | |
from Bio.SeqFeature import SeqFeature, FeatureLocation | |
from Bio.Seq import Seq | |
from Bio import SeqIO | |
ntmap = {'A': (1, 0, 0, 0), | |
'C': (0, 1, 0, 0), | |
'G': (0, 0, 1, 0), | |
'T': (0, 0, 0, 1) | |
} | |
def get_seqcode(seq): | |
return np.array(reduce(add, map(lambda c: ntmap[c], seq.upper()))).reshape((1, len(seq), -1)) | |
def Seq_DeepCpf1_model(input_shape): | |
Seq_deepCpf1_Input_SEQ = Input(shape=input_shape) | |
Seq_deepCpf1_C1 = Convolution1D(80, 5, activation='relu')(Seq_deepCpf1_Input_SEQ) | |
Seq_deepCpf1_P1 = AveragePooling1D(2)(Seq_deepCpf1_C1) | |
Seq_deepCpf1_F = Flatten()(Seq_deepCpf1_P1) | |
Seq_deepCpf1_DO1 = Dropout(0.3)(Seq_deepCpf1_F) | |
Seq_deepCpf1_D1 = Dense(80, activation='relu')(Seq_deepCpf1_DO1) | |
Seq_deepCpf1_DO2 = Dropout(0.3)(Seq_deepCpf1_D1) | |
Seq_deepCpf1_D2 = Dense(40, activation='relu')(Seq_deepCpf1_DO2) | |
Seq_deepCpf1_DO3 = Dropout(0.3)(Seq_deepCpf1_D2) | |
Seq_deepCpf1_D3 = Dense(40, activation='relu')(Seq_deepCpf1_DO3) | |
Seq_deepCpf1_DO4 = Dropout(0.3)(Seq_deepCpf1_D3) | |
Seq_deepCpf1_Output = Dense(1, activation='linear')(Seq_deepCpf1_DO4) | |
Seq_deepCpf1 = Model(inputs=[Seq_deepCpf1_Input_SEQ], outputs=[Seq_deepCpf1_Output]) | |
return Seq_deepCpf1 | |
# seq-ca model (DeepCpf1) | |
def DeepCpf1_model(input_shape): | |
DeepCpf1_Input_SEQ = Input(shape=input_shape) | |
DeepCpf1_C1 = Convolution1D(80, 5, activation='relu')(DeepCpf1_Input_SEQ) | |
DeepCpf1_P1 = AveragePooling1D(2)(DeepCpf1_C1) | |
DeepCpf1_F = Flatten()(DeepCpf1_P1) | |
DeepCpf1_DO1 = Dropout(0.3)(DeepCpf1_F) | |
DeepCpf1_D1 = Dense(80, activation='relu')(DeepCpf1_DO1) | |
DeepCpf1_DO2 = Dropout(0.3)(DeepCpf1_D1) | |
DeepCpf1_D2 = Dense(40, activation='relu')(DeepCpf1_DO2) | |
DeepCpf1_DO3 = Dropout(0.3)(DeepCpf1_D2) | |
DeepCpf1_D3_SEQ = Dense(40, activation='relu')(DeepCpf1_DO3) | |
DeepCpf1_Input_CA = Input(shape=(1,)) | |
DeepCpf1_D3_CA = Dense(40, activation='relu')(DeepCpf1_Input_CA) | |
DeepCpf1_M = Multiply()([DeepCpf1_D3_SEQ, DeepCpf1_D3_CA]) | |
DeepCpf1_DO4 = Dropout(0.3)(DeepCpf1_M) | |
DeepCpf1_Output = Dense(1, activation='linear')(DeepCpf1_DO4) | |
DeepCpf1 = Model(inputs=[DeepCpf1_Input_SEQ, DeepCpf1_Input_CA], outputs=[DeepCpf1_Output]) | |
return DeepCpf1 | |
def fetch_ensembl_transcripts(gene_symbol): | |
url = f"https://rest.ensembl.org/lookup/symbol/homo_sapiens/{gene_symbol}?expand=1;content-type=application/json" | |
response = requests.get(url) | |
if response.status_code == 200: | |
gene_data = response.json() | |
if 'Transcript' in gene_data: | |
return gene_data['Transcript'] | |
else: | |
print("No transcripts found for gene:", gene_symbol) | |
return None | |
else: | |
print(f"Error fetching gene data from Ensembl: {response.text}") | |
return None | |
def fetch_ensembl_sequence(transcript_id): | |
url = f"https://rest.ensembl.org/sequence/id/{transcript_id}?content-type=application/json" | |
response = requests.get(url) | |
if response.status_code == 200: | |
sequence_data = response.json() | |
if 'seq' in sequence_data: | |
return sequence_data['seq'] | |
else: | |
print("No sequence found for transcript:", transcript_id) | |
return None | |
else: | |
print(f"Error fetching sequence data from Ensembl: {response.text}") | |
return None | |
def find_crispr_targets(sequence, chr, start, strand, pam="TTTN", target_length=34): | |
targets = [] | |
len_sequence = len(sequence) | |
for i in range(len_sequence - target_length + 1): | |
target_seq = sequence[i:i + target_length] | |
if target_seq[4:7] == 'TTT': | |
tar_start = start + i | |
tar_end = start + i + target_length | |
gRNA = target_seq[8:28] | |
targets.append([target_seq, gRNA, chr, str(tar_start), str(tar_end), str(strand)]) | |
return targets | |
def format_prediction_output(targets, seq_deepCpf1): | |
formatted_data = [] | |
for target in targets: | |
# Predict | |
encoded_seq = get_seqcode(target[0]) # 'target' seems to be the full sequence including PAM | |
prediction = seq_deepCpf1.predict(encoded_seq) | |
# Format output | |
gRNA = target[1] # gRNA is presumably the guide RNA sequence | |
chr = target[2] # Chromosome | |
start = target[3] # Start position | |
end = target[4] # End position | |
strand = target[5] # Strand | |
target_seq = target[0] # Full target sequence including PAM | |
formatted_data.append([chr, start, end, strand, target_seq, gRNA, prediction[0][0]]) | |
return formatted_data | |
def process_gene(gene_symbol, model_path): | |
transcripts = fetch_ensembl_transcripts(gene_symbol) | |
all_data = [] | |
gene_sequence = '' # Initialize an empty string for the gene sequence | |
# Load the model | |
seq_deepCpf1 = Seq_DeepCpf1_model(input_shape=(34, 4)) | |
seq_deepCpf1.load_weights(model_path) | |
if transcripts: | |
for transcript in transcripts: | |
transcript_id = transcript['id'] | |
chr = transcript.get('seq_region_name', 'unknown') | |
start = transcript.get('start', 0) | |
strand = transcript.get('strand', 'unknown') | |
# Fetch the sequence here and concatenate if multiple transcripts | |
gene_sequence += fetch_ensembl_sequence(transcript_id) or '' | |
if gene_sequence: | |
targets = find_crispr_targets(gene_sequence, chr, start, strand) | |
if targets: | |
formatted_data = format_prediction_output(targets, seq_deepCpf1) | |
all_data.extend(formatted_data) | |
else: | |
print("Failed to retrieve transcripts.") | |
return all_data, gene_sequence | |
def create_genbank_features(formatted_data): | |
features = [] | |
for data in formatted_data: | |
try: | |
# Attempt to convert start and end positions to integers | |
start = int(data[1]) | |
end = int(data[2]) | |
except ValueError as e: | |
# Log the error and skip this iteration if conversion fails | |
print(f"Error converting start/end to int: {data[1]}, {data[2]} - {e}") | |
continue # Skip this iteration | |
# Proceed as normal if conversion is successful | |
strand = 1 if data[3] == '+' else -1 | |
location = FeatureLocation(start=start, end=end, strand=strand) | |
feature = SeqFeature(location=location, type="misc_feature", qualifiers={ | |
'label': data[5], # gRNA as label | |
'note': f"Prediction: {data[6]}" # Prediction score in note | |
}) | |
features.append(feature) | |
return features | |
def generate_genbank_file_from_data(formatted_data, gene_sequence, gene_symbol, output_path): | |
features = create_genbank_features(formatted_data) | |
record = SeqRecord(Seq(gene_sequence), id=gene_symbol, name=gene_symbol, | |
description='CRISPR Cas12 predicted targets', features=features) | |
record.annotations["molecule_type"] = "DNA" | |
SeqIO.write(record, output_path, "genbank") | |
def create_csv_from_df(df, output_path): | |
df.to_csv(output_path, index=False) | |
def generate_bed_file_from_data(formatted_data, output_path): | |
with open(output_path, 'w') as bed_file: | |
for data in formatted_data: | |
try: | |
# Ensure data has the expected number of elements | |
if len(data) < 7: | |
raise ValueError("Incomplete data item") | |
chrom = data[0] | |
start = data[1] | |
end = data[2] | |
strand = '+' if data[3] == '+' else '-' | |
gRNA = data[5] | |
score = data[6] # Ensure this index exists | |
bed_file.write(f"{chrom}\t{start}\t{end}\t{gRNA}\t{score}\t{strand}\n") | |
except ValueError as e: | |
print(f"Skipping an item due to error: {e}") | |
continue |