Mercurial > repos > jjohnson > igvtools
view igvtools_count.xml @ 1:ae2bc4e5fefc draft default tip
Fix igvtools_tile.xml tdf output and add log file output
| author | Jim Johnson <jj@umn.edu> |
|---|---|
| date | Tue, 27 Nov 2012 16:32:10 -0600 |
| parents | 2eb1e2924c1a |
| children |
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<tool id="igvtools_count" name="IGVtools count" version="1.0"> <description>average feature density across the genome</description> <command interpreter="bash">igvtools count #if $zoom.__str__ != '': -z $zoom #end if #if $window.__str__ != '': -w $window #end if #if $extend.__str__ != '': -e $extend #end if #if $window_functions.__str__ != '': -f '$window_functions' #end if ## IGVTools relies on the file extension to determine format #if $input.datatype.file_ext == 'bam': #set $input_name='input_file.bam' #elif $input.datatype.file_ext == 'sam': #set $input_name='input_file.sam' #elif $input.datatype.file_ext == 'bed': #set $input_name='input_file.bed' #elif $input.datatype.file_ext == 'psl': #set $input_name='input_file.psl' #end if `ln -s $input $input_name; echo $input_name` '$output_fmt' $refGenomeSource.ref </command> <inputs> <conditional name="refGenomeSource"> <param name="refGenomeSource_type" type="select" label="Will you select a reference genome from your history or use a built-in reference?"> <option value="built-in">Use a built-in reference</option> <option value="history">Use one from the history</option> </param> <when value="built-in"> <param name="ref" type="select" label="Select a reference genome"> <options from_file="igv_indices.loc"> <column name="dbkey" index="0" /> <column name="name" index="1" /> <column name="value" index="2" /> <filter type="sort_by" column="1" /> <validator type="no_options" message="No indexes are available" /> </options> </param> </when> <when value="history"> <param name="ref" type="data" format="igv.genome" metadata_name="dbkey" label="Select a reference from history" /> </when> </conditional> <param name="input" type="data" format="sam,bam,bed,psl" label="Input file" help="The input BAM,SAM,BED,PSL feature file"/> <param name="zoom" type="integer" value="7" optional="true" label="-z maximum zoom level to precompute" help="The default value is 7 and is sufficient for most files. To reduce file size at the expense of IGV performance this value can be reduced." /> <param name="window" type="integer" value="25" optional="true" label="-w Window size" help="The window size over which coverage is averaged. Defaults to 25 bp." /> <param name="extend" type="integer" value="" optional="true" label="Extend feature length" help="The read or feature is extended by the specified distance in bp prior to counting. This option is useful for chip-seq and rna-seq applications. The value is generally set to the average fragment length of the library." /> <param name="window_functions" type="select" display="checkboxes" multiple="True" label="-f Functions to calculate over windows" help="If none are selected, will default to mean"> <option value="mean" selected="true">mean</option> <option value="min">min</option> <option value="max">max</option> </param> <param name="output_fmt" type="select" display="checkboxes" multiple="True" force_select="true" label="Select output format" help="If none are selected, will default to mean"> <option value="output.tdf" selected="true">IGV tdf</option> <option value="output.wig">wig</option> </param> </inputs> <outputs> <data format="igv.tdf" name="output_tdf" metadata_source="input" label="${tool.name} on ${on_string}: igv.tdf" from_work_dir="output.tdf"> <filter>('output.tdf' in output_fmt)</filter> </data> <data format="wig" name="output_wig" metadata_source="input" label="${tool.name} on ${on_string}: igv.wig" from_work_dir="output.wig"> <filter>('output.wig' in output_fmt)</filter> </data> </outputs> <tests> </tests> <help> **What it does** The IGVTools_ count command computes average feature density over a specified window size across the genome. Common usages include computing coverage for alignment files and counting hits in Chip-seq experiments. By default, the resulting file will be displayed as a bar chart when loaded into IGV_. .. _IGVTools: http://www.broadinstitute.org/software/igv/igvtools_commandline .. _IGV: http://www.broadinstitute.org/igv/ ------ To cite your use of IGV in your publication:: James T. Robinson, Helga Thorvaldsdottir, Wendy Winckler, Mitchell Guttman, Eric S. Lander, Gad Getz, Jill P. Mesirov. Integrative Genomics Viewer. Nature Biotechnology 29, 24-26 (2011) ------ **Input formats** Supported input file formats are: .sam, .bam, .aligned, .psl, .pslx, and .bed. ------ **Outputs** The output formats are IGV tiled data file (TDF) file (.tdf) and/or WIG file (.wig) ------- **IGVTools count parameter list** This is an exhaustive list of igvtools count options: For **count**:: -z Integer Specifies the maximum zoom level to precompute. The default value is 7 and is sufficient for most files. To reduce file size at the expense of IGV performance this value can be reduced. -w Integer The window size over which coverage is averaged. Defaults to 25 bp. -e Integer The read or feature is extended by the specified distance in bp prior to counting. This option is useful for chip-seq and rna-seq applications. The value is generally set to the average fragment length of the library. -f list A comma delimited list specifying window functions to use when reducing the data to precomputed tiles. Possible values are min, max, and mean. By default only the mean is calculated. </help> </tool>