Mercurial > repos > bgruening > nanopolish_methylation
view nanopolish_methylation.xml @ 4:a8d4be409446 draft
planemo upload for repository https://github.com/bgruening/galaxytools/tree/master/tools/nanopolish commit 25c22b467760e4784e199125292927bd2274a189-dirty
| author | bgruening |
|---|---|
| date | Sun, 23 Jun 2019 05:54:36 -0400 |
| parents | 02e3c674d917 |
| children | 12efe2f03697 |
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<tool id="nanopolish_methylation" name="Nanopolish methylation" version="0.11.1"> <description>- Classify nucleotides as methylated or not.</description> <macros> <import>macros.xml</import> </macros> <expand macro="requirements" /> <command detect_errors="exit_code"><![CDATA[ ln -s '$input_merged' reads.fasta && #if $input_reads_raw.extension == 'fast5': mkdir fast5_files && ln -s '$input_reads_raw' fast5_files/read1.fast5 && #else if $input_reads_raw.extension == 'fast5.tar': ln -s '$input_reads_raw' fast5_files.tar && mkdir fast5_files && tar -xf fast5_files.tar -C fast5_files && #else if $input_reads_raw.extension == 'fast5.tar.bz2': ln -s '$input_reads_raw' fast5_files.tar.bz2 && mkdir fast5_files && tar -xjf fast5_files.tar.bz2 -C fast5_files && #else: ln -s '$input_reads_raw' fast5_files.tar.gz && mkdir fast5_files && tar -xzf fast5_files.tar.gz -C fast5_files && #end if nanopolish index -d fast5_files/ #if $adv.input_seq_summary: -s '$adv.input_seq_summary' #end if reads.fasta && ln -s '$b' reads.bam && ln -s '${b.metadata.bam_index}' reads.bam.bai && #if $reference_source.reference_source_selector == 'history': ln -f -s '$reference_source.ref_file' genome.fa && #else: ln -f -s '$reference_source.ref_file.fields.path' genome.fa && #end if nanopolish call-methylation -r reads.fasta -b reads.bam -g genome.fa #if str($batchsize): -K $batchsize #end if --threads "\${GALAXY_SLOTS:-4}" #if $w and str($w).strip(): -w "${w}" #end if > methylation_calls.tsv ]]></command> <inputs> <!-- index inputs --> <param type="data" name="input_merged" format="fasta,fastq" label="Basecalled merged reads.fa"/> <param type="data" name="input_reads_raw" format="fast5.tar.gz,fast5.tar.bz2,fast5.tar" label="Flat archive file of raw fast5 files"/> <!-- variants consensus inputs --> <param type="data" argument="-b" format="bam" label="Reads aligned to the reference genome" /> <conditional name="reference_source"> <param name="reference_source_selector" type="select" label="Load reference genome from"> <option value="cached">Local cache</option> <option value="history">History</option> </param> <when value="cached"> <param name="ref_file" type="select" label="Using reference genome" help="REFERENCE_SEQUENCE"> <options from_data_table="all_fasta"> </options> <validator type="no_options" message="A built-in reference genome is not available for the build associated with the selected input file"/> </param> </when> <when value="history"> <param name="ref_file" type="data" format="fasta" label="Use the following dataset as the reference sequence" help="REFERENCE_SEQUENCE; You can upload a FASTA sequence to the history and use it as reference" /> </when> </conditional> <section name="adv" title="Optional data inputs"> <!-- optional inputs --> <param type="data" name="input_seq_summary" format="txt" optional="true" label="Sequencing summary file from albacore" help="(-s)"/> </section> <param argument="-w" type="text" optional="true" label="find variants in window of region chromsome:start-end" /> <param name="batchsize" type="integer" optional="true" value="" label="Batch size" help="(-K)"/> </inputs> <outputs> <!-- variants consensus outputs --> <data name="output_methylation_calls" format="tabular" from_work_dir="methylation_calls.tsv" label="called methylation sites" /> </outputs> <tests> <test> <param name="input_merged" ftype="fasta" value="reads.fasta" /> <param name="input_reads_raw" ftype="fast5.tar.gz" value="fast5_files.tar.gz" /> <param name="b" value="reads.sorted.bam" /> <param name="reference_source_selector" value="history" /> <param name="ref_file" value="draft.fa" /> <param name="w" value="tig00000001:200000-202000" /> <param name="batchsize" value="512" /> <output name="output_methylation_calls" file="methylation_calls.tsv" /> </test> <test> <param name="input_merged" ftype="fasta" value="reads.fasta" /> <param name="input_reads_raw" ftype="fast5.tar.gz" value="fast5_files.tar.gz" /> <param name="reference_source_selector" value="history" /> <param name="ref_file" value="draft.fa"/> <param name="b" value="reads.sorted.bam" /> <param name="w" value="tig00000001:200000-202000" /> <param name="batchsize" value="512" /> <output name="output_methylation_calls" file="methylation_calls.tsv" /> </test> </tests> <help><![CDATA[ Usage: nanopolish call-methylation [OPTIONS] --reads reads.fa --bam alignments.bam --genome genome.fa Classify nucleotides as methylated or not. Quickstart tutorial and manual available at: http://nanopolish.readthedocs.io/en/latest/quickstart_call_methylation.html ]]></help> <expand macro="citations" /> </tool>