Mercurial > repos > fcaramia > edger
diff htseq.pl @ 4:ebd59bc6855c draft
Uploaded
author | fcaramia |
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date | Wed, 12 Sep 2012 23:45:33 -0400 |
parents | |
children | 6324eefd9e91 |
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--- /dev/null Thu Jan 01 00:00:00 1970 +0000 +++ b/htseq.pl Wed Sep 12 23:45:33 2012 -0400 @@ -0,0 +1,107 @@ +#!/usr/bin/perl + +use strict; +use warnings; +use Getopt::Std; +use File::Basename; +$| = 1; + +# Grab and set all options +my %OPTIONS = (a => 0, i => "gene_id", m => "intersection-nonempty", s => "no", t => "exon"); +getopts('a:cg:i:m:o:r:s:t:', \%OPTIONS); + +die qq( +Usage: HTSeq.pl [OPTIONS] Group1=sample1=<SAM/BAM file> [Group1=sample2=<SAM/BAM file> ... Group2=sampleN=<SAM/BAM file> ...] + +OPTIONS: -a STR skip all reads with alignment quality lower than the given minimum value (default: $OPTIONS{a}) + -c reduce the matrix by removing any feature with no counts + -g STR the features file in the GFF/GTF format + -i STR GFF attribute to be used as feature ID (default: $OPTIONS{i}) + -m STR mode to handle reads overlapping more than one feature. Possible values for <mode> are union, intersection-strict and intersection-nonempty (default: $OPTIONS{m}) + -o STR output file name for expression matrix + -r STR the name of the output report + -s STR whether the data is from a strand-specific assay (default: $OPTIONS{s}) + -t STR feature type (3rd column in GFF file) to be used, all features of other type are ignored (default, suitable for RNA-Seq and Ensembl GTF files: $OPTIONS{t}) + +) if(@ARGV == 0); + +my $sam_out; +my @counts; +my @features; +my %report; +my @samplenames; +my $current_group; +my @groups; +my @files; +my $groupcount = 0; +my %grouphash; + +foreach my $input (@ARGV) { + my ($group, $sample, $input) = split "::", $input; + if(! defined $grouphash{$group}) { + $groupcount++; + $grouphash{$group} = "G${groupcount}:$group"; + } + push @groups, $grouphash{$group}; + push @samplenames, $sample; + push @files, $input; +} + +for(my $index = 0; $index <= $#files; $index++) { + my $input_file = $files[$index]; + my $sample = $samplenames[$index]; + + # run htseq + my @htseq; + my $COMM; + my $file_type = `file $input_file`; + if(grep /text$/, $file_type ) { + $COMM = "htseq-count -q -m $OPTIONS{m} -s $OPTIONS{s} -a $OPTIONS{a} -t $OPTIONS{t} -i $OPTIONS{i} $input_file $OPTIONS{g}"; + @htseq = `$COMM`; + } else { + $COMM = "samtools view $input_file | htseq-count -q -m $OPTIONS{m} -s $OPTIONS{s} -a $OPTIONS{a} -t $OPTIONS{t} -i $OPTIONS{i} - $OPTIONS{g}"; + @htseq = `$COMM`; + } + + my $row = 0; + $report{$sample} = "Command Used: $COMM\n"; + + for(my $row = 0; $row <= $#htseq; $row++) { + # store the report is an hash + if(grep /^no_feature|^ambiguous|^too_low_aQual|^not_aligned|^alignment_not_unique/, $htseq[$row]) { + $report{$sample} .= $htseq[$row]; + } else { + # store the counts in a matrix + chomp $htseq[$row]; + my ($feature, $value) = split "\t", $htseq[$row]; + $counts[$row][$index] = $value; + if($input_file eq $files[0]) { + push @features, $feature; + } + } + } +} + +# print the matrix +open(MATRIX, ">$OPTIONS{o}") || die "Could Not Create Output File $OPTIONS{o}!\n"; +print MATRIX "#\t".join("\t", @groups)."\n"; +print MATRIX "#Feature\t".join("\t", @samplenames)."\n"; +for(my $row = 0; $row <= $#features; $row++) { + if(defined $OPTIONS{c}) { + my $rowsum = 0; + $rowsum += $_ foreach @{ $counts[$row] }; + if(!$rowsum) { + next; + } + } + print MATRIX "$features[$row]\t".join("\t", @{ $counts[$row] })."\n"; +} +close(MATRIX); + +# print the report +open(REPORT, ">$OPTIONS{r}") || die "Could Not Create Output File $OPTIONS{r}!\n"; +print REPORT "$groups[$_]:$samplenames[$_]\n$report{$samplenames[$_]}\n" foreach (0..$#samplenames); +close(REPORT); + + +