diff vsnp_add_zero_coverage.py @ 0:0ad85e7db2fc draft

"planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/vsnp commit 6a0c9a857c1f4638ef18e106b1f8c0681303acc5"
author iuc
date Sun, 27 Sep 2020 10:07:44 +0000
parents
children aed013f6b13b
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--- /dev/null	Thu Jan 01 00:00:00 1970 +0000
+++ b/vsnp_add_zero_coverage.py	Sun Sep 27 10:07:44 2020 +0000
@@ -0,0 +1,188 @@
+#!/usr/bin/env python
+
+import argparse
+import multiprocessing
+import os
+import pandas
+import pysam
+import queue
+import re
+import shutil
+from Bio import SeqIO
+
+INPUT_BAM_DIR = 'input_bam_dir'
+INPUT_VCF_DIR = 'input_vcf_dir'
+OUTPUT_VCF_DIR = 'output_vcf_dir'
+OUTPUT_METRICS_DIR = 'output_metrics_dir'
+
+
+def get_base_file_name(file_path):
+    base_file_name = os.path.basename(file_path)
+    if base_file_name.find(".") > 0:
+        # Eliminate the extension.
+        return os.path.splitext(base_file_name)[0]
+    elif base_file_name.endswith("_vcf"):
+        # The "." character has likely
+        # changed to an "_" character.
+        return base_file_name.rstrip("_vcf")
+    return base_file_name
+
+
+def get_coverage_and_snp_count(task_queue, reference, output_metrics, output_vcf, timeout):
+    while True:
+        try:
+            tup = task_queue.get(block=True, timeout=timeout)
+        except queue.Empty:
+            break
+        bam_file, vcf_file = tup
+        # Create a coverage dictionary.
+        coverage_dict = {}
+        coverage_list = pysam.depth(bam_file, split_lines=True)
+        for line in coverage_list:
+            chrom, position, depth = line.split('\t')
+            coverage_dict["%s-%s" % (chrom, position)] = depth
+        # Convert it to a data frame.
+        coverage_df = pandas.DataFrame.from_dict(coverage_dict, orient='index', columns=["depth"])
+        # Create a zero coverage dictionary.
+        zero_dict = {}
+        for record in SeqIO.parse(reference, "fasta"):
+            chrom = record.id
+            total_len = len(record.seq)
+            for pos in list(range(1, total_len + 1)):
+                zero_dict["%s-%s" % (str(chrom), str(pos))] = 0
+        # Convert it to a data frame with depth_x
+        # and depth_y columns - index is NaN.
+        zero_df = pandas.DataFrame.from_dict(zero_dict, orient='index', columns=["depth"])
+        coverage_df = zero_df.merge(coverage_df, left_index=True, right_index=True, how='outer')
+        # depth_x "0" column no longer needed.
+        coverage_df = coverage_df.drop(columns=['depth_x'])
+        coverage_df = coverage_df.rename(columns={'depth_y': 'depth'})
+        # Covert the NaN to 0 coverage and get some metrics.
+        coverage_df = coverage_df.fillna(0)
+        coverage_df['depth'] = coverage_df['depth'].apply(int)
+        total_length = len(coverage_df)
+        average_coverage = coverage_df['depth'].mean()
+        zero_df = coverage_df[coverage_df['depth'] == 0]
+        total_zero_coverage = len(zero_df)
+        total_coverage = total_length - total_zero_coverage
+        genome_coverage = "{:.2%}".format(total_coverage / total_length)
+        # Process the associated VCF input.
+        column_names = ["CHROM", "POS", "ID", "REF", "ALT", "QUAL", "FILTER", "INFO", "FORMAT", "Sample"]
+        vcf_df = pandas.read_csv(vcf_file, sep='\t', header=None, names=column_names, comment='#')
+        good_snp_count = len(vcf_df[(vcf_df['ALT'].str.len() == 1) & (vcf_df['REF'].str.len() == 1) & (vcf_df['QUAL'] > 150)])
+        base_file_name = get_base_file_name(vcf_file)
+        if total_zero_coverage > 0:
+            header_file = "%s_header.csv" % base_file_name
+            with open(header_file, 'w') as outfile:
+                with open(vcf_file) as infile:
+                    for line in infile:
+                        if re.search('^#', line):
+                            outfile.write("%s" % line)
+            vcf_df_snp = vcf_df[vcf_df['REF'].str.len() == 1]
+            vcf_df_snp = vcf_df_snp[vcf_df_snp['ALT'].str.len() == 1]
+            vcf_df_snp['ABS_VALUE'] = vcf_df_snp['CHROM'].map(str) + "-" + vcf_df_snp['POS'].map(str)
+            vcf_df_snp = vcf_df_snp.set_index('ABS_VALUE')
+            cat_df = pandas.concat([vcf_df_snp, zero_df], axis=1, sort=False)
+            cat_df = cat_df.drop(columns=['CHROM', 'POS', 'depth'])
+            cat_df[['ID', 'ALT', 'QUAL', 'FILTER', 'INFO']] = cat_df[['ID', 'ALT', 'QUAL', 'FILTER', 'INFO']].fillna('.')
+            cat_df['REF'] = cat_df['REF'].fillna('N')
+            cat_df['FORMAT'] = cat_df['FORMAT'].fillna('GT')
+            cat_df['Sample'] = cat_df['Sample'].fillna('./.')
+            cat_df['temp'] = cat_df.index.str.rsplit('-', n=1)
+            cat_df[['CHROM', 'POS']] = pandas.DataFrame(cat_df.temp.values.tolist(), index=cat_df.index)
+            cat_df = cat_df[['CHROM', 'POS', 'ID', 'REF', 'ALT', 'QUAL', 'FILTER', 'INFO', 'FORMAT', 'Sample']]
+            cat_df['POS'] = cat_df['POS'].astype(int)
+            cat_df = cat_df.sort_values(['CHROM', 'POS'])
+            body_file = "%s_body.csv" % base_file_name
+            cat_df.to_csv(body_file, sep='\t', header=False, index=False)
+            if output_vcf is None:
+                output_vcf_file = os.path.join(OUTPUT_VCF_DIR, "%s.vcf" % base_file_name)
+            else:
+                output_vcf_file = output_vcf
+            with open(output_vcf_file, "w") as outfile:
+                for cf in [header_file, body_file]:
+                    with open(cf, "r") as infile:
+                        for line in infile:
+                            outfile.write("%s" % line)
+        else:
+            if output_vcf is None:
+                output_vcf_file = os.path.join(OUTPUT_VCF_DIR, "%s.vcf" % base_file_name)
+            else:
+                output_vcf_file = output_vcf
+            shutil.copyfile(vcf_file, output_vcf_file)
+        bam_metrics = [base_file_name, "", "%4f" % average_coverage, genome_coverage]
+        vcf_metrics = [base_file_name, str(good_snp_count), "", ""]
+        if output_metrics is None:
+            output_metrics_file = os.path.join(OUTPUT_METRICS_DIR, "%s.tabular" % base_file_name)
+        else:
+            output_metrics_file = output_metrics
+        metrics_columns = ["File", "Number of Good SNPs", "Average Coverage", "Genome Coverage"]
+        with open(output_metrics_file, "w") as fh:
+            fh.write("# %s\n" % "\t".join(metrics_columns))
+            fh.write("%s\n" % "\t".join(bam_metrics))
+            fh.write("%s\n" % "\t".join(vcf_metrics))
+        task_queue.task_done()
+
+
+def set_num_cpus(num_files, processes):
+    num_cpus = int(multiprocessing.cpu_count())
+    if num_files < num_cpus and num_files < processes:
+        return num_files
+    if num_cpus < processes:
+        half_cpus = int(num_cpus / 2)
+        if num_files < half_cpus:
+            return num_files
+        return half_cpus
+    return processes
+
+
+if __name__ == '__main__':
+    parser = argparse.ArgumentParser()
+
+    parser.add_argument('--output_metrics', action='store', dest='output_metrics', required=False, default=None, help='Output metrics text file')
+    parser.add_argument('--output_vcf', action='store', dest='output_vcf', required=False, default=None, help='Output VCF file')
+    parser.add_argument('--reference', action='store', dest='reference', help='Reference dataset')
+    parser.add_argument('--processes', action='store', dest='processes', type=int, help='User-selected number of processes to use for job splitting')
+
+    args = parser.parse_args()
+
+    # The assumption here is that the list of files
+    # in both INPUT_BAM_DIR and INPUT_VCF_DIR are
+    # equal in number and named such that they are
+    # properly matched if the directories contain
+    # more than 1 file (i.e., hopefully the bam file
+    # names and vcf file names will be something like
+    # Mbovis-01D6_* so they can be # sorted and properly
+    # associated with each other).
+    bam_files = []
+    for file_name in sorted(os.listdir(INPUT_BAM_DIR)):
+        file_path = os.path.abspath(os.path.join(INPUT_BAM_DIR, file_name))
+        bam_files.append(file_path)
+    vcf_files = []
+    for file_name in sorted(os.listdir(INPUT_VCF_DIR)):
+        file_path = os.path.abspath(os.path.join(INPUT_VCF_DIR, file_name))
+        vcf_files.append(file_path)
+
+    multiprocessing.set_start_method('spawn')
+    queue1 = multiprocessing.JoinableQueue()
+    num_files = len(bam_files)
+    cpus = set_num_cpus(num_files, args.processes)
+    # Set a timeout for get()s in the queue.
+    timeout = 0.05
+
+    # Add each associated bam and vcf file pair to the queue.
+    for i, bam_file in enumerate(bam_files):
+        vcf_file = vcf_files[i]
+        queue1.put((bam_file, vcf_file))
+
+    # Complete the get_coverage_and_snp_count task.
+    processes = [multiprocessing.Process(target=get_coverage_and_snp_count, args=(queue1, args.reference, args.output_metrics, args.output_vcf, timeout, )) for _ in range(cpus)]
+    for p in processes:
+        p.start()
+    for p in processes:
+        p.join()
+    queue1.join()
+
+    if queue1.empty():
+        queue1.close()
+        queue1.join_thread()