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view picard_CollectRnaSeqMetrics.xml @ 140:08b3cb5ce651 draft
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author | devteam |
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date | Thu, 27 Feb 2014 01:03:15 -0500 |
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<tool name="CollectRnaSeqMetrics" id="picard_CollectRnaSeqMetrics" version="1.106.0"> <description>Collect RNA-Seq Metrics</description> <requirements><requirement type="package" version="1.106.0">picard</requirement></requirements> <command interpreter="python"> picard_wrapper.py -i "${input_file}" -d "${html_file.files_path}" -t "${html_file}" -n "${out_prefix}" --tmpdir "${__new_file_path__}" --assumesorted ${ASSUME_SORTED} --refflat ${REF_FLAT} #if $identify_ribosomal.opt == "yes" --ribosomalintervals ${identify_ribosomal.RIBOSOMAL_INTERVALS} #end if --malevel "${malevel}" --minlength ${MINIMUM_LENGTH} --strandspecificity ${STRAND_SPECIFICITY} --rrnafragmentpercentage ${RRNA_FRAGMENT_PERCENTAGE} #for $i in $IGNORE_SEQUENCES --ignoreseq "${i.IGNORE_SEQUENCE}" #end for -j "\$JAVA_JAR_PATH/CollectRnaSeqMetrics.jar" </command> <stdio> <exit_code range="0" level="warning" description="Tool finished correctly" /> </stdio> <inputs> <param format="sam" name="input_file" type="data" label="Input SAM file." help="" /> <param name="out_prefix" value="RNA-Seq Metrics" type="text" label="Title for the output file" help="Use this remind you what the job was for." size="80" /> <param format="data" name="REF_FLAT" type="data" label="Gene annotations in refFlat form. Format described here: http://genome.ucsc.edu/goldenPath/gbdDescriptionsOld.html#RefFlat Required." help="" /> <conditional name="identify_ribosomal"> <param name="opt" type="select" label="Identify ribosomal bases" help="If 'no' is selected, no bases will be identified as being ribosomal."> <option value="no">no</option> <option value="yes">yes</option> </param> <when value="no" /> <when value="yes"> <param format="data" name="RIBOSOMAL_INTERVALS" type="data" label="Location of rRNA sequences in genome, in interval_list format. If not specified no bases will be identified as being ribosomal. Format described here: http://picard.sourceforge.net/javadoc/net/sf/picard/util/IntervalList.html Default value: null." help="" /> </when> </conditional> <param name="STRAND_SPECIFICITY" type="select" label="For strand-specific library prep." help="For unpaired reads, use FIRST_READ_TRANSCRIPTION_STRAND if the reads are expected to be on the transcription strand."> <option value="NONE" selected="True">None</option> <option value="FIRST_READ_TRANSCRIPTION_STRAND">FIRST_READ_TRANSCRIPTION_STRAND</option> <option value="SECOND_READ_TRANSCRIPTION_STRAND">SECOND_READ_TRANSCRIPTION_STRAND</option> </param> <param name="MINIMUM_LENGTH" type="text" value="500" label="When calculating coverage based values (e.g. CV of coverage) only use transcripts of this length or greater." help="" /> <repeat name="IGNORE_SEQUENCES" title="Ignore Sequences"> <param name="IGNORE_SEQUENCE" label="Ignore Sequence" type="text" help="If a read maps to a sequence specified with this option, all the bases in the read are counted as ignored bases." /> </repeat> <param name="RRNA_FRAGMENT_PERCENTAGE" type="text" value="0.8" label="This percentage of the length of a fragment must overlap one of the ribosomal intervals for a read or read pair by this must in order to be considered rRNA." help="" /> <param name="malevel" value="0" type="select" multiple="true" label="Metric Accumulation Level" help="Level(s) at which metrics will be accumulated"> <option value="ALL_READS" selected="true">All reads (default)</option> <option value="SAMPLE" default="true">Sample</option> <option value="LIBRARY" default="true">Library</option> <option value="READ_GROUP" default="true">Read group</option> </param> <param checked="True" truevalue="true" falsevalue="false" name="ASSUME_SORTED" type="boolean" label="If true (default), then the sort order in the header file will be ignored." /> </inputs> <outputs> <data format="html" name="html_file" label="${out_prefix}.html"/> </outputs> <tests> <test> <!-- python picard_wrapper.py -i "/home/~/PICARD-in.sam" -d "/home/~/outputrnaseqùetrics_files" -t "/home/~/outputrnaseqmetrics.htm" -n "RNA-Seq Metrics" --tmpdir "/home/dorine/galaxypicard/galaxy-central/database/tmp" --assumesorted true --refflat /home/~/refFlat.txt --malevel "ALL_READS" --minlength 500 --strandspecificity NONE --rrnafragmentpercentage 0.8 -j "/home/~/CollectRnaSeqMetrics.jar" --> <param name="inputFile" value="PICARD-in.sam" /> <param name="out_prefix" value="RNA-Seq Metrics" /> <param name="ASSUME_SORTED" value="true" /> <param name="REF_FLAT" value="refFlat.txt" /> <param name="malevel" value="ALL_READS" /> <param name="MINIMUM_LENGTH" value="500" /> <param name="STRAND_SPECIFICITY" value="NONE" /> <param name="RRNA_FRAGMENT_PERCENTAGE" value="O.8" /> <output name="html_file" file="outputrnaseqmetrics.html" ftype="html" lines_diff="30"/> </test> </tests> <help> Picard documentation says: CollectRnaSeqMetrics Documentation: http://picard.sourceforge.net/command-line-overview.shtml#CollectRnaSeqMetrics Program to collect metrics about the alignment of RNA to various functional classes of loci in the genome: coding, intronic, UTR, intergenic, ribosomal. Also determines strand-specificity for strand-specific libraries. </help> </tool>