Mercurial > repos > nick > allele_counts_1
view allele-counts.py @ 21:1fc7bef38c5f draft default tip
"planemo upload for repository https://github.com/galaxyproject/dunovo commit ac9577f0047ad984b307fe2c4b40e2eb45a0e6e2-dirty"
| author | nick |
|---|---|
| date | Fri, 03 Apr 2020 19:47:34 +0000 |
| parents | 44c3abd1b767 |
| children |
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#!/usr/bin/python3 """ Run with -h option or see DESCRIPTION for description. This script's functionality is being obsoleted by the new, and much more sanely written, nvc-filter.py. New in this version: - Calculate strand bias - Rename MINOR.FREQ.PERC to MAF Naive Variant Caller variant count parsing one-liner: $ cat variants.vcf | grep -v '^#' | cut -f 10 | cut -d ':' -f 4 | tr ',=' '\t:' """ import os import sys import errno import random from optparse import OptionParser COLUMNS = ['sample', 'chr', 'pos', 'A', 'C', 'G', 'T', 'coverage', 'alleles', 'major', 'minor', 'freq', 'bias'] COLUMN_LABELS = ['SAMPLE', 'CHR', 'POS', 'A', 'C', 'G', 'T', 'CVRG', 'ALLELES', 'MAJOR', 'MINOR', 'MAF', 'BIAS'] CANONICAL_VARIANTS = ['A', 'C', 'G', 'T'] USAGE = """Usage: %prog [options] -i variants.vcf -o alleles.tsv cat variants.vcf | %prog [options] > alleles.tsv""" OPT_DEFAULTS = {'infile':'-', 'outfile':'-', 'freq_thres':1.0, 'covg_thres':100, 'print_header':False, 'stdin':False, 'stranded':False, 'no_filter':False, 'debug_loc':'', 'seed':''} DESCRIPTION = """This will parse the VCF output of the "Naive Variant Caller" (aka "BAM Coverage") Galaxy tool. For each position reported, it counts the number of reads of each base, determines the major allele, minor allele (second most frequent variant), and number of alleles above a threshold. So currently it only considers SNVs (ACGT), including in the coverage figure. By default it reads from stdin and prints to stdout. Prints a tab-delimited set of statistics to stdout. To print output column labels, run "$ echo -n | ./allele-counts.py -H". The columns are: 1:SAMPLE 2:CHR 3:POS 4:A 5:C 6:G 7:T 8:CVRG 9:ALLELES 10:MAJOR 11:MINOR 12:MAF 13:BIAS, unless the --stranded option is used, in which case they are: 1:SAMPLE 2:CHR 3:POS 4:+A 5:+C 6:+G 7:+T 8:-A 9:-C 10:-G 11:-T 12:CVRG 13:ALLELES 14:MAJOR 15:MINOR 16:MAF 17:BIAS. """ EPILOG = """Requirements: The input VCF must report the variants for each strand. The variants should be case-sensitive (e.g. all capital base letters). Strand bias: Both strands must show the same bases passing the frequency threshold (but not necessarily in the same order). If the site fails this test, the number of alleles is reported as 0.""" def get_options(defaults, usage, description='', epilog=''): """Get options, print usage text.""" parser = OptionParser(usage=usage, description=description, epilog=epilog) parser.add_option('-i', '--infile', dest='infile', default=defaults.get('infile'), help='Read input VCF data from this file instead of stdin.') parser.add_option('-o', '--outfile', dest='outfile', default=defaults.get('outfile'), help='Print output data to this file instead of stdout.') parser.add_option('-f', '--freq-thres', dest='freq_thres', type='float', default=defaults.get('freq_thres'), help=('Frequency threshold for counting alleles, given in percentage: -f 1 ' +'= 1% frequency. Default is %default%.')) parser.add_option('-c', '--covg-thres', dest='covg_thres', type='int', default=defaults.get('covg_thres'), help=('Coverage threshold. Each site must be supported by at least this ' +'many reads on each strand. Otherwise the site will not be printed in ' +'the output. The default is %default reads per strand.')) parser.add_option('-n', '--no-filter', dest='no_filter', action='store_const', const=not(defaults.get('no_filter')), default=defaults.get('no_filter'), help=('Operate without a frequency threshold or coverage threshold. ' +'Equivalent to "-c 0 -f 0".')) parser.add_option('-H', '--header', dest='print_header', action='store_const', const=not(defaults.get('print_header')), default=defaults.get('print_header'), help=('Print header line. This is a #-commented line with the column ' +'labels. Off by default.')) parser.add_option('-s', '--stranded', dest='stranded', action='store_const', const=not(defaults.get('stranded')), default=defaults.get('stranded'), help='Report variant counts by strand, in separate columns. Off by default.') parser.add_option('-r', '--rand-seed', dest='seed', default=defaults.get('seed'), help=('Seed for random number generator.')) parser.add_option('-d', '--debug', dest='debug_loc', default=defaults.get('debug_loc'), help=('Turn on debug mode and specify a single site to process using UCSC ' +'coordinate format. You can also append a sample ID after another ":" ' +'to restrict it further.')) (options, args) = parser.parse_args() return (options, args) def main(): (options, args) = get_options(OPT_DEFAULTS, USAGE, DESCRIPTION, EPILOG) infile = options.infile outfile = options.outfile print_header = options.print_header freq_thres = options.freq_thres / 100 covg_thres = options.covg_thres stranded = options.stranded debug_loc = options.debug_loc seed = options.seed if options.no_filter: freq_thres = 0 covg_thres = 0 if seed: random.seed(seed) debug = False print_sample = '' if debug_loc: debug = True coords = debug_loc.split(':') print_chr = coords[0] print_pos = '' if len(coords) > 1: print_pos = coords[1] if len(coords) > 2: print_sample = coords[2] # set infile_handle to either stdin or the input file if infile == OPT_DEFAULTS.get('infile'): infile_handle = sys.stdin sys.stderr.write("Reading from standard input..\n") else: if os.path.exists(infile): infile_handle = open(infile, 'r') else: fail('Error: Input VCF file '+infile+' not found.') # set outfile_handle to either stdout or the output file if outfile == OPT_DEFAULTS.get('outfile'): outfile_handle = sys.stdout else: try: outfile_handle = open(outfile, 'w') except IOError: fail('Error: The given output filename '+outfile+' could not be opened.') # Take care of column names, print header if len(COLUMNS) != len(COLUMN_LABELS): fail('Error: Internal column names list do not match column labels list.') if stranded: COLUMNS[3:7] = ['+A', '+C', '+G', '+T', '-A', '-C', '-G', '-T'] COLUMN_LABELS[3:7] = ['+A', '+C', '+G', '+T', '-A', '-C', '-G', '-T'] if print_header: outfile_handle.write('#'+'\t'.join(COLUMN_LABELS)+"\n") # main loop # each iteration processes one VCF line and prints one or more output lines # one VCF line = one site, one or more samples # one output line = one site, one sample sample_names = [] for line in infile_handle: line = line.rstrip('\r\n') # header lines if line[0] == '#': if line[0:6].upper() == '#CHROM': sample_names = line.split('\t')[9:] continue if not sample_names: fail("Error in input VCF: Data line encountered before header line. " +"Failed on line:\n"+line) site_data = read_site(line, sample_names, CANONICAL_VARIANTS) if debug: if print_pos != site_data['pos']: continue if print_chr != site_data['chr'] and print_chr != '': continue if print_sample != '': for sample in site_data['samples'].keys(): if sample.lower() != print_sample.lower(): site_data['samples'].pop(sample, None) if len(site_data['samples']) == 0: sys.stderr.write("Error: Sample '"+print_sample+"' not found.\n") sys.exit(1) site_summary = summarize_site(site_data, sample_names, CANONICAL_VARIANTS, freq_thres, covg_thres, stranded, debug=debug) if debug and site_summary[0]['print']: print(line.split('\t')[9].split(':')[-1]) try: print_site(outfile_handle, site_summary, COLUMNS) except IOError as ioe: if ioe.errno == errno.EPIPE: sys.exit(0) # keeps Galaxy from giving an error if there were messages on stderr sys.exit(0) def read_site(line, sample_names, canonical): """Read in a line, parse the variants into a data structure, and return it. The line should be actual site data, not a header line, so check beforehand. Only the variants in 'canonical' will be read; all others are ignored. Note: the line is assumed to have been chomped. The returned data is stored in a dict, with the following structure: { 'chr': 'chr1', 'pos': '2617', 'samples': { 'THYROID': { '+A': 32, '-A': 45, '-G': 1, }, 'BLOOD': { '+A': 2, '-C': 1, '+G': 37, '-G': 42, }, }, } """ site = {} fields = line.split('\t') if len(fields) < 9: fail("Error in input VCF: wrong number of fields in data line. " "Failed on line:\n"+line) site['chr'] = fields[0] site['pos'] = fields[1] samples = fields[9:] if len(samples) < len(sample_names): fail("Error in input VCF: missing sample fields in data line. " "Failed on line:\n"+line) elif len(samples) > len(sample_names): fail("Error in input VCF: more sample fields in data line than in header. " "Failed on line:\n"+line) sample_counts = {} for i in range(len(samples)): variant_counts = {} counts = samples[i].split(':')[-1] counts = counts.split(',') for count in counts: if not count or count == '.': continue fields = count.split('=') if len(fields) != 2: fail("Error in input VCF: Incorrect variant data format (must contain " "a single '='). Failed on data \"{}\" in line:\n{}" .format(count, line)) (variant, reads) = fields if variant[1:] not in canonical: continue if not variant.startswith('-') and not variant.startswith('+'): fail("Error in input VCF: variant data not strand-specific. Failed on " "data \"{}\" on line:\n{}".format(variant, line)) try: variant_counts[variant] = int(float(reads)) except ValueError: fail("Error in input VCF: Variant count not a valid number. Failed on " "variant count string \"{}\"\nIn the following line:\n{}" .format(reads, line)) sample_counts[sample_names[i]] = variant_counts site['samples'] = sample_counts return site def summarize_site(site, sample_names, canonical, freq_thres, covg_thres, stranded=False, debug=False): """Take the raw data from the VCF line and transform it into the summary data to be printed in the output format.""" site_summary = [] for sample_name in sample_names: sample = {'print':False} variants = site['samples'].get(sample_name) sample['sample'] = sample_name sample['chr'] = site['chr'] sample['pos'] = site['pos'] coverage = sum(variants.values()) # get stranded coverage covg_plus = 0 covg_minus = 0 for variant in variants: if variant[0] == '+': covg_plus += variants[variant] elif variant[0] == '-': covg_minus += variants[variant] # stranded coverage threshold if covg_plus < covg_thres or covg_minus < covg_thres: site_summary.append(sample) continue else: sample['print'] = True # get an ordered list of read counts for all variants (both strands) bases = get_read_counts(variants, '+-') ranked_bases = process_read_counts(bases, sort=True, debug=debug) # prepare stranded or unstranded lists of base counts base_count_lists = [] if stranded: strands = ['+', '-'] base_count_lists.append(get_read_counts(variants, '+')) base_count_lists.append(get_read_counts(variants, '-')) else: strands = [''] base_count_lists.append(ranked_bases) # record read counts into output dict # If stranded, this will loop twice, once for each strand, and prepend '+' # or '-' to the base name. If not stranded, it will loop once, and prepend # nothing (''). for (strand, base_count_list) in zip(strands, base_count_lists): for base_count in base_count_list: sample[strand+base_count[0]] = base_count[1] # fill in any zeros for base in canonical: if strand+base not in sample: sample[strand+base] = 0 sample['alleles'] = count_alleles(variants, freq_thres, debug=debug) # If there's a tie for 2nd, randomly choose one to be 2nd if len(ranked_bases) >= 3 and ranked_bases[1][1] == ranked_bases[2][1]: swap = random.choice([True,False]) if swap: tmp_base = ranked_bases[1] ranked_bases[1] = ranked_bases[2] ranked_bases[2] = tmp_base if debug: print("ranked +-: "+str(ranked_bases)) sample['coverage'] = coverage try: sample['major'] = ranked_bases[0][0] except IndexError: sample['major'] = '.' try: sample['minor'] = ranked_bases[1][0] sample['freq'] = round(ranked_bases[1][1]/coverage, 5) except IndexError: sample['minor'] = '.' sample['freq'] = 0.0 # Now that we've decided major and minor, we can calculate strand bias bias = get_strand_bias(sample, variants) if bias is None: sample['bias'] = '.' else: sample['bias'] = round(bias, 5) site_summary.append(sample) return site_summary def get_read_counts(stranded_counts, strands='+-'): """Do a simple sum of the read counts per variant, on the specified strands. Arguments: stranded_counts: Dict of the stranded variants (keys) and their read counts (values). strands: Which strand(s) to count. Can be '+', '-', or '+-' for both (default). Return value: summed_counts: A list of the alleles and their read counts. The elements are tuples (variant, read count).""" variants = stranded_counts.keys() summed_counts = {} for variant in variants: strand = variant[0] base = variant[1:] if strand in strands: summed_counts[base] = stranded_counts[variant] + summed_counts.get(base, 0) return list(summed_counts.items()) def process_read_counts(variant_counts, freq_thres=0, sort=False, debug=False): """Process a list of read counts by frequency filtering and/or sorting. Arguments: variant_counts: List of the non-stranded variants and their read counts. The elements are tuples (variant, read count). freq_thres: The frequency threshold each allele needs to pass to be included. sort: Whether to sort the list in descending order of read counts. Return value: variant_counts: A list of the processed alleles and their read counts. The elements are tuples (variant, read count).""" # get coverage for the specified strands coverage = 0 for variant in variant_counts: coverage += variant[1] if coverage <= 0: return [] # sort the list of alleles by read count if sort: variant_counts.sort(reverse=True, key=lambda variant: variant[1]) if debug: print('coverage: '+str(coverage)+', freq_thres: '+str(freq_thres)) for variant in variant_counts: print((variant[0]+': '+str(variant[1])+'/'+str(float(coverage))+' = '+ str(variant[1]/coverage))) # remove bases below the frequency threshold if freq_thres > 0: variant_counts = [variant for variant in variant_counts if variant[1]/coverage >= freq_thres] return variant_counts def count_alleles(variant_counts, freq_thres, debug=False): """Determine how many alleles to report, based on filtering rules. The current rule determines which bases pass the frequency threshold on each strand individually, then compares the two sets of bases. If they are the same (regardless of order), the allele count is the number of bases. Otherwise it is zero.""" allele_count = 0 alleles_plus = get_read_counts(variant_counts, '+') alleles_plus = process_read_counts(alleles_plus, freq_thres=freq_thres, sort=False, debug=debug) alleles_minus = get_read_counts(variant_counts, '-') alleles_minus = process_read_counts(alleles_minus, freq_thres=freq_thres, sort=False, debug=debug) if debug: print('+ '+str(alleles_plus)) print('- '+str(alleles_minus)) # Check if each strand reports the same set of alleles. # Sorting by base is to compare lists without regard to order (as sets). alleles_plus_sorted = sorted([base[0] for base in alleles_plus if base[1]]) alleles_minus_sorted = sorted([base[0] for base in alleles_minus if base[1]]) if alleles_plus_sorted == alleles_minus_sorted: allele_count = len(alleles_plus) return allele_count def get_strand_bias(sample, variants): """Based on method 1 (SB) of Guo et al., 2012 If there a denominator would be 0, there is no valid result and this will return None. This occurs when there are no reads on one of the strands, or when there are no minor allele reads.""" # using same variable names as in paper a = variants.get('+'+sample['major'], 0) # forward major allele b = variants.get('+'+sample['minor'], 0) # forward minor allele c = variants.get('-'+sample['major'], 0) # reverse major allele d = variants.get('-'+sample['minor'], 0) # reverse minor allele # no minor allele reads try: return abs(b/(a+b) - d/(c+d)) / ((b+d) / (a+b+c+d)) except ZeroDivisionError: return None def print_site(filehandle, site, columns): """Print the output lines for one site (one per sample). filehandle must be open.""" for sample in site: if sample['print']: fields = [str(sample.get(column)) for column in columns] filehandle.write('\t'.join(fields)+"\n") def fail(message): sys.stderr.write(message+'\n') sys.exit(1) if __name__ == "__main__": main()