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author | nate |
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date | Thu, 04 May 2017 14:16:09 -0400 |
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<tool id="trinity_psc" name="Trinity" version="0.0.1"> <!-- Written by Jeremy Goecks, now maintained here by bhaas and additional modifications by Nate Coraor --> <description>(Beta) De novo assembly of RNA-Seq data Using Trinity on PSC's Bridges</description> <requirements> <!-- These are versions available as modules on Bridges --> <requirement type="package" version="1.1.2">bowtie</requirement> <requirement type="package" version="1.3">samtools</requirement> <requirement type="package" version="jre7">java</requirement> <requirement type="package" version="5.18.4-threads">perl</requirement> <requirement type="package" version="2.2.0">trinity</requirement> </requirements> <command> MEM=`expr "\${GALAXY_SLOTS:-16}" \* 48 - 16` ; workdir=`pwd`; echo "workdir is \$workdir"; cd \$LOCAL; echo "Running Trinity from `pwd`"; Trinity --no_version_check --max_memory "\${MEM}G" --CPU "\${GALAXY_SLOTS:-16}" --bflyHeapSpaceMax "32G" --bflyHeapSpaceInit "2G" --bflyGCThreads "6" #if $additional_params.use_additional == "yes" and $additional_params.normalize_reads == "yes": --normalize_reads #end if ## Inputs. #if str($inputs.paired_or_single) == "paired": --left $inputs.left_input --right $inputs.right_input #if $inputs.left_input.ext == 'fa': --seqType fa #else: --seqType fq #end if #if str($inputs.library_type) != "undefined": --SS_lib_type $inputs.library_type #end if --group_pairs_distance $inputs.group_pairs_distance #else: --single $inputs.input #if str($inputs.input.ext) == 'fa': --seqType fa #else: --seqType fq #end if #if str($inputs.library_type) != "undefined": --SS_lib_type $inputs.library_type #end if #end if ## Additional parameters. #if str($additional_params.use_additional) == "yes": --min_kmer_cov $additional_params.min_kmer_cov --max_reads_per_graph $additional_params.max_reads_per_graph #if $additional_params.bfly_opts != 'None': --bfly_opts " $additional_params.bfly_opts " #end if #end if ## direct to output > $trinity_log 2>&1 ## if Trinity fails, output the end of the log to stderr for Galaxy, and touch the output file for Pulsar || (ec=\$? ; cp -p $trinity_log \$workdir; cd \$workdir; cat $trinity_log >&2 ; mkdir -p trinity_out_dir ; touch trinity_out_dir/Trinity.fasta ; exit \$ec); mkdir -p \$workdir/trinity_out_dir; cp -p trinity_out_dir/Trinity* \$workdir/trinity_out_dir; cd \$workdir; </command> <stdio> <exit_code range="1:" level="fatal" description="Program failed" /> <exit_code range=":-1" level="fatal" description="DRM killed job" /> </stdio> <inputs> <conditional name="inputs"> <param name="paired_or_single" type="select" label="Paired or Single-end data?"> <option value="paired">Paired</option> <option value="single">Single</option> </param> <when value="paired"> <param format="fasta,fastq" name="left_input" type="data" label="Left/Forward strand reads" help=""/> <param format="fasta,fastq" name="right_input" type="data" label="Right/Reverse strand reads" help=""/> <param name="library_type" type="select" label="Strand-specific Library Type"> <option value="undefined">Not set</option> <option value="FR">FR</option> <option value="RF">RF</option> </param> <param name="group_pairs_distance" type="integer" value="500" min="1" label="Group pairs distance" help="Maximum length expected between fragment pairs"/> <param name="path_reinforcement_distance" type="integer" value="75" min="1" label="Path reinforcement distance" help="Minimum read overlap required for path extension in the graph" /> </when> <when value="single"> <param format="fasta,fastq" name="input" type="data" label="Single-end reads" help=""/> <param name="library_type" type="select" label="Strand-specific Library Type"> <option value="undefined">Not set</option> <option value="F">F</option> <option value="R">R</option> </param> <param name="path_reinforcement_distance" type="integer" value="40" min="1" label="Path reinforcement distance" help="Minimum read overlap required for path extension in the graph" /> </when> </conditional> <conditional name="additional_params"> <param name="use_additional" type="select" label="Use Additional Params?"> <option value="no">No</option> <option value="yes">Yes</option> </param> <when value="no"> </when> <when value="yes"> <param name="min_kmer_cov" type="integer" value="1" min="1" label="inchworm_min_kmer_cov" help="Minimum kmer coverage required by Inchworm for initial contig construction" /> <param name="max_reads_per_graph" type="integer" value="20000000" min="10000" label="chrysalis_max_reads_per_graph" help="Maximum number of reads to be anchored within each transcript graph by Chrysalis" /> <param name="bfly_opts" type="text" value="None" label="bfly_opts" help="Options to pass on to Butterfly" /> <param name="min_contig_length" type="integer" value="200" min="1" label="Minimum Contig Length" help=""/> <param name="normalize_reads" type="boolean" truevalue="yes" falsevalue="no" help="(--normalize_reads) Normalize reads, can decrease runtime and memory requirements for datasets exceeding 300M pairs"/> </when> </conditional> </inputs> <outputs> <data format="txt" name="trinity_log" label="${tool.name} on ${on_string}: log" /> <data format="fasta" name="assembled_transcripts" label="${tool.name} on ${on_string}: Assembled Transcripts" from_work_dir="trinity_out_dir/Trinity.fasta"/> </outputs> <tests> </tests> <help> Trinity is a de novo transcript assembler that uses RNA-seq data as input. This tool runs all Trinity_ commands--Inchworm, Chrysalis, and Butterfly--in a single pass. This version of Trinity runs on Bridges_ at the `Pittsburgh Supercomputing Center`_ using a version of Trinity 2.2.0 optimized for the unique memory profile of that system. .. _Trinity: http://trinityrnaseq.github.io .. _Pittsburgh Supercomputing Center: http://www.psc.edu .. _Bridges: http://www.psc.edu/bridges </help> </tool>