Mercurial > repos > iuc > plasmidfinder
changeset 1:eccc7495c3d9 draft
planemo upload for repository https://github.com/mesocentre-clermont-auvergne/galaxy-tools/tree/master/tools/plasmidfinder commit 69aab27f0210af0f0986d63575f9bfdb3f9d1f6a
author | iuc |
---|---|
date | Fri, 14 Oct 2022 11:54:49 +0000 |
parents | 2b6e795b22a9 |
children | e23b96d79dc0 |
files | macro.xml plasmidfinder.xml |
diffstat | 2 files changed, 13 insertions(+), 17 deletions(-) [+] |
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--- a/macro.xml Mon Sep 19 08:47:42 2022 +0000 +++ b/macro.xml Fri Oct 14 11:54:49 2022 +0000 @@ -1,7 +1,7 @@ <macros> <token name="@TOOL_VERSION@">2.1.6</token> - <token name="@VERSION_SUFFIX@">0</token> + <token name="@VERSION_SUFFIX@">1</token> <token name="@PROFILE@">21.05</token> <token name="@THREADS@">\${GALAXY_SLOTS:-7}</token>
--- a/plasmidfinder.xml Mon Sep 19 08:47:42 2022 +0000 +++ b/plasmidfinder.xml Fri Oct 14 11:54:49 2022 +0000 @@ -17,7 +17,7 @@ -t '$options.threshold' #if $input.input_file.ext == 'fasta' or $input.input_file.ext == 'fasta.gz' -mp blastn - #else if $input.input_file.ext == 'fastqsanger.gz' or $input.input_file.ext == 'fastqsanger' + #elif $input.input_file.ext == 'fastqsanger' or $input.input_file.ext == 'fastqsanger.gz' -mp kma #end if -x @@ -31,7 +31,7 @@ </command> <inputs> <section name="input" title="Input parameters" expanded="true"> - <param name="input_file" type="data" format="fasta,fastq,fasta.gz,fastq.gz" label="Choose a fasta or fastq file" help="File to be analyzed"/> + <param name="input_file" type="data" format="fasta,fasta.gz,fastqsanger,fastqsanger.gz" label="Choose a fasta or fastq file" help="File to be analyzed"/> <param name="database_name" type="select" label="PlasmidFinder database"> <options from_data_table="plasmidfinder_db"> <validator message="No PlasmidFinder database is available" type="no_options"/> @@ -39,16 +39,16 @@ </param> </section> <section name="options" title="Options"> - <param name="min_cov" type="float" min="0" max="1" value="0.6" label="Minimal coverage" help="Choose a minimum coverage value (default: 0.6)"/> - <param name="threshold" type="float" min="0" max="1" value="0.95" label="Minimal identity" help="Choose a minimum identity value (default: 0.95)"/> + <param name="min_cov" type="float" min="0" max="1" value="0.6" label="Minimal coverage" help=" Fraction of matching sequence on the total target sequence(default: 0.6)"/> + <param name="threshold" type="float" min="0" max="1" value="0.95" label="Minimal identity" help=" Fraction of shared nucleotide on the match (default: 0.95)"/> </section> <section name="output_files" title="Output file selection"> <param name="output_selection" type="select" display="checkboxes" multiple="true" label="Output files selection"> <option value="data_json">JSON file result</option> - <option value="hit_fasta" selected="true">Hits in genome</option> - <option value="plasmid_fasta" selected="true">Plasmid hits</option> - <option value="result_tsv" selected="true">Plasmid results</option> - <option value="result_txt" selected="true">Raw results</option> + <option value="hit_fasta" selected="true">Matching sequences in the genome for plasmid</option> + <option value="plasmid_fasta" selected="true">Plasmid sequences discovered in the genome</option> + <option value="result_tsv" selected="true">Plasmid match list</option> + <option value="result_txt" selected="true">Plasmid match list in raw format</option> <option value="logfile">Log file</option> </param> </section> @@ -128,20 +128,16 @@ <help><![CDATA[ **What it does** PlasmidFinder characterize plasmid sequences into whole genome sequencing. - It is based on [plasmidfinder database](https://bitbucket.org/genomicepidemiology/plasmidfinder_db/) with hundreds sequences. + It is based on the [plasmidfinder database](https://bitbucket.org/genomicepidemiology/plasmidfinder_db/) with hundreds sequences. **Input** - It can analyse raw data using a k-mer approach based on KMA or a blastn for genome assembly. - A database is need obtained from the plasmidfinder database. - **Options** - You can modify the coverage value (% of matching sequence on the total target sequence) - You can modify the identity threshold (% of shared nucleotide on the match) + PlasmidFinder takes raw data (with a k-mer analysisi) as reads or genome assembly (blastn analysis) to search plasmids. **Output** Some output files are availables - - A fasta file with all available hits detected in the genome + - A fasta file with all available sequences detected in the genome - A fasta file with all plasmid sequences from the database - A summary of the analysis in tabular format - A Raw result file in text format - - A JSON file could be use for other boinformatic analaysis + - A JSON file could be use for other boinformatic analysis - A log file with analysis parameters ]]></help>