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view trinity.xml @ 10:831abd20e690 draft
planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/trinity commit e23a8ad798830209db722d5496d19ec7a5e06214
| author | iuc |
|---|---|
| date | Mon, 01 Aug 2016 14:42:55 -0400 |
| parents | e4a9e0798360 |
| children | 03884591c766 |
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<tool id="trinity" name="Trinity" version="@WRAPPER_VERSION@.0"> <description>de novo assembly of RNA-Seq data</description> <macros> <import>macros.xml</import> </macros> <expand macro="requirements"> <requirement type="package" version="1.1.2">bowtie</requirement> <requirement type="package" version="1.2">samtools</requirement> <requirement type="set_environment">TRINITY_MEM_OPTIONS</requirement> </expand> <expand macro="stdio"/> <command><![CDATA[ Trinity ## Inputs. #if $inputs.paired_or_single == "paired": --left ${ ','.join(['"%s"' % x for x in $inputs.left_input]) } --right ${ ','.join(['"%s"' % x for x in $inputs.right_input]) } #if $inputs.left_input[0].is_of_type('fasta'): --seqType fa #else: --seqType fq #end if #if $inputs.strand.is_strand_specific: --SS_lib_type $inputs.strand.library_type #end if $inputs.jaccard_clip #else: --single ${ ','.join(['"%s"' % x for x in $inputs.input]) } #if $inputs.input[0].is_of_type('fasta'): --seqType fa #else: --seqType fq #end if #if $inputs.strand.is_strand_specific: --SS_lib_type $inputs.strand.library_type #end if #end if $norm ## Additional parameters. #if $additional_params.min_contig_length: --min_contig_length $additional_params.min_contig_length #end if #if $additional_params.long_reads: --long_reads $additional_params.long_reads #end if #if $additional_params.guided.is_guided == "yes": --genome_guided_bam $additional_params.guided.genome_guided_bam #if $additional_params.guided.genome_guided_min_coverage: --genome_guided_min_coverage $additional_params.guided.genome_guided_min_coverage #end if #if $additional_params.guided.genome_guided_min_reads_per_partition: --genome_guided_min_reads_per_partition $additional_params.guided.genome_guided_min_reads_per_partition #end if #end if #if $additional_params.min_kmer_cov: --min_kmer_cov $additional_params.min_kmer_cov #end if ## CPU and butterfly options. --CPU \${GALAXY_SLOTS:-4} \${TRINITY_MEM_OPTIONS:---max_memory 1G} --bfly_opts "-V 10 --stderr" ## > $trinity_log 2>&1 ]]></command> <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,fastqsanger" argument="--left" name="left_input" multiple="true" type="data" label="Left/Forward strand reads" help=""/> <param format="fasta,fastqsanger" argument="--right" name="right_input" multiple="true" type="data" label="Right/Reverse strand reads" help=""/> <conditional name="strand"> <param name="is_strand_specific" type="boolean" checked="false" label="Strand specific data"/> <when value="false"> </when> <when value="true"> <param name="library_type" argument="--SS_lib_type" type="select" label="Strand-specific Library Type"> <option value="FR">Forward-Reverse</option> <option value="RF">Reverse-Forward</option> </param> </when> </conditional> <param name="jaccard_clip" argument="--jaccard_clip" type="boolean" truevalue="--jaccard_clip" falsevalue="" checked="false" label="Jaccard Clip options" help="set if you expect high gene density with UTR overlap"/> </when> <when value="single"> <param format="fasta,fastqsanger" name="input" argument="--single" multiple="true" type="data" label="Single-end reads" help=""/> <conditional name="strand"> <param name="is_strand_specific" type="boolean" checked="false" label="Strand specific data"/> <when value="false"> </when> <when value="true"> <param name="library_type" argument="--SS_lib_type" type="select" label="Strand-specific Library Type"> <option value="F">F</option> <option value="R">R</option> </param> </when> </conditional> </when> </conditional> <param name="norm" type="boolean" argument="--normalize_reads" truevalue="--normalize_reads" falsevalue="" checked="true" label="Run in silico normalization of reads" help="Defaults to max. read coverage of 50."/> <section name="additional_params" title="Additional Options" expanded="False"> <param name="min_contig_length" argument="--min_contig_length" type="integer" optional="true" value="200" min="1" label="Minimum Contig Length" help="All contigs shorter than this will be discarded"/> <conditional name="guided"> <param name="is_guided" type="select" label="Use the genome guided mode?" help="If you already mapped the reads to the genome, Trinity can use this information"> <option value="no">No</option> <option value="yes">Yes</option> </param> <when value="no"> </when> <when value="yes"> <param format="bam" name="genome_guided_bam" argument="--genome_guided_bam" type="data" label="Coordinate-sorted BAM file" /> <param name="genome_guided_min_coverage" argument="--genome_guided_min_coverage" type="integer" optional="true" value="1" min="1" label="Minimum read coverage for identifying an expressed region of the genome"/> <param name="genome_guided_min_reads_per_partition" argument="--genome_guided_min_reads_per_partition" type="integer" optional="true" value="10" min="1" label="Minimum number of reads per partition"/> </when> </conditional> <param format="fasta" name="long_reads" argument="--long_reads" type="data" optional="true" label="Error-corrected or circular consensus (CCS) pac bio reads" help="Experimental feature! Long reads must be in the same orientation as short reads if they are strand specific"/> <param name="min_kmer_cov" argument="--min_kmer_cov" type="integer" optional="true" value="1" min="1" label="Minimum count for K-mers to be assembled"/> </section> </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> <test> <param name="paired_or_single" value="paired"/> <param name="left_input" value="reads.left.fq" ftype="fastqsanger"/> <param name="right_input" value="reads.right.fq" ftype="fastqsanger"/> <param name="is_strand_specific" value="true"/> <param name="norm" value="false"/> <param name="library_type" value="RF"/> <output name="assembled_transcripts" file="raw/Trinity.fasta" compare="sim_size" delta="500" /> </test> <test> <param name="paired_or_single" value="paired"/> <param name="left_input" value="reads.left.fq" ftype="fastqsanger"/> <param name="right_input" value="reads.right.fq" ftype="fastqsanger"/> <param name="is_strand_specific" value="true"/> <param name="norm" value="true"/> <param name="library_type" value="RF"/> <output name="assembled_transcripts" file="norm/Trinity.fasta" compare="sim_size" delta="500" /> </test> </tests> <help> Trinity_ assembles transcript sequences from Illumina RNA-Seq data. .. _Trinity: http://trinityrnaseq.github.io </help> <expand macro="citation" /> </tool>