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view picard_FastqToSam.xml @ 0:1cd7f3b42609
Uploaded tool.
author | devteam |
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date | Tue, 23 Oct 2012 13:14:29 -0400 |
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children | bf1c3f9f8282 |
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<tool id="picard_FastqToSam" name="FASTQ to BAM" version="1.56.0"> <description>creates an unaligned BAM file</description> <requirements><requirement type="package" version="1.56.0">picard</requirement></requirements> <!-- Dan Blankenberg --> <command>java -XX:DefaultMaxRAMFraction=1 -XX:+UseParallelGC -jar "\$JAVA_JAR_PATH/FastqToSam.jar" FASTQ="${input_fastq1}" #if str( $input_fastq2) != "None": FASTQ2="${input_fastq2}" #end if QUALITY_FORMAT="${ dict( fastqsanger='Standard', fastqcssanger='Standard', fastqillumina='Illumina', fastqsolexa='Solexa' )[ $input_fastq1.ext ] }" ##Solexa, Illumina, Standard OUTPUT="${output_bam}" READ_GROUP_NAME="${read_group_name}" SAMPLE_NAME="${sample_name}" #if $param_type.param_type_selector == "advanced": #if str( $param_type.library_name ) != "": LIBRARY_NAME="${param_type.library_name}" #end if #if str( $param_type.platform_unit ) != "": PLATFORM_UNIT="${param_type.platform_unit}" #end if #if str( $param_type.platform ) != "": PLATFORM="${param_type.platform}" #end if #if str( $param_type.sequencing_center ) != "": SEQUENCING_CENTER="${param_type.sequencing_center}" #end if #if str( $param_type.predicted_insert_size ) != "": PREDICTED_INSERT_SIZE="${param_type.predicted_insert_size}" #end if #if str( $param_type.description.value ) != "": DESCRIPTION="${param_type.description}" #end if #if str( $param_type.run_date ) != "": RUN_DATE="${param_type.run_date}" #end if #if str( $param_type.min_q ) != "": MIN_Q="${param_type.min_q}" #end if #if str( $param_type.min_q ) != "": MAX_Q="${param_type.max_q}" #end if SORT_ORDER="${param_type.sort_order}" #else: SORT_ORDER=coordinate ##unsorted, queryname, coordinate; always use coordinate #end if 2>&1 || echo "Error running Picard FastqToSAM" >&2 </command> <inputs> <param name="input_fastq1" type="data" format="fastqsanger,fastqillumina,fastqsolexa,fastqcssanger" label="FASTQ file" /> <!-- confirm that fastqcssanger also works --> <param name="input_fastq2" type="data" format="fastqsanger,fastqillumina,fastqsolexa,fastqcssanger" optional="True" label="Second FASTQ of paired end data" help="Only needed when using paired end data." > <options options_filter_attribute="ext" from_parameter="tool.app.datatypes_registry.datatypes_by_extension" transform_lines="obj.keys()"> <column name="name" index="0"/> <column name="value" index="0"/> <filter type="param_value" ref="input_fastq1" ref_attribute="ext" column="0"/> </options> </param> <param name="read_group_name" type="text" value="A" label="Read Group Name" /> <param name="sample_name" type="text" value="unknown sample" label="Sample Name" /> <conditional name="param_type"> <param name="param_type_selector" type="select" label="Basic or Advanced options"> <option value="basic" selected="True">Basic</option> <option value="advanced">Advanced</option> </param> <when value="basic"> <!-- Do nothing here --> </when> <when value="advanced"> <param name="library_name" type="text" value="" label="Library Name" /> <param name="platform_unit" type="text" value="" label="Platform Unit" /> <param name="platform" type="text" value="" label="Platform" /> <param name="sequencing_center" type="text" value="" label="Sequencing Center" /> <param name="predicted_insert_size" type="integer" value="" optional="True" label="Predicted Insert Size" /> <param name="description" type="text" value="" label="Description" /> <param name="run_date" type="text" value="" label="Run Date" /> <param name="min_q" type="integer" optional="True" value="0" label="Min Q" /> <param name="max_q" type="integer" optional="True" value="93" label="Max Q" /> <param name="sort_order" type="select" label="Sort order"> <option value="coordinate" selected="True">coordinate</option> <option value="queryname">queryname</option> <option value="unsorted">unsorted</option> </param> </when> </conditional> </inputs> <outputs> <data format="bam" name="output_bam" /> </outputs> <tests> <test> <param name="input_fastq1" value="bwa_wrapper_in2.fastqsanger" ftype="fastqsanger" /> <param name="input_fastq2" /> <param name="read_group_name" value="A" /> <param name="sample_name" value="unknown sample" /> <param name="param_type_selector" value="basic" /> <output name="output_bam" file="picard_fastq_to_sam_out1.bam" ftype="bam"/> </test> <test> <param name="input_fastq1" value="bwa_wrapper_in2.fastqsanger" ftype="fastqsanger" /> <param name="input_fastq2" value="bwa_wrapper_in3.fastqsanger" ftype="fastqsanger" /> <param name="read_group_name" value="A" /> <param name="sample_name" value="unknown sample" /> <param name="param_type_selector" value="basic" /> <output name="output_bam" file="picard_fastq_to_sam_out2.bam" ftype="bam"/> </test> </tests> <help> **What it does** Picard: FastqToSam converts FASTQ files to unaligned BAM files. ------ Please cite the website "http://picard.sourceforge.net". ------ **Input formats** FastqToSam accepts FASTQ input files. If using paired-end data, you should select two FASTQ files. ------ **Outputs** The output is in BAM format, see http://samtools.sourceforge.net for more details. ------- **FastqToSam settings** This is list of FastqToSam options:: READ_GROUP_NAME=String Read group name Default value: A. This option can be set to 'null' to clear the default value. SAMPLE_NAME=String Sample name to insert into the read group header Required. LIBRARY_NAME=String The library name to place into the LB attribute in the read group header Default value: null. PLATFORM_UNIT=String The platform unit (often run_barcode.lane) to insert into the read group header Default value: null. PLATFORM=String The platform type (e.g. illumina, solid) to insert into the read group header Default value: null. SEQUENCING_CENTER=String The sequencing center from which the data originated Default value: null. PREDICTED_INSERT_SIZE=Integer Predicted median insert size, to insert into the read group header Default value: null. DESCRIPTION=String Inserted into the read group header Default value: null. </help> </tool>