table_recalibration: table_recalibration.xml comparison

comparison table_recalibration.xml @ 1:30e1dd77e99c draft default tip

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author	devteam
date	Mon, 14 Apr 2014 08:48:25 -0400
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+:30e1dd77e99c
+<tool id="gatk_table_recalibration" name="Table Recalibration" version="0.0.5">
+<description>on BAM files</description>
+<requirements>
+<requirement type="package" version="1.4">gatk</requirement>
+<requirement type="package" version="0.1.18">samtools</requirement>
+</requirements>
+<macros>
+<import>gatk_macros.xml</import>
+</macros>
+<command interpreter="python">gatk_wrapper.py
+--max_jvm_heap_fraction "1"
+--stdout "${output_log}"
+-d "-I" "${reference_source.input_bam}" "${reference_source.input_bam.ext}" "gatk_input"
+#if str( $reference_source.input_bam.metadata.bam_index ) != "None":
+-d "" "${reference_source.input_bam.metadata.bam_index}" "bam_index" "gatk_input" ##hardcode galaxy ext type as bam_index
+#end if
+-p 'java
+-jar "\$JAVA_JAR_PATH/GenomeAnalysisTK.jar"
+-T "TableRecalibration"
+-o "${output_bam}"
+-et "NO_ET" ##ET no phone home
+##--num_threads 4 ##hard coded, for now
+##-log "${output_log}" ##don't use this to log to file, instead directly capture stdout
+#if $reference_source.reference_source_selector != "history":
+-R "${reference_source.ref_file.fields.path}"
+#end if
+--recal_file "${input_recal}"
+--disable_bam_indexing
+'
+#include source=$standard_gatk_options#
+##start analysis specific options
+#if $analysis_param_type.analysis_param_type_selector == "advanced":
+-p '
+#if $analysis_param_type.default_read_group_type.default_read_group_type_selector == "set":
+--default_read_group "${analysis_param_type.default_read_group_type.default_read_group}"
+#end if
+#if str( $analysis_param_type.default_platform ) != "default":
+--default_platform "${analysis_param_type.default_platform}"
+#end if
+#if str( $analysis_param_type.force_read_group_type.force_read_group_type_selector ) == "set":
+--force_read_group "${analysis_param_type.force_read_group_type.force_read_group}"
+#end if
+#if str( $analysis_param_type.force_platform ) != "default":
+--force_platform "${analysis_param_type.force_platform}"
+#end if
+${analysis_param_type.exception_if_no_tile}
+#if str( $analysis_param_type.solid_options_type.solid_options_type_selector ) == "set":
+#if str( $analysis_param_type.solid_options_type.solid_recal_mode ) != "default":
+--solid_recal_mode "${analysis_param_type.solid_options_type.solid_recal_mode}"
+#end if
+#if str( $analysis_param_type.solid_options_type.solid_nocall_strategy ) != "default":
+--solid_nocall_strategy "${analysis_param_type.solid_options_type.solid_nocall_strategy}"
+#end if
+#end if
+${analysis_param_type.simplify_bam}
+--preserve_qscores_less_than "${analysis_param_type.preserve_qscores_less_than}"
+--smoothing "${analysis_param_type.smoothing}"
+--max_quality_score "${analysis_param_type.max_quality_score}"
+--window_size_nqs "${analysis_param_type.window_size_nqs}"
+--homopolymer_nback "${analysis_param_type.homopolymer_nback}"
+${analysis_param_type.do_not_write_original_quals}
+'
+#end if
+</command>
+<inputs>
+<param name="input_recal" type="data" format="csv" label="Covariates table recalibration file" help="-recalFile,--recal_file &amp;lt;recal_file&amp;gt;" />
+<conditional name="reference_source">
+<expand macro="reference_source_selector_param" />
+<when value="cached">
+<param name="input_bam" type="data" format="bam" label="BAM file" help="-I,--input_file &amp;lt;input_file&amp;gt;">
+<validator type="unspecified_build" />
+<validator type="dataset_metadata_in_data_table" table_name="gatk_picard_indexes" metadata_name="dbkey" metadata_column="dbkey" message="Sequences are not currently available for the specified build." /> <!-- fixme!!! this needs to be a select -->
+</param>
+<param name="ref_file" type="select" label="Using reference genome" help="-R,--reference_sequence &amp;lt;reference_sequence&amp;gt;" >
+<options from_data_table="gatk_picard_indexes">
+<filter type="data_meta" key="dbkey" ref="input_bam" column="dbkey"/>
+</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="input_bam" type="data" format="bam" label="BAM file" help="-I,--input_file &amp;lt;input_file&amp;gt;" />
+<param name="ref_file" type="data" format="fasta" label="Using reference file" help="-R,--reference_sequence &amp;lt;reference_sequence&amp;gt;">
+<options>
+<filter type="data_meta" key="dbkey" ref="input_bam" />
+</options>
+</param>
+</when>
+</conditional>
+<expand macro="gatk_param_type_conditional" />
+<expand macro="analysis_type_conditional">
+<conditional name="default_read_group_type">
+<param name="default_read_group_type_selector" type="select" label="Set default Read Group" help="--default_read_group">
+<option value="default" selected="True">Don't Set</option>
+<option value="set">Set</option>
+</param>
+<when value="default">
+<!-- do nothing here -->
+</when>
+<when value="set">
+<param name="default_read_group" type="text" value="Unknown" label="If a read has no read group then default to the provided String"/>
+</when>
+</conditional>
+<param name="default_platform" type="select" label="Set default Platform" help="--default_platform">
+<option value="default" selected="True">Don't Set</option>
+<option value="illumina">illumina</option>
+<option value="454">454</option>
+<option value="solid">solid</option>
+</param>
+<conditional name="force_read_group_type">
+<param name="force_read_group_type_selector" type="select" label="Force Read Group" help="--force_read_group">
+<option value="default" selected="True">Don't Force</option>
+<option value="set">Force</option>
+</param>
+<when value="default">
+<!-- do nothing here -->
+</when>
+<when value="set">
+<param name="force_read_group" type="text" value="Unknown" label="If provided, the read group ID of EVERY read will be forced to be the provided String."/>
+</when>
+</conditional>
+<param name="force_platform" type="select" label="Force Platform" help="--force_platform">
+<option value="default" selected="True">Don't Force</option>
+<option value="illumina">illumina</option>
+<option value="454">454</option>
+<option value="solid">solid</option>
+</param>
+<param name="exception_if_no_tile" type="boolean" checked="False" truevalue="--exception_if_no_tile" falsevalue="" label="Throw an exception when no tile can be found" help="--exception_if_no_tile"/>
+<conditional name="solid_options_type">
+<param name="solid_options_type_selector" type="select" label="Set SOLiD specific options">
+<option value="default" selected="True">Don't Set</option>
+<option value="set">Set</option>
+</param>
+<when value="default">
+<!-- do nothing here -->
+</when>
+<when value="set">
+<param name="solid_recal_mode" type="select" label="How should we recalibrate solid bases in which the reference was inserted" help="-sMode,--solid_recal_mode &amp;lt;solid_recal_mode&amp;gt;">
+<option value="default" selected="True">Don't set</option>
+<option value="DO_NOTHING">DO_NOTHING</option>
+<option value="SET_Q_ZERO">SET_Q_ZERO</option>
+<option value="SET_Q_ZERO_BASE_N">SET_Q_ZERO_BASE_N</option>
+<option value="REMOVE_REF_BIAS">REMOVE_REF_BIAS</option>
+</param>
+<param name="solid_nocall_strategy" type="select" label="Behavior of the recalibrator when it encounters no calls" help="-solid_nocall_strategy,--solid_nocall_strategy &amp;lt;solid_nocall_strategy&amp;gt;">
+<option value="default" selected="True">Don't set</option>
+<option value="THROW_EXCEPTION">THROW_EXCEPTION</option>
+<option value="LEAVE_READ_UNRECALIBRATED">LEAVE_READ_UNRECALIBRATED</option>
+<option value="PURGE_READ">PURGE_READ</option>
+</param>
+</when>
+</conditional>
+<param name="simplify_bam" type="boolean" checked="False" truevalue="-simplifyBAM" falsevalue="" label="Simplify BAM" help="-simplifyBAM,--simplifyBAM"/>
+<param name="window_size_nqs" type="integer" value="5" label="Window size used by MinimumNQSCovariate" help="--window_size_nqs"/>
+<param name="homopolymer_nback" type="integer" value="7" label="Number of previous bases to look at in HomopolymerCovariate" help="-nback,--homopolymer_nback &amp;lt;homopolymer_nback&amp;gt;" />
+<param name="preserve_qscores_less_than" type="integer" value="5" label="Bases with quality scores less than this threshold won't be recalibrated" help="-pQ,--preserve_qscores_less_than &amp;lt;preserve_qscores_less_than&amp;gt;"/>
+<param name="smoothing" type="integer" value="1" label="smoothing" help="-sm,--smoothing &amp;lt;smoothing&amp;gt;"/>
+<param name="max_quality_score" type="integer" value="50" label="Max quality score" help="-maxQ,--max_quality_score &amp;lt;max_quality_score&amp;gt;"/>
+<param name="do_not_write_original_quals" type="boolean" checked="False" truevalue="--doNotWriteOriginalQuals" falsevalue="" label="Do Not Write Original Quality tag" help="-noOQs,--doNotWriteOriginalQuals"/>
+</expand>
+</inputs>
+<outputs>
+<data format="bam" name="output_bam" label="${tool.name} on ${on_string} (BAM)" />
+<data format="txt" name="output_log" label="${tool.name} on ${on_string} (log)" />
+</outputs>
+<tests>
+<test>
+<param name="input_recal" value="gatk/gatk_count_covariates/gatk_count_covariates_out_1.csv" ftype="csv" />
+<param name="reference_source_selector" value="history" />
+<param name="ref_file" value="phiX.fasta" ftype="fasta" />
+<param name="input_bam" value="gatk/gatk_indel_realigner/gatk_indel_realigner_out_1.bam" ftype="bam" />
+<param name="gatk_param_type_selector" value="basic" />
+<param name="analysis_param_type_selector" value="basic" />
+<output name="output_bam" file="gatk/gatk_table_recalibration/gatk_table_recalibration_out_1.bam" ftype="bam" lines_diff="4" />
+<output name="output_log" file="gatk/gatk_table_recalibration/gatk_table_recalibration_out_1.log.contains" compare="contains" />
+</test>
+</tests>
+<help>
+**What it does**
+This walker is designed to work as the second pass in a two-pass processing step, doing a by-read traversal.  For each base in each read this walker calculates various user-specified covariates (such as read group, reported quality score, cycle, and dinuc) Using these values as a key in a large hashmap the walker calculates an empirical base quality score and overwrites the quality score currently in the read. This walker then outputs a new bam file with these updated (recalibrated) reads.  Note: This walker expects as input the recalibration table file generated previously by CovariateCounterWalker. Note: This walker is designed to be used in conjunction with CovariateCounterWalker.
+For more information on base quality score recalibration using the GATK, see this `tool specific page &lt;http://www.broadinstitute.org/gsa/wiki/index.php/Base_quality_score_recalibration&gt;`_.
+To learn about best practices for variant detection using GATK, see this `overview &lt;http://www.broadinstitute.org/gsa/wiki/index.php/Best_Practice_Variant_Detection_with_the_GATK_v3&gt;`_.
+If you encounter errors, please view the `GATK FAQ &lt;http://www.broadinstitute.org/gsa/wiki/index.php/Frequently_Asked_Questions&gt;`_.
+------
+**Inputs**
+GenomeAnalysisTK: TableRecalibration accepts an aligned BAM and a recalibration CSV input files.
+**Outputs**
+The output is in BAM format.
+Go `here &lt;http://www.broadinstitute.org/gsa/wiki/index.php/Input_files_for_the_GATK&gt;`_ for details on GATK file formats.
+-------
+**Settings**::
+default_read_group             If a read has no read group then default to the provided String.
+default_platform               If a read has no platform then default to the provided String. Valid options are illumina, 454, and solid.
+force_read_group               If provided, the read group ID of EVERY read will be forced to be the provided String. This is useful to collapse all data into a single read group.
+force_platform                 If provided, the platform of EVERY read will be forced to be the provided String. Valid options are illumina, 454, and solid.
+window_size_nqs                The window size used by MinimumNQSCovariate for its calculation
+homopolymer_nback              The number of previous bases to look at in HomopolymerCovariate
+exception_if_no_tile           If provided, TileCovariate will throw an exception when no tile can be found. The default behavior is to use tile = -1
+solid_recal_mode               How should we recalibrate solid bases in whichthe reference was inserted? Options = DO_NOTHING, SET_Q_ZERO, SET_Q_ZERO_BASE_N, or REMOVE_REF_BIAS (DO_NOTHING|SET_Q_ZERO|SET_Q_ZERO_BASE_N|REMOVE_REF_BIAS)
+solid_nocall_strategy          Defines the behavior of the recalibrator when it encounters no calls in the color space. Options = THROW_EXCEPTION, LEAVE_READ_UNRECALIBRATED, or PURGE_READ (THROW_EXCEPTION|LEAVE_READ_UNRECALIBRATED|PURGE_READ)
+recal_file                     Filename for the input covariates table recalibration .csv file
+out                            The output BAM file
+bam_compression                Compression level to use for writing BAM files
+disable_bam_indexing           Turn off on-the-fly creation of indices for output BAM files.
+simplifyBAM                    If provided, output BAM files will be simplified to include just key reads for downstream variation discovery analyses (removing duplicates, PF-, non-primary reads), as well stripping all extended tags from the kept reads except the read group identifier
+preserve_qscores_less_than     Bases with quality scores less than this threshold won't be recalibrated, default=5. In general it's unsafe to change qualities scores below &lt; 5, since base callers use these values to indicate random or bad bases
+smoothing                      Number of imaginary counts to add to each bin bin order to smooth out bins with few data points, default=1
+max_quality_score              The integer value at which to cap the quality scores, default=50
+doNotWriteOriginalQuals        If true, we will not write the original quality (OQ) tag for each read
+@CITATION_SECTION@
+</help>
+</tool>

Mercurial > repos > devteam > table_recalibration

comparison table_recalibration.xml @ 1:30e1dd77e99c draft default tip