Mercurial > repos > eiriche > bsmap
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author | eiriche |
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date | Fri, 30 Nov 2012 09:15:14 -0500 |
parents | 413c742682f7 |
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<tool id="bsmap" name="BSMAP Mapper"> <requirements> <requirement type='package'> bsmap </requirement> </requirements> <command interpreter="bash"> bsmap_wrapper.sh ##Reference genome ##ref="${reference.fields.path}" #if $refGenomeSource.genomeSource == "history": ref="${refGenomeSource.myFile}" #else ref="${refGenomeSource.builtinFile.fields.path}" #end if ##Output files (SAM output, BSMAP summary) mapped=$mapped ##Temp directory tempdir=$mapped.files_path summary=$summary #if str($singlePaired.sPaired) == "single": library="single" mate1=$singlePaired.sInput1 #if str($singlePaired.sParams.sSettingsType) == "full": fullparam=true qual=$singlePaired.sParams.qual threshold=$singlePaired.sParams.threshold lowqual=$singlePaired.sParams.lowqual adapter=$singlePaired.sParams.adapter firstn=$singlePaired.sParams.firstn repeat_reads=$singlePaired.sParams.repeat_reads seed_size=$singlePaired.sParams.seed_size mismatch=$singlePaired.sParams.mismatch equal_best=$singlePaired.sParams.equal_best start=$singlePaired.sParams.start end=$singlePaired.sParams.end index_interval=$singlePaired.sParams.index_interval seed_random=$singlePaired.sParams.seed_random rrbs=$singlePaired.sParams.rrbs mode=$singlePaired.sParams.mode align_info=$singlePaired.sParams.align_info #end if #else: library="paired" mate1=$singlePaired.pInput1 mate2=$singlePaired.pInput2 unpaired=$unpaired #if str($singlePaired.pParams.pSettingsType) == "full": fullparam=true qual=$singlePaired.pParams.qual threshold=$singlePaired.pParams.threshold lowqual=$singlePaired.pParams.lowqual adapter=$singlePaired.pParams.adapter firstn=$singlePaired.pParams.firstn repeat_reads=$singlePaired.pParams.repeat_reads seed_size=$singlePaired.pParams.seed_size mismatch=$singlePaired.pParams.mismatch equal_best=$singlePaired.pParams.equal_best start=$singlePaired.pParams.start end=$singlePaired.pParams.end index_interval=$singlePaired.pParams.index_interval seed_random=$singlePaired.pParams.seed_random rrbs=$singlePaired.pParams.rrbs mode=$singlePaired.pParams.mode align_info=$singlePaired.pParams.align_info maxinsert=$singlePaired.pParams.maxinsert mininsert=$singlePaired.pParams.mininsert #end if #end if </command> <inputs> <conditional name="refGenomeSource"> <param name="genomeSource" type="select" label="Will you select a reference genome from your history or use a built-in reference?"> <option value="builtin">Use a built-in reference</option> <option value="history">Use one from the history</option> </param> <when value="builtin"> <param name="builtinFile" type="select" label="Select the reference genome"> <options from_data_table="bsmap_fasta"> <filter type="sort_by" column="2" /> <validator type="no_options" message="No reference genomes are available" /> </options> </param> </when> <when value="history"> <param name="myFile" type="data" format="fasta" label="Select the reference genome" /> </when> </conditional> <conditional name="singlePaired"> <param name="sPaired" type="select" label="Is this library mate-paired?"> <option value="single">Single-end</option> <option value="paired">Paired-end</option> </param> <when value="single"> <param name="sInput1" type="data" format="fastq,fasta" label="FASTQ file" help="Must have ASCII encoded quality scores"/> <conditional name="sParams"> <param name="sSettingsType" type="select" label="BSMAP settings to use" help="For most mapping needs use Commonly used settings. If you want full control use Full parameter list"> <option value="preSet">Commonly used</option> <option value="full">Full parameter list</option> </param> <when value="preSet" /> <when value="full"> <param name="qual" type="select" label="Select the type of FastQ qualities"> <option value="33">phred33-quals</option> <option value="64">phred64-quals</option> </param> <param name="threshold" type="integer" value="0" label="Quality threshold in trimming" help="0-40, default=0 (no trim)" min="0" max="40" /> <param name="lowqual" type="integer" value="5" label="Filter low-quality reads containing >n Ns" help="default=5" /> <param name="adapter" type="text" value="none" label="3-end adapter sequence" help="default: none (no trim)" /> <param name="firstn" type="integer" value="144" label="Map the first N nucleotides of the read" help="default:144 (map the whole read)" /> <param name="repeat_reads" type="select" label="How to report repeat hits"> <option value="0">none(unique hit only)</option> <option value="1">random one</option> </param> <param name="seed_size" type="integer" value="16" label="Seed size" min="8" max="16" help="default=16(WGBS mode), 12(RRBS mode)" /> <param name="mismatch" type="integer" value="2" label="Maximum number of mismatches allowed on a read" max="15" /> <param name="equal_best" type="integer" value="20" label="Maximum number of equal best hits to count" max="1000" /> <param name="start" type="integer" value="1" label="Start from the Nth read or read pair" /> <param name="end" type="integer" value="4294967295" label="End at the Nth read or read pair" /> <param name="index_interval" type="integer" value="4" label="Index interval" /> <param name="seed_random" type="integer" value="-1" label="Seed for random number generation used in selecting multiple hits" help="other seed values generate pseudo random number based on read index number, to allow reproducible mapping results" /> <param name="rrbs" type="text" value="none" label="Activating RRBS mapping mode and set restriction enzyme digestion sites" help="digestion position marked by '-', example: -D C-CGG for MspI digestion. default: none (whole genome shotgun bisulfite mapping mode)" /> <param name="mode" type="select" label="Set mapping strand information"> <option value="0">only map to 2 forward strands</option> <option value="1">map SE or PE reads to all 4 strands</option> </param> <param name="align_info" type="text" value="none" label="Set alignment information for the additional nucleotide transition" help="is in the form of two different nucleotides N1N2,indicating N1 in the reads could be mapped to N2 in the reference sequences. default: -M TC, corresponds to C=>U(T) transition in bisulfite conversion. example: -M GA could be used to detect A=>I(G) transition in RNA editing." /> </when> <!-- full --> </conditional> <!-- sParams --> </when> <!-- single --> <when value="paired"> <param name="pInput1" type="data" format="fastq,fasta" label="Forward FASTQ file" /> <param name="pInput2" type="data" format="fastq,fasta" label="Reverse FASTQ file" /> <conditional name="pParams"> <param name="pSettingsType" type="select" label="BSMAP settings to use" help="For most mapping needs use Commonly used settings. If you want full control use Full parameter list"> <option value="preSet">Commonly used</option> <option value="full">Full parameter list</option> </param> <when value="preSet" /> <when value="full"> <param name="qual" type="select" label="Select the type of FastQ qualities"> <option value="33">phred33-quals</option> <option value="64">phred64-quals</option> </param> <param name="mininsert" type="integer" value="28" label="Minimal insert size allowed" /> <param name="maxinsert" type="integer" value="500" label="Maximal insert size allowed" /> <param name="threshold" type="integer" value="0" label="Quality threshold in trimming" help="0-40, default=0 (no trim)" min="0" max="40" /> <param name="lowqual" type="integer" value="5" label="Filter low-quality reads containing >n Ns" help="default=5" /> <param name="adapter" type="text" value="none" label="3-end adapter sequence" help="default: none (no trim)" /> <param name="firstn" type="integer" value="144" label="Map the first N nucleotides of the read" help="default:144 (map the whole read)" /> <param name="repeat_reads" type="select" label="How to report repeat hits"> <option value="0">none(unique hit only)</option> <option value="1">random one</option> </param> <param name="seed_size" type="integer" value="16" label="Seed size" min="8" max="16" help="default=16(WGBS mode), 12(RRBS mode)" /> <param name="mismatch" type="integer" value="2" label="Maximum number of mismatches allowed on a read" max="15" /> <param name="equal_best" type="integer" value="20" label="Maximum number of equal best hits to count" max="1000" /> <param name="start" type="integer" value="1" label="Start from the Nth read or read pair" /> <param name="end" type="integer" value="4294967295" label="End at the Nth read or read pair" /> <param name="index_interval" type="integer" value="4" label="Index interval" /> <param name="seed_random" type="integer" value="-1" label="Seed for random number generation used in selecting multiple hits" help="other seed values generate pseudo random number based on read index number, to allow reproducible mapping results" /> <param name="rrbs" type="text" value="none" label="Activating RRBS mapping mode and set restriction enzyme digestion sites" help="digestion position marked by '-', example: -D C-CGG for MspI digestion. default: none (whole genome shotgun bisulfite mapping mode)" /> <param name="mode" type="select" label="Set mapping strand information"> <option value="0">only map to 2 forward strands</option> <option value="1">map SE or PE reads to all 4 strands</option> </param> <param name="align_info" type="text" value="none" label="Set alignment information for the additional nucleotide transition" help="is in the form of two different nucleotides N1N2,indicating N1 in the reads could be mapped to N2 in the reference sequences. default: -M TC, corresponds to C=>U(T) transition in bisulfite conversion. example: -M GA could be used to detect A=>I(G) transition in RNA editing." /> </when> <!-- full --> </conditional> <!-- pParams --> </when> <!-- paired --> </conditional> <!-- singlePaired --> </inputs> <outputs> <data name="mapped" format="sam" label="BSMAP Mapped Reads" /> <data name="summary" format="txt" label="BSMAP Mapping Summary" /> <data name="unpaired" format ="sam" label="BSMAP Unpaired Hits"> <filter>(singlePaired['sPaired'] == 'paired')</filter> </data> </outputs> <help> **What it does** BSMAP is a short reads mapping software for bisulfite sequencing reads. It has the following features: - read length up to 144 nt, allow up to 15 mismatches, gap size up to 3 bp. - support single end and pair end mapping. support multi-thread mapping. - support both "Lister protocol" (sequence 2 forward strands only) and "Cokus protocol" (sequence all 4 bisulfite converted strands) - reads are directly mapped to original reference genome sequence, no need to preprocess the reads and reference genome to convert C to T. - support both whole genome bisulfite sequencing (WGBS) mode and reduced representation bisulfite sequencing (RRBS) mode, allow changing the digestion site information to support different digestion enzymes for RRBS. - allow trimming adapter sequences and low quality nucleotides from the 3'end of reads - allow trade off between speed/memory usage/mapping sensitivity. For human genome, the RRBS mode uses ~3GB. In WGBS mode, the typical memory usage is ~9GB, but can be as low as 5GB. - allow alignment for other nucleotide transitions, for example, can be set to detect the A=>I(G) transition in RNA editing. .. _BSMAP: http://code.google.com/p/bsmap/ **Input formats** BSMAP accepts files in FASTA/FASTQ format. **Outputs** The output contains the following files: - mapped reads in SAM format - mapping summary - unpaired hits (only for paired-end mapping) </help> <tests> </tests> </tool>