Mercurial > repos > dereeper > sniplay3
view VCFToolsFilter.pl @ 2:15319113c0a5 draft
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author | dereeper |
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date | Thu, 12 Feb 2015 15:54:24 -0500 |
parents | 9dec9f724a50 |
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#!/usr/bin/perl use strict; use Switch; use Getopt::Long; use Bio::SeqIO; my $usage = qq~Usage:$0 <args> [<opts>] where <args> are: -i, --input <VCF input> -o, --out <Output basename> <opts> are: -s, --samples <Samples to be analyzed. Comma separated list> -c, --chromosomes <Chromosomes to be analyzed. Comma separated list> -e, --export <Output format (VCF/freq/plink. Default: VCF> -f, --frequency <Minimum MAF. Default: 0.001> -m, --max_freq <Maximum MAF. Default: 0.5> -a, --allow_missing <Allowed missing data proportion per site. Must be comprised between 0 and 1. Default: 1> -n, --nb_alleles <Accepted number of alleles (min,max). Default: 2,4> -t, --type <Type of polymorphisms to keep (ALL/SNP/INDEL). Default: ALL> -b, --bounds <Lower bound and upper bound for a range of sites to be processed (start,end). Default: 1, 100000000> ~; $usage .= "\n"; my ($input,$out); #my $indel_size_max = 500; #my $indel_size_min = 1; my $frequency_max = 0.5; my $frequency_min = 0.001; my $pos_max = 100000000000; my $pos_min = 0; my $filter_snp_type = "all"; my $missing_data = 1; my $export = "VCF"; my $type = "ALL"; my $nb_alleles; my $bounds; my $samples; my $chromosomes; GetOptions( "input=s" => \$input, "out=s" => \$out, "samples=s" => \$samples, "chromosomes=s" => \$chromosomes, "frequency=s" => \$frequency_min, "max_freq=s" => \$frequency_max, "allow_missing=s"=> \$missing_data, "export=s" => \$export, "type=s" => \$type, "nb_alleles=s" => \$nb_alleles, "bounds=s" => \$bounds, ); die $usage if ( !$input || !$out); my @dnasamples; if ($samples) { @dnasamples = split(",",$samples); } my @nalleles; if ($nb_alleles) { @nalleles = split(",",$nb_alleles); } my @boundaries; if ($bounds) { @boundaries = split(",",$bounds); } my @chromosomes_list; if ($chromosomes) { @chromosomes_list = split(",",$chromosomes); } my $experiment = "chromosomes"; my $table = ""; my %genes; my @snp_ids; my @snp_ids_and_positions; my @snp_ids_and_positions_all; my $gene; my $snp_num = 0; my %ref_sequences; my %snps_of_gene; my $indiv_cmd = ""; if (@dnasamples) { $indiv_cmd = "--indv " . join(" --indv ",@dnasamples); } my $chrom_cmd = ""; if (@chromosomes_list) { $chrom_cmd = "--chr " . join(" --chr ",@chromosomes_list); } my $export_cmd = "--recode"; if ($export eq "freq") { $export_cmd = "--freq"; } if ($export eq "plink") { $export_cmd = "--plink"; } my $nb_alleles_cmd = "--min-alleles 1 --max-alleles 4"; if (@nalleles) { $nb_alleles_cmd = "--min-alleles $nalleles[0] --max-alleles $nalleles[1]"; } my $bounds_cmd = "--from-bp 1 --to-bp 100000000"; if (@boundaries) { $bounds_cmd = "--from-bp $boundaries[0] --to-bp $boundaries[1]"; } my $type_cmd = ""; if ($type eq "INDEL") { $type_cmd = "--keep-only-indels"; } if ($type eq "SNP") { $type_cmd = "--remove-indels"; } system("vcftools --vcf $input --out $out --keep-INFO-all --remove-filtered-all $type_cmd $export_cmd $chrom_cmd $indiv_cmd $nb_alleles_cmd --maf $frequency_min --max-maf $frequency_max --max-missing $missing_data >>vcftools.log 2>&1");