picard: picard_SamToFastq.xml comparison

comparison picard_SamToFastq.xml @ 8:e417b1d6288d draft

planemo upload for repository https://github.com/galaxyproject/tools-devteam/tree/master/tools/picard commit bf94a1505c131fb3f67c867b6e1d886780efa42e

author	devteam
date	Tue, 06 Dec 2016 10:04:26 -0500
parents	08f69add4d06
children	41b8d087a2d2

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-:08f69add4d06
+:e417b1d6288d
 <macros>
 <import>picard_macros.xml</import>
 </macros>
 <expand macro="requirements" />
 <command detect_errors="exit_code"><![CDATA[
 echo "BAM" > $report &&    ## This is necessary for output dataset detection (see output tags below)
 @java_options@
+@symlink_element_identifier@
 picard
 SamToFastq
-INPUT="${inputFile}"
+INPUT='$inputFile.element_identifier'
 #if str( $output_per_rg ) == "true":
 OUTPUT_PER_RG=true
 OUTPUT_DIR=.
 #elif str( $output_per_rg ) == "false" and str( $interleave ) == "false":
 FASTQ=READ1.fastq
 SECOND_END_FASTQ=READ2.fastq
 UNPAIRED_FASTQ=UNPAIRED_READS.fastq
 #elif str( $output_per_rg ) == "false" and str( $interleave ) == "true":
 FASTQ=INTERLEAVED.fastq
 #end if
 RE_REVERSE="${re_reverse}"
 INTERLEAVE="${interleave}"
 INCLUDE_NON_PF_READS="${include_non_pf_reads}"
 CLIPPING_ATTRIBUTE="${clipping_attribute}"
 CLIPPING_ACTION="${clipping_action}"
 READ1_TRIM="${read1_trim}"
 #if int($read1_max_bases_to_write) > -1:
 READ1_MAX_BASES_TO_WRITE="${read1_max_bases_to_write}"
 #end if
 READ2_TRIM="${read2_trim}"
 #if int($read2_max_bases_to_write) > -1:
 READ2_MAX_BASES_TO_WRITE="${read2_max_bases_to_write}"
 #end if
 INCLUDE_NON_PRIMARY_ALIGNMENTS="${include_non_primary_alignments}"
 VALIDATION_STRINGENCY="${validation_stringency}"
 QUIET=true
 VERBOSITY=ERROR
 ]]></command>
 <inputs>
 <param format="sam,bam" name="inputFile" type="data" label="Select SAM/BAM dataset or dataset collection" help="If empty, upload or import a SAM/BAM dataset"/>
 <param name="output_per_rg" type="boolean" checked="False" label="Do you want to output a fastq file per read group (two fastq files per read group if the group is paired)" help="OUTPUT_PER_RG; default=False"/>
 <param name="re_reverse" type="boolean" checked="True" label="Re-reverse bases and qualities of reads with negative strand flag set before writing them to fastq" help="RE_REVERSE; default=True"/>
 <param name="interleave" type="boolean" label="Will generate an interleaved fastq if paired, each line will have /1 or /2 to describe which end it came from" help="INTERLEAVE; default=False"/>
 <param name="include_non_pf_reads" type="boolean" label="Include non-PF reads from the SAM/BAM dataset into the output FASTQ" help="INCLUDE_NON_PF_READS; PF means 'passes filtering'. Reads whose 'not passing quality controls' flag is set are non-PF reads; default=False"/>
 <param name="read1_trim" type="integer" value="0" min="0" label="The number of bases to trim from the beginning of read 1" help="READ1_TRIM; default=0"/>
 <param name="read1_max_bases_to_write" type="integer" value="-1" label="The maximum number of bases to write from read 1 after trimming" help="READ1_MAX_BASES_TO_WRITE; If there are fewer than this many bases left after trimming, all will be written. If this value is null then all bases left after trimming will be written; default=null (-1)"/>
 <param name="read2_trim" type="integer" value="0" min="0" label="The number of bases to trim from the beginning of read 2" help="READ2_TRIM; default=0"/>
 <param name="read2_max_bases_to_write" type="integer" value="-1" label="The maximum number of bases to write from read 2 after trimming" help="READ2_MAX_BASES_TO_WRITE; If there are fewer than this many bases left after trimming, all will be written. If this value is null then all bases left after trimming will be written; default=null (-1)"/>
 <param name="include_non_primary_alignments" type="boolean" label="If true, include non-primary alignments in the output" help="INCLUDE_NON_PRIMARY_ALIGNMENTS; Support of non-primary alignments in SamToFastq is not comprehensive, so there may be exceptions if this is set to true and there are paired reads with non-primary alignments; default=False"/>
 <expand macro="VS" />
 </inputs>
 <outputs>
 <!-- here dataset discovery is based on fact that if OUTPUT_PER_RG=true this tool automatically adds .fastq extension to emitted files -->
 <data format="txt" name="report" label="SamToFastq run" hidden="true">
 <discover_datasets pattern="(?P&lt;designation&gt;.+)\.fastq" ext="fastqsanger" visible="true"/>
 </data>
 </outputs>
 <tests>
 <test>
 <param name="inputFile" value="picard_SamToFastq.bam" ftype="bam"/>
 <param name="output_per_rg" value="false"/>
 <param name="re_reverse" value="true"/>
 <param name="clipping_action" value="null" />
 <param name="read1_trim" value="0" />
 <param name="read1_max_bases_to_write" value="-1"/>
 <param name="read2_trim" value="0" />
 <param name="read2_max_bases_to_write" value="-1"/>
 <param name="include_non_primary_alignments" value="false"/>
 <output name="report">
 <assert_contents>
 <has_line line="BAM" />
 </assert_contents>
 <discovered_dataset designation="INTERLEAVED" file="picard_SamToFastq_test1.fq" ftype="fastqsanger"/>
 </output>
 </test>
 </tests>
 <help>
 **Purpose**
 Extracts read sequences and qualities from the input SAM/BAM dataset and outputs them in Sanger fastq format. In the RE_REVERSE=True mode (default behavior), if the read is aligned and the alignment is to the reverse strand on the genome, the read's sequence from input SAM.BAM dataset will be reverse-complemented prior to writing it to fastq in order restore correctly the original read sequence as it was generated by the sequencer.
 @dataset_collections@
 @description@
 FASTQ=File
 F=File                        Output fastq file (single-end fastq or, if paired, first end of the pair fastq).
 Required.  Cannot be used in conjuction with option(s) OUTPUT_PER_RG (OPRG)
 SECOND_END_FASTQ=File
 F2=File                       Output fastq file (if paired, second end of the pair fastq).  Default value: null.
 Cannot be used in conjuction with option(s) OUTPUT_PER_RG (OPRG)
 UNPAIRED_FASTQ=File
 FU=File                       Output fastq file for unpaired reads; may only be provided in paired-fastq mode  Default
 value: null.  Cannot be used in conjuction with option(s) OUTPUT_PER_RG (OPRG)
 OUTPUT_PER_RG=Boolean
 OPRG=Boolean                  Output a fastq file per read group (two fastq files per read group if the group is
 paired).  Default value: false. Possible values: {true, false}  Cannot be used in
 conjuction with option(s) SECOND_END_FASTQ (F2) UNPAIRED_FASTQ (FU) FASTQ (F)
 OUTPUT_DIR=File
 ODIR=File                     Directory in which to output the fastq file(s).  Used only when OUTPUT_PER_RG is true.
 Default value: null.
 RE_REVERSE=Boolean
 RC=Boolean                    Re-reverse bases and qualities of reads with negative strand flag set before writing them
 to fastq  Default value: true. Possible values: {true, false}
 INTERLEAVE=Boolean
 INTER=Boolean                 Will generate an interleaved fastq if paired, each line will have /1 or /2 to describe
 which end it came from  Default value: false. Possible values: {true, false}
 INCLUDE_NON_PF_READS=Boolean
 NON_PF=Boolean                Include non-PF reads from the SAM file into the output FASTQ files. PF means 'passes
 filtering'. Reads whose 'not passing quality controls' flag is set are non-PF reads.
 Default value: false. Possible values: {true, false}
 CLIPPING_ATTRIBUTE=String
 CLIP_ATTR=String              The attribute that stores the position at which the SAM record should be clipped  Default
 value: null.
 CLIPPING_ACTION=String
 CLIP_ACT=String               The action that should be taken with clipped reads: 'X' means the reads and qualities
 should be trimmed at the clipped position; 'N' means the bases should be changed to Ns in
 the clipped region; and any integer means that the base qualities should be set to that
 value in the clipped region.  Default value: null.
 READ1_TRIM=Integer
 R1_TRIM=Integer               The number of bases to trim from the beginning of read 1.  Default value: 0.
 READ1_MAX_BASES_TO_WRITE=Integer
 R1_MAX_BASES=Integer          The maximum number of bases to write from read 1 after trimming. If there are fewer than
 this many bases left after trimming, all will be written.  If this value is null then all
 bases left after trimming will be written.  Default value: null.
 READ2_TRIM=Integer
 R2_TRIM=Integer               The number of bases to trim from the beginning of read 2.  Default value: 0.
 READ2_MAX_BASES_TO_WRITE=Integer
 R2_MAX_BASES=Integer          The maximum number of bases to write from read 2 after trimming. If there are fewer than
 this many bases left after trimming, all will be written.  If this value is null then all
 bases left after trimming will be written.  Default value: null.
 INCLUDE_NON_PRIMARY_ALIGNMENTS=Boolean
 If true, include non-primary alignments in the output.  Support of non-primary alignments
 in SamToFastq is not comprehensive, so there may be exceptions if this is set to true and
 there are paired reads with non-primary alignments.  Default value: false.
 Possible values: {true, false}
 @more_info@
 </help>
 </tool>

Mercurial > repos > devteam > picard

comparison picard_SamToFastq.xml @ 8:e417b1d6288d draft