Mercurial > repos > nick > duplex
view duplex.xml @ 1:b63d6673f883 draft
Bump version number and install from a stable, tagged Github release.
author | nick |
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date | Mon, 23 Nov 2015 22:53:35 -0500 |
parents | d2e46adc199e |
children | ba2a53b970ca |
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<?xml version="1.0"?> <tool id="duplex" name="Make consensus reads" version="0.2"> <description>from duplex sequencing data</description> <requirements> <requirement type="package" version="0.2">duplex</requirement> <requirement type="set_environment">DUPLEX_DIR</requirement> </requirements> <command detect_errors="exit_code"><![CDATA[ python \$DUPLEX_DIR/duplex.py -r $min_reads -q $qual_thres -F $qual_format $input #if $keep_sscs: --sscs-file $sscs #end if > duplex.fa && awk -f \$DUPLEX_DIR/utils/outconv.awk -v target=1 duplex.fa > $output1 && awk -f \$DUPLEX_DIR/utils/outconv.awk -v target=2 duplex.fa > $output2 ]]> </command> <inputs> <param name="input" type="data" format="tabular" label="Aligned input reads" /> <param name="min_reads" type="integer" value="3" min="1" label="Minimum reads per family" help="Single-strand families with fewer than this many reads will be skipped."/> <param name="qual_thres" type="integer" value="25" min="1" label="Minimum base quality" help="Bases with a PHRED score less than this will not be counted in the consensus making."/> <param name="qual_format" type="select" label="FASTQ format" help="Solexa should also work for Illumina 1.3+ and 1.5+, and Sanger should work for Illumina 1.8+"> <option value="sanger" selected="true">Sanger (PHRED 0 = "!")</option> <option value="solexa">Solexa (PHRED 0 = "@")</option> </param> <param name="keep_sscs" type="boolean" truevalue="true" falsevalue="" label="Output single-strand consensus sequences" /> </inputs> <outputs> <data name="output1" format="fasta" label="$tool.name on $on_string (mate 1)"/> <data name="output2" format="fasta" label="$tool.name on $on_string (mate 2)"/> <data name="sscs" format="fasta" label="$tool.name on $on_string (SSCS)"> <filter>keep_sscs</filter> </data> </outputs> <tests> <test> <param name="input" value="families.msa.tsv"/> <output name="output1" file="families.cons_1.fa"/> <output name="output2" file="families.cons_2.fa"/> </test> </tests> <help> **What it does** This is for processing duplex sequencing data. It creates single-strand and duplex consensus reads from aligned read families. ----- **Input** This expects the output format of the "Align families" tool. ----- **Output** This will output final, duplex consensus reads in two FASTA files (first and second reads in the pairs). Optionally, you can save the single-strand reads too, in a separate FASTA file. </help> </tool>