Mercurial > repos > galaxyp > translate_bed_sequences
view translate_bed_sequences.xml @ 2:4221664a2bd0 draft default tip
"planemo upload for repository https://github.com/galaxyproteomics/tools-galaxyp/tree/master/tools/translate_bed_sequences commit 2a470e2c775a7427aa530e058510e4dc7b6d8e80"
| author | galaxyp |
|---|---|
| date | Tue, 07 Apr 2020 11:45:53 -0400 |
| parents | 6bbce76c78c1 |
| children |
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<tool id="translate_bed_sequences" name="Translate BED Sequences" version="0.2.0"> <description>3 frame translation of BED augmented with a sequence column</description> <requirements> <requirement type="package" version="1.76">biopython</requirement> </requirements> <stdio> <exit_code range="1:" level="fatal" description="Error" /> </stdio> <command> python '$__tool_directory__/translate_bed_sequences.py' --input '$input' #if $fa_db: --fa_db='$fa_db' #end if #if $fa_sep: --fa_sep='$fa_sep' #end if #if $id_prefix: --id_prefix='$id_prefix' #end if #if $reference: --reference $reference #else: --reference ${input.metadata.dbkey} #end if #if $refsource: --refsource $refsource #end if #if $seqtype: --seqtype $seqtype #end if #if $score_name: --score_name $score_name #end if #if $filter.filterseqs == 'yes': #if $filter.leading_bp: --leading_bp $filter.leading_bp #end if #if $filter.trailing_bp: --trailing_bp $filter.trailing_bp #end if #else: --unfiltered #end if #if $trim.trimseqs == 'no': --untrimmed #if str($trim.max_stop_codons) != '': --max_stop_codons $trim.max_stop_codons #end if #end if #if str($min_length) != '': --min_length $min_length #end if --bed $translated_bed --output '$output' </command> <inputs> <param name="input" type="data" format="bed" label="BED file with added sequence column" help="Output from 'Extract Genomic DNA' run on tophat junctions.bed "/> <param name="fa_db" type="text" value="" optional="true" label="fasta ID source, e.g. generic" help="Any Compomics application such as PeptideShaker, requires a source"> </param> <param name="fa_sep" type="text" value="" optional="true" label="fasta ID line separator character" help="Only used when a fasta ID source is given, defaults to the pipe character"> </param> <param name="id_prefix" type="text" value="" optional="true" label="ID prefix for generated IDs" help="Can be used to distinguish samples"> <validator type="regex" message="Allowed chars:a-z A-Z 0-9 _ - |">^[a-zA-Z0-9_-|]*$</validator> </param> <param name="refsource" type="text" value="Ensembl" optional="true" label="Genome reference source" help=""/> <param name="reference" type="text" value="" optional="true" label="Genome reference name" help="By default, the database metadata will be used."/> <param name="seqtype" type="text" value="" optional="true" label="The SEQTYPE:STATUS to include in the fasta ID lines" help="For example: pep:splice"/> <param name="score_name" type="text" value="" optional="true" label="Add the bed score field fasta ID line with this tag name" help="For example: with the tag name 'depth' and bed score 12: depth:12"/> <conditional name="filter"> <param name="filterseqs" type="select" label="Filter out translations with stop codons before the splice site"> <option value="yes" selected="true">Yes</option> <option value="no">No</option> </param> <when value="yes"> <param name="leading_bp" type="integer" value="" min="0" optional="true" label="Stop codon filtering start position base pairs" help="Do not reject translation is stop_codons are within base pairs of the BED start position for positive strand"/> <param name="trailing_bp" type="integer" value="" min="0" optional="true" label="Stop codon filtering end position base pairs" help="Do not reject translation is stop_codons are within base pairs of the BED end position for negative strand"/> </when> <when value="no"/> </conditional> <conditional name="trim"> <param name="trimseqs" type="select" label="Trim translations to stop codons"> <option value="yes" selected="true">Yes</option> <option value="no">No</option> </param> <when value="no"> <param name="max_stop_codons" type="integer" value="" min="0" optional="true" label="Maximum number of stop codons allowed in a translation to be reported"/> </when> </conditional> <param name="min_length" type="integer" value="" min="0" optional="true" label="Minimum length of a translation to be reported"/> </inputs> <outputs> <data name="translated_bed" metadata_source="input" format="bed" label="${tool.name} on ${on_string} bed" /> <data name="output" metadata_source="input" format="fasta" label="${tool.name} on ${on_string} fasta" /> </outputs> <tests> <test> <param name="input" value="Extract_Genomic_DNA.bed" ftype="bed" dbkey="hg19"/> <param name="reference" value="GRCh37"/> <param name="seqtype" value="pep:novel"/> <param name="score_name" value="depth"/> <output name="output" file="translated_bed_sequences.fa"/> </test> </tests> <help> **Translate BED Sequences** This tool takes a BED input file that has been processed by the Galaxy tool "Extract Genomic DNA" to add a 13th column with the transcript sequence. It generates a peptide fasta file with the 3-frame translations of the spliced sequence defined by each entry in the input BED file. </help> </tool>