Mercurial > repos > jeremie > delly_
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author | jeremie |
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date | Tue, 17 Jun 2014 08:46:45 -0400 |
parents | 6fda22b6c486 |
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<tool id="delly" name="delly" version=""> <description>structural variant prediction method</description> <parallelism method="basic"></parallelism> <command interpreter="python"> delly.py -b $bam -t #if $checkDel: DEL #end if #if $checkDup: DUP #end if #if $checkInv: INV #end if #if $checkTra: TRA #end if -q $map_qual -s $mad_cutoff -g $genome -m $min_flank -e $epsilon -o $output </command> <inputs> <param format="bam" name="bam" type="data" label="bam file" help="" /> <param name="checkDel" type="boolean" label="Check Deletion?" checked="true"/> <param name="checkDup" type="boolean" label="Check Duplication?" checked="true"/> <param name="checkInv" type="boolean" label="Check Inversion?" checked="true"/> <param name="checkTra" type="boolean" label="Check Translation?" checked="true"/> <param name="map_qual" type="integer" label="min. paired-end mapping quality" value="0" /> <param name="mad_cutoff" type="integer" label="insert size cutoff, median+s*MAD (deletions only)" value="5" /> <param name="min_flank" type="integer" label="minimum flanking sequence size" value="13" /> <param name="epsilon" type="float" label="allowed epsilon deviation of PE vs. SR deletion" value="0.1" /> <param name="genome" type="text" label="genome" value="null" /> </inputs> <outputs> <data format="vcf" name="output" label="VCF output of delly" /> </outputs> <help> DELLY is an integrated structural variant prediction method that can detect deletions, tandem duplications, inversions and translocations at single-nucleotide resolution in short-read massively parallel sequencing data. It uses paired-ends and split-reads to sensitively and accurately delineate genomic rearrangements throughout the genome. DELLY (Version: 0.5.5) Contact: Tobias Rausch (rausch@embl.de) Generic options: -? [ --help ] show help message -t [ --type ] arg (=DEL) SV analysis type (DEL, DUP, INV, TRA) -o [ --outfile ] arg (="sv.vcf") SV output file -x [ --exclude ] arg (="") file with chr to exclude PE options: -q [ --map-qual ] arg (=0) min. paired-end mapping quality -s [ --mad-cutoff ] arg (=5) insert size cutoff, median+s*MAD (deletions only) SR options: -g [ --genome ] arg genome fasta file -m [ --min-flank ] arg (=13) minimum flanking sequence size Genotyping options: -v [ --vcfgeno ] arg (="site.vcf") input vcf file for genotyping only -u [ --geno-qual ] arg (=20) min. mapping quality for genotyping </help> <tests> <test> </test> </tests> </tool>