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planemo upload for repository https://github.com/bgruening/galaxytools/tree/master/tools/trim_galore commit 07148c518916e16602ea26473d00358fe04bc3b6-dirty
author | bgruening |
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date | Mon, 25 Jan 2016 04:44:33 -0500 |
parents | 11962ce40855 |
children | f1e71aeaa923 |
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<tool id="trim_galore" name="Trim Galore!" version="0.4.1"> <!-- Wrapper compatible with Trim Galore! version 0.4 --> <description>adaptive quality and adapter trimmer</description> <macros> <macro name="adapter_trimming"> <conditional name="trimming"> <param name="trimming_select" type="select" label="Trimming reads?"> <option value="">Automatic detection</option> <option value="--illumina">Illumina universal</option> <option value="--nextera">Nextera transposase</option> <option value="--small_rna">Illumina small RNA adapters</option> <option value="user">User defined adapter trimming</option> </param> <when value=""/> <when value="--illumina"/> <when value="--nextera"/> <when value="--small_rna"/> <when value="user"> <param name="adapter" type="text" value="AGATCGGAAGAGC" label="Adapter sequence to be trimmed off"> <validator type="regex" message="Adapter sequence must contain DNA characters only (A,C,T,G or N)">^[ACTGNactgn]*$</validator> </param> <yield/> </when> </conditional> </macro> <macro name="paired_adapter_trimming"> <expand macro="adapter_trimming"> <param name="adapter2" type="text" optional="True" value="" label="Adapter sequence to be trimmed off read 2"> <validator type="regex" message="Adapter sequence must contain DNA characters only (A,C,T,G or N)">^[ACTGNactgn]*$</validator> </param> </expand> <param name="trim1" type="boolean" truevalue="--trim1" falsevalue="" checked="False" label="Trims 1 bp off every read from its 3' end." help="" /> <param name="three_prime_clip_R1" type="integer" value="" optional="True" label="Remove N bp from the 3' end of read 1"> <help>Instructs Trim Galore! to remove N bp from the 3' end of read 1 after adapter/quality trimming has been performed. This may remove some unwanted bias from the 3' end that is not directly related to adapter sequence or basecall quality. (--three_prime_clip_R1)</help> </param> <param name="three_prime_clip_R2" type="integer" value="" optional="True" label="Remove N bp from the 3' end of read 1"> <help>Instructs Trim Galore! to remove N bp from the 3' end of read 2 after adapter/quality trimming has been performed. This may remove some unwanted bias from the 3' end that is not directly related to adapter sequence or basecall quality. (--three_prime_clip_R2)</help> </param> </macro> </macros> <requirements> <requirement type="package" version="1.8">cutadapt</requirement> </requirements> <version_command interpreter="perl">trim_galore --version</version_command> <command> <![CDATA[ ## trim_galore removes .fastq and .fq file extensions of input files. ## This is essential if Galaxy provides links to files (with real extensions) ## but that behaviour is causing an inconsistency in output filenaming. ## We work around this by linking every file to cwd without file extension #if $singlePaired.sPaired == "single": ln -s "${singlePaired.input_singles}" ./input_singles; #elif $singlePaired.sPaired == "paired": ln -s "${singlePaired.input_mate1}" ./input_mate1; ln -s "${singlePaired.input_mate2}" ./input_mate2; #else: ln -s "${singlePaired.input_mate_pairs.forward}" ./input_mate1; ln -s "${singlePaired.input_mate_pairs.reverse}" ./input_mate2; #end if perl $__tool_directory__/trim_galore ## we only support fastqsanger --phred33 #if $params.settingsType == "custom": ## default 20 --quality $params.quality ## default 1 --stringency $params.stringency ## default 0.1 -e $params.error_rate ## default 20 --length $params.min_length #if $params.clip_R1: --clip_R1 $params.clip_R1 #end if #if $params.clip_R2: --clip_R2 $params.clip_R2 #end if #if $params.retain_unpaired.retain_unpaired_select == "retain_unpaired_output": --retain_unpaired --length_1 $params.retain_unpaired.length_1 --length_2 $params.retain_unpaired.length_2 #end if #end if ## RBBS specific options. #if $rrbs.settingsType == "custom": $rrbs.rrbs $rrbs.non_directional #end if --output_dir ./ --suppress_warn #if $params.settingsType == "custom" and not $params.report: --no_report_file #end if #if $singlePaired.trimming.trimming_select == 'user': ## default 'AGATCGGAAGAGC' #if $singlePaired.trimming.adapter.strip() != '': --adapter $singlePaired.trimming.adapter #end if #else: $singlePaired.trimming.trimming_select #end if #if $singlePaired.three_prime_clip_R1: --three_prime_clip_R1 $singlePaired.three_prime_clip_R1 #end if #if $singlePaired.sPaired == "single": ## input sequence ./input_singles #else: --paired $singlePaired.trim1 #if $singlePaired.trimming.trimming_select == 'user': #if $singlePaired.trimming.adapter2 and $singlePaired.trimming.adapter2.strip() != '': --adapter2 $singlePaired.trimming.adapter2 #end if #end if #if $singlePaired.three_prime_clip_R2: --three_prime_clip_R2 $singlePaired.three_prime_clip_R2 #end if ## input sequences ./input_mate1 ./input_mate2 #end if ## Trim Galore! run is finished. Move the report files to the proper place #if $params.settingsType == "custom" and $params.report: && cat ./*_trimming_report.txt > $report_file; #end if ]]> </command> <inputs> <!-- Input Parameters --> <conditional name="singlePaired"> <param name="sPaired" type="select" label="Is this library paired- or single-end?"> <option value="single">Single-end</option> <option value="paired">Paired-end</option> <option value="paired_collection">Paired Collection</option> </param> <when value="single"> <param name="input_singles" type="data" format="fastqsanger" label="Reads in FASTQ format" /> <expand macro="adapter_trimming"/> <param name="three_prime_clip_R1" type="integer" value="" optional="True" label="Remove N bp from the 3' end"> <help>Instructs Trim Galore! to remove N bp from the 3' end of read 1 after adapter/quality trimming has been performed. This may remove some unwanted bias from the 3' end that is not directly related to adapter sequence or basecall quality. (--three_prime_clip_R1)</help> </param> </when> <when value="paired"> <param name="input_mate1" type="data" format="fastqsanger" label="Reads in FASTQ format" /> <param name="input_mate2" type="data" format="fastqsanger" label="Reads in FASTQ format" /> <expand macro="paired_adapter_trimming" /> </when> <when value="paired_collection"> <param name="input_mate_pairs" format="fastqsanger" type="data_collection" collection_type="paired" label="Select a paired collection" help="See help section for an explanation of dataset collections"/> <expand macro="paired_adapter_trimming" /> </when> </conditional> <conditional name="params"> <param name="settingsType" type="select" label="Trim Galore! advanced settings" help="You can use the default settings or set custom values for any of Trim Galore!'s parameters."> <option value="default">Use defaults</option> <option value="custom">Full parameter list</option> </param> <when value="default" /> <!-- Full/advanced params. --> <when value="custom"> <param name="quality" type="integer" value="20" label="Trim low-quality ends from reads in addition to adapter removal" help="For more information please see below." /> <param name="stringency" type="integer" value="1" label="Overlap with adapter sequence required to trim a sequence" /> <param name="error_rate" type="float" value="0.1" label="Maximum allowed error rate" /> <param name="min_length" type="integer" value="20" label="Discard reads that became shorter than length INT" /> <param name="clip_R1" type="integer" optional="True" min="0" label="Instructs Trim Galore! to remove INT bp from the 5' end of read 1" /> <param name="clip_R2" type="integer" optional="True" min="0" label="Instructs Trim Galore! to remove INT bp from the 5' end of read 2" /> <param name="report" type="boolean" truevalue="true" falsevalue="false" checked="False" label="Generate a report file" help="" /> <conditional name="retain_unpaired"> <param name="retain_unpaired_select" type="select" label="specify if you would like to retain unpaired reads"> <option value="no_output">Do not output unpaired reads</option> <option value="retain_unpaired_output">Output unpaired reads</option> </param> <when value="no_output" /> <!-- Output params. --> <when value="retain_unpaired_output"> <param name="length_1" type="integer" value="35" label="Unpaired single-end read length cutoff needed for read 1 to be written" /> <param name="length_2" type="integer" value="35" label="Unpaired single-end read length cutoff needed for read 2 to be written" /> </when> <!-- output --> </conditional> <!-- retain_unpaired --> </when> <!-- full --> </conditional> <!-- params --> <conditional name="rrbs"> <param name="settingsType" type="select" label="RRBS specific settings"> <option value="default">Use defaults (no RRBS)</option> <option value="custom">Full parameter list</option> </param> <when value="default" /> <!-- Full/advanced params. --> <when value="custom"> <param name="rrbs" type="boolean" truevalue="--rrbs" falsevalue="" checked="True" label="Specifies that the input file was an MspI digested RRBS sample" /> <param name="non_directional" type="boolean" truevalue="--non_directional" falsevalue="" checked="False" label="Selecting this option for non-directional RRBS libraries" /> </when> <!-- full --> </conditional> <!-- params --> </inputs> <outputs> <data format="fastqsanger" name="trimmed_reads_single" from_work_dir="input_singles_trimmed.fq" label="${tool.name} on ${on_string}: trimmed reads"> <filter>singlePaired['sPaired'] == "single"</filter> </data> <collection name="trimmed_reads_paired_collection" type="paired" label="${tool.name} on ${on_string}: paired reads"> <data name="forward" format="fastqsanger" from_work_dir="input_mate1_val_1.fq" /> <data name="reverse" format="fastqsanger" from_work_dir="input_mate2_val_2.fq" /> <filter>singlePaired['sPaired'] == "paired_collection"</filter> </collection> <collection name="trimmed_reads_unpaired_collection" type="paired" label="${tool.name} on ${on_string}: unpaired reads"> <data name="forward" format="fastqsanger" from_work_dir="input_mate1_unpaired_1.fq" /> <data name="reverse" format="fastqsanger" from_work_dir="input_mate2_unpaired_2.fq" /> <filter>params['settingsType'] == "custom"</filter> <filter>params['retain_unpaired']['retain_unpaired_select'] == "retain_unpaired_output"</filter> <filter>singlePaired['sPaired'] == "paired_collection"</filter> </collection> <data format="fastqsanger" name="trimmed_reads_pair1" from_work_dir="input_mate1_val_1.fq" label="${tool.name} on ${on_string}: trimmed reads pair 1"> <filter>singlePaired['sPaired'] == "paired"</filter> </data> <data format="fastqsanger" name="trimmed_reads_pair2" from_work_dir="input_mate2_val_2.fq" label="${tool.name} on ${on_string}: trimmed reads pair 2"> <filter>singlePaired['sPaired'] == "paired"</filter> </data> <data format="fastqsanger" name="unpaired_reads_1" from_work_dir="input_mate1_unpaired_1.fq" label="${tool.name} on ${on_string}: unpaired reads (1)"> <filter>params['settingsType'] == "custom"</filter> <filter>params['retain_unpaired']['retain_unpaired_select'] == "retain_unpaired_output"</filter> <filter>singlePaired['sPaired'] == "paired"</filter> </data> <data format="fastqsanger" name="unpaired_reads_2" from_work_dir="input_mate2_unpaired_2.fq" label="${tool.name} on ${on_string}: unpaired reads (2)"> <filter>params['settingsType'] == "custom"</filter> <filter>params['retain_unpaired']['retain_unpaired_select'] == "retain_unpaired_output"</filter> <filter>singlePaired['sPaired'] == "paired"</filter> </data> <data format="txt" name="report_file" label="${tool.name} on ${on_string}: report file"> <filter>params['settingsType'] == "custom"</filter> <filter>params['report'] == True</filter> </data> </outputs> <tests> <test> <param name="input_singles" value="sanger_full_range_original_sanger.fastqsanger" ftype="fastqsanger" /> <param name="sPaired" value="single" /> <param name="settingsType" value="custom" /> <param name="report" value="true" /> <output name="trimmed_reads_single" file="sanger_full_range_results1.fastqsanger" ftype="fastqsanger"/> <output name="report_file" file="sanger_full_range_report_results1.txt" ftype="txt" lines_diff="2" /> </test> <test> <param name="input_singles" value="sanger_full_range_original_sanger.fastqsanger" ftype="fastqsanger" /> <param name="sPaired" value="single" /> <param name="trimming_select" value="--illumina" /> <output name="trimmed_reads_single" file="sanger_full_range_results2.fastqsanger" ftype="fastqsanger"/> </test> <test> <param name="input_singles" value="sanger_full_range_original_sanger.fastqsanger" ftype="fastqsanger" /> <param name="sPaired" value="single" /> <param name="adapter" value="AAAGAGC" /> <output name="trimmed_reads_single" file="sanger_full_range_results3.fastqsanger" ftype="fastqsanger"/> </test> <test> <param name="input_mate1" value="bwa-mem-fastq1.fq" ftype="fastqsanger" /> <param name="input_mate2" value="bwa-mem-fastq2.fq" ftype="fastqsanger" /> <param name="sPaired" value="paired" /> <param name="settingsType" value="custom" /> <param name="report" value="true" /> <output name="trimmed_reads_pair1" file="paired_example_pair1_results2.fastqsanger" ftype="fastqsanger"/> <output name="trimmed_reads_pair2" file="paired_example_pair2_results2.fastqsanger" ftype="fastqsanger"/> <output name="report_file" file="paired_example_results2.txt" ftype="txt" lines_diff="8" /> </test> <test> <param name="input_mate_pairs"> <collection type="paired"> <element name="forward" value="bwa-mem-fastq1.fq" ftype="fastqsanger" /> <element name="reverse" value="bwa-mem-fastq2.fq" ftype="fastqsanger" /> </collection> </param> <param name="sPaired" value="paired_collection" /> <param name="settingsType" value="custom" /> <param name="report" value="true" /> <param name="retain_unpaired_select" value="retain_unpaired_output" /> <output name="report_file" file="paired_collection_example_results3.txt" ftype="txt" lines_diff="8" /> <output_collection name="trimmed_reads_paired_collection" type="paired"> <element name="forward" file="paired_collection_example_pair1_results3.fastqsanger" ftype="fastqsanger"/> <element name="reverse" file="paired_collection_example_pair2_results3.fastqsanger" ftype="fastqsanger"/> </output_collection> <output_collection name="trimmed_reads_unpaired_collection" type="paired"> <element name="forward" file="paired_collection_example_unpair1_results3.fastqsanger" ftype="fastqsanger"/> <element name="reverse" file="paired_collection_example_unpair2_results3.fastqsanger" ftype="fastqsanger"/> </output_collection> </test> </tests> <help> <![CDATA[ **What it does** `Trim Galore!`_ is a wrapper script to automate quality and adapter trimming as well as quality control, with some added functionality to remove biased methylation positions for RRBS sequence files (for directional, non-directional (or paired-end) sequencing). It's main features are: * For adapter trimming, Trim Galore! uses the first 13 bp of Illumina standard adapters ('AGATCGGAAGAGC') by default (suitable for both ends of paired-end libraries), but accepts other adapter sequence, too * For MspI-digested RRBS libraries, Trim Galore! performs quality and adapter trimming in two subsequent steps. This allows it to remove 2 additional bases that contain a cytosine which was artificially introduced in the end-repair step during the library preparation * For any kind of FASTQ file other than MspI-digested RRBS, Trim Galore! can perform single-pass adapter and quality trimming * The Phred quality of basecalls and the stringency for adapter removal can be specified individually * Trim Galore! can remove sequences if they become too short during the trimming process. For paired-end files Trim Galore! removes entire sequence pairs if one (or both) of the two reads became shorter than the set length cutoff. Reads of a read-pair that are longer than a given threshold but for which the partner read has become too short can optionally be written out to single-end files. This ensures that the information of a read pair is not lost entirely if only one read is of good quality * Trim Galore! can trim paired-end files by 1 additional bp from the 3' end of all reads to avoid problems with invalid alignments with Bowtie 1 .. _Trim Galore!: http://www.bioinformatics.babraham.ac.uk/projects/trim_galore/ It is developed by Felix Krueger at the Babraham Institute. ]]> </help> <citations></citations> </tool>