Mercurial > repos > joachim-jacob > qualimap_suite
view bamqc.xml @ 3:9537dd9dd18b draft
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author | joachim-jacob |
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date | Tue, 12 Feb 2013 04:50:47 -0500 |
parents | 934cd08c77af |
children | 3d690162d629 |
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<tool id="qualimap_bamqc" name="Analyse SAM/BAM with bamqc" version="0.0.1"> <!-- Additional info: wrapper compatible with versions ..... --> <description> to asses mapping quality metrics. </description> <version_command> qualimap --version </version_command> <requirements> <requirement type="package">qualimap</requirement> </requirements> <command interpreter="perl"> ## it is recommended that you write a wrapper for your tool ## and pass all parameters to that tool, which parses them. bamqc_wrapper.pl $configfile </command> <inputs> <param format="sam,bam" name="bam" type="data" label="Alignments in the BAM or SAM format" help="The set of aligned reads." /> <param type="boolean" name="c" checked="TRUE" truevalue="-c" falsevalue="" label="paint chromosome limits inside charts" /> <conditional name="customgtf"> <param name="upload" type="select" label="BETA! Analyze the alignment data for the regions of interest you provide"> <option value="yes">Yes</option> <option value="no" selected="true">No</option> </param> <when value="yes"> <param name="gff" type="data" format="bed,gtf,gff3" label="Choose your feature annotation file" help="Provide your BED, GTF or GFF file"/> <param name="os" type="boolean" checked="FALSE" truevalue="-os" falsevalue="" label="compute also regions outside stats" help="If checked, the information about the reads that are mapped outside of the regions of interest will be also computed and shown in a separate section" /> <param type="select" name="p" label="The sequencing protocol strand specificity" help="Can be non-strand-specific, forward-stranded orreverse-stranded. This information is required to calculate the number of correct strand reads."> <option value="NON-STRAND-SPECIFIC">Non-strand-specific</option> <option value="STRAND-SPECIFIC-FORWARD">Strand-specific forward</option> <option value="STRAND-SPECIFIC-REVERSE">Strand-specific reverse</option> </param> </when> <when value="no"/> </conditional> <param name="hm" type="text" size="3" value="3" label="minimum size for a homopolymer to be considered in indel analysis" help="Only homopolymers of this size or larger will be considered when estimating homopolymer indels count"/> <param name="nr" type="text" size="6" value="1000" label="number of reads in the chunk" help="In order to reduce the load of I/O, reads are analyzed in chunks. Each chunk contains the selected number of reads which will be loaded into memory and analyzed by a single thread. Smaller numbers may result in lower performance, but also the memory consumption will be reduced. The default value is 1000 reads"/> </inputs> <outputs> <data format="html" name="bamqc_result" label="${tool.name} on ${on_string}"> <!-- <data format="html" name="bamqc_result" label="${tool.name} on ${on_string}" from_work_dir="bamqc_output/qualimapReport.html"> --> </data> </outputs> <configfiles> <!-- this config file collects all parameter settings --> <configfile name="configfile"> ## first we pass some galaxy environment variables galtemp==${__new_file_path__} bamqc_result==$bamqc_result outputdir==$bamqc_result.files_path bam==$bam c==$c hm==$hm nr==$nr #if $customgtf.upload=="yes" gff==$customgtf.gff os==$customgtf.os p==$customgtf.p #end if </configfile> </configfiles> <tests> </tests> <help> **Tool Overview** Bamqc_ allows for simply but throroughly checking of the quality of mapping. .. _Bamqc: http://qualimap.bioinfo.cipf.es// ------ </help> </tool>