Spaces:

NiniCat
/

CRISPRTool

Sleeping

File size: 9,596 Bytes

import tensorflow as tf
from keras import regularizers
from keras.layers import Input, Dense, Dropout, Activation, Conv1D
from keras.layers import GlobalAveragePooling1D, AveragePooling1D
from keras.layers import Bidirectional, LSTM
from keras import Model
from keras.metrics import MeanSquaredError

import pandas as pd
import numpy as np

import requests
from functools import reduce
from operator import add
import tabulate
from difflib import SequenceMatcher
from Bio import SeqIO
from Bio.SeqRecord import SeqRecord
from Bio.SeqFeature import SeqFeature, FeatureLocation
from Bio.Seq import Seq

import cyvcf2
import parasail

import re

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 BiLSTM_model(input_shape):
    input = Input(shape=input_shape)

    conv1 = Conv1D(128, 5, activation="relu")(input)
    pool1 = AveragePooling1D(2)(conv1)
    drop1 = Dropout(0.1)(pool1)

    conv2 = Conv1D(128, 5, activation="relu")(drop1)
    pool2 = AveragePooling1D(2)(conv2)
    drop2 = Dropout(0.1)(pool2)

    lstm1 = Bidirectional(LSTM(128,
                               dropout=0.1,
                               activation='tanh',
                               return_sequences=True,
                               kernel_regularizer=regularizers.l2(1e-4)))(drop2)
    avgpool = GlobalAveragePooling1D()(lstm1)

    dense1 = Dense(128,
                   kernel_regularizer=regularizers.l2(1e-4),
                   bias_regularizer=regularizers.l2(1e-4),
                   activation="relu")(avgpool)
    drop3 = Dropout(0.1)(dense1)

    dense2 = Dense(32,
                   kernel_regularizer=regularizers.l2(1e-4),
                   bias_regularizer=regularizers.l2(1e-4),
                   activation="relu")(drop3)
    drop4 = Dropout(0.1)(dense2)

    dense3 = Dense(32,
                   kernel_regularizer=regularizers.l2(1e-4),
                   bias_regularizer=regularizers.l2(1e-4),
                   activation="relu")(drop4)
    drop5 = Dropout(0.1)(dense3)

    output = Dense(1, activation="linear")(drop5)

    model = Model(inputs=[input], outputs=[output])
    return model

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, end, strand, transcript_id, exon_id, pam="TTTN", target_length=34):
    targets = []
    len_sequence = len(sequence)
    #complement = {'A': 'T', 'T': 'A', 'C': 'G', 'G': 'C'}
    dnatorna = {'A': 'A', 'T': 'U', 'C': 'C', 'G': 'G'}

    for i in range(len_sequence - target_length + 1):
        target_seq = sequence[i:i + target_length]
        if target_seq[4:7] == 'TTT':
            if strand == -1:
                tar_start = end - i - target_length + 1
                tar_end = end -i
                #seq_in_ref = ''.join([complement[base] for base in target_seq])[::-1]
            else:
                tar_start = start + i
                tar_end = start + i + target_length - 1
                #seq_in_ref = target_seq
            gRNA = ''.join([dnatorna[base] for base in target_seq[8:28]])
            targets.append([target_seq, gRNA, chr, str(tar_start), str(tar_end), str(strand), transcript_id, exon_id])
            #targets.append([target_seq, gRNA, chr, str(tar_start), str(tar_end), str(strand), transcript_id, exon_id, seq_in_ref])
    return targets

def format_prediction_output(targets, model_path):
    # Loading weights for the model
    Crispr_BiLSTM = BiLSTM_model(input_shape=(34, 4))
    Crispr_BiLSTM.load_weights(model_path)

    formatted_data = []
    for target in targets:
        # Predict
        encoded_seq = get_seqcode(target[0])
        prediction = float(list(Crispr_BiLSTM.predict(encoded_seq, verbose=0)[0])[0])
        if prediction > 100:
            prediction = 100

        # Format output
        gRNA = target[1]
        chr = target[2]
        start = target[3]
        end = target[4]
        strand = target[5]
        transcript_id = target[6]
        exon_id = target[7]
        #seq_in_ref = target[8]
        #formatted_data.append([chr, start, end, strand, transcript_id, exon_id, target[0], gRNA, seq_in_ref, prediction])
        formatted_data.append([chr, start, end, strand, transcript_id, exon_id, target[0], gRNA, prediction])

    return formatted_data


def process_gene(gene_symbol, model_path):
    transcripts = fetch_ensembl_transcripts(gene_symbol)
    results = []
    all_exons = []  # To accumulate all exons
    all_gene_sequences = []  # To accumulate all gene sequences

    if transcripts:
        for transcript in transcripts:
            Exons = transcript['Exon']
            all_exons.extend(Exons)  # Add all exons from this transcript to the list
            transcript_id = transcript['id']

            for Exon in Exons:
                exon_id = Exon['id']
                gene_sequence = fetch_ensembl_sequence(exon_id)
                if gene_sequence:
                    all_gene_sequences.append(gene_sequence)  # Add this gene sequence to the list
                    chr = Exon['seq_region_name']
                    start = Exon['start']
                    end = Exon['end']
                    strand = Exon['strand']

                    targets = find_crispr_targets(gene_sequence, chr, start, end, strand, transcript_id, exon_id)
                    if targets:
                        # Predict on-target efficiency for each gRNA site
                        formatted_data = format_prediction_output(targets, model_path)
                        results.extend(formatted_data)  # Flatten the results
                else:
                    print(f"Failed to retrieve gene sequence for exon {exon_id}.")
    else:
        print("Failed to retrieve transcripts.")

    output = []
    for result in results:
        for item in result:
            output.append(item)

    # Return the sorted output, combined gene sequences, and all exons
    return results, all_gene_sequences, all_exons

def create_genbank_features(data):
    features = []

    # If the input data is a DataFrame, convert it to a list of lists
    if isinstance(data, pd.DataFrame):
        formatted_data = data.values.tolist()
    elif isinstance(data, list):
        formatted_data = data
    else:
        raise TypeError("Data should be either a list or a pandas DataFrame.")

    for row in formatted_data:
        try:
            start = int(row[1])
            end = int(row[2])
        except ValueError as e:
            print(f"Error converting start/end to int: {row[1]}, {row[2]} - {e}")
            continue

        strand = 1 if row[3] == '+' else -1
        location = FeatureLocation(start=start, end=end, strand=strand)
        feature = SeqFeature(location=location, type="misc_feature", qualifiers={
            'label': row[7],  # Use gRNA as the label
            'note': f"Prediction: {row[8]}"  # Include the prediction score
        })
        features.append(feature)

    return features


def generate_genbank_file_from_df(df, gene_sequence, gene_symbol, output_path):
    # Ensure gene_sequence is a string before creating Seq object
    if not isinstance(gene_sequence, str):
        gene_sequence = str(gene_sequence)

    features = create_genbank_features(df)

    # Now gene_sequence is guaranteed to be a string, suitable for Seq
    seq_obj = Seq(gene_sequence)
    record = SeqRecord(seq_obj, id=gene_symbol, name=gene_symbol,
                       description=f'CRISPR Cas12 predicted targets for {gene_symbol}', features=features)
    record.annotations["molecule_type"] = "DNA"
    SeqIO.write(record, output_path, "genbank")


def create_bed_file_from_df(df, output_path):
    with open(output_path, 'w') as bed_file:
        for index, row in df.iterrows():
            chrom = row["Chr"]
            start = int(row["Start Pos"])
            end = int(row["End Pos"])
            strand = '+' if row["Strand"] == '1' else '-'
            gRNA = row["gRNA"]
            score = str(row["Prediction"])
            # transcript_id is not typically part of the standard BED columns but added here for completeness
            transcript_id = row["Transcript"]

            # Writing only standard BED columns; additional columns can be appended as needed
            bed_file.write(f"{chrom}\t{start}\t{end}\t{gRNA}\t{score}\t{strand}\n")


def create_csv_from_df(df, output_path):
    df.to_csv(output_path, index=False)