Mercurial > repos > kevyin > homer
diff findPeaks.xml @ 16:687df269e597 draft
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author | kevyin |
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date | Wed, 19 Dec 2012 17:28:55 -0500 |
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--- /dev/null Thu Jan 01 00:00:00 1970 +0000 +++ b/findPeaks.xml Wed Dec 19 17:28:55 2012 -0500 @@ -0,0 +1,122 @@ +<tool id="homer_findPeaks" name="homer_findPeaks" version="0.1.2"> + <requirements> + <requirement type="package" version="4.1">homer</requirement> + </requirements> + <description>Homer's peakcaller. Requires tag directories (see makeTagDirectory)</description> + <!--<version_command></version_command>--> + <command> + findPeaks $tagDir.extra_files_path $options -o $outputPeakFile + + #if $control_tagDir: + -i $control_tagDir.extra_files_path + #end if + + 2> $out_log || echo "Error running findPeaks." >&2 + </command> + <inputs> + <param format="homerTagDirectory" name="tagDir" type="data" label="tag directory" help="Must be made with homer_makeTagDirectory" /> + <param format="homerTagDirectory" name="control_tagDir" type="data" optional="True" label="Control tag directory" help="Must be made with homer_makeTagDirectory" /> + <param type="text" name="options" label="Extra options" value="" help="See link below for more options"> + <sanitizer> + <valid initial="string.printable"> + <remove value="'"/> + <remove value="/"/> + </valid> + <mapping initial="none"> + <add source="'" target="__sq__"/> + </mapping> + </sanitizer> + </param> + </inputs> + <outputs> + <!--<data format="html" name="html_outfile" label="index" />--> + <!--<data format="html" hidden="True" name="html_outfile" label="index.html" />--> + <data format="txt" name="outputPeakFile" label="${tool.name} on #echo os.path.splitext(str($tagDir.name))[0]#.txt" /> + <data format="txt" name="out_log" label="${tool.name} on #echo os.path.splitext(str($tagDir.name))[0]#.log" /> + </outputs> + <tests> + <test> + <!--<param name="input_file" value="extract_genomic_dna.fa" />--> + <!--<output name="html_file" file="sample_output.html" ftype="html" />--> + </test> + </tests> + + <help> + + .. class:: infomark + + **Homer findPeaks** + + For more options, look under: "Command line options for findPeaks" + + http://biowhat.ucsd.edu/homer/ngs/peaks.html + + TIP: use homer_bed2pos and homer_pos2bed to convert between the homer peak positions and the BED format. + +**Parameter list** + +Command line options (not all of them are supported):: + + Usage: findPeaks <tag directory> [options] + + Finds peaks in the provided tag directory. By default, peak list printed to stdout + + General analysis options: + -o <filename|auto> (file name for to output peaks, default: stdout) + "-o auto" will send output to "<tag directory>/peaks.txt", ".../regions.txt", + or ".../transcripts.txt" depending on the "-style" option + -style <option> (Specialized options for specific analysis strategies) + factor (transcription factor ChIP-Seq, uses -center, output: peaks.txt, default) + histone (histone modification ChIP-Seq, region based, uses -region -size 500 -L 0, regions.txt) + groseq (de novo transcript identification from GroSeq data, transcripts.txt) + tss (TSS identification from 5' RNA sequencing, tss.txt) + dnase (Hypersensitivity [crawford style (nicking)], peaks.txt) + + chipseq/histone options: + -i <input tag directory> (Experiment to use as IgG/Input/Control) + -size <#> (Peak size, default: auto) + -minDist <#> (minimum distance between peaks, default: peak size x2) + -gsize <#> (Set effective mappable genome size, default: 2e9) + -fragLength <#|auto> (Approximate fragment length, default: auto) + -inputFragLength <#|auto> (Approximate fragment length of input tags, default: auto) + -tbp <#> (Maximum tags per bp to count, 0 = no limit, default: auto) + -inputtbp <#> (Maximum tags per bp to count in input, 0 = no limit, default: auto) + -strand <both|separate> (find peaks using tags on both strands or separate, default:both) + -norm # (Tag count to normalize to, default 10000000) + -region (extends start/stop coordinates to cover full region considered "enriched") + -center (Centers peaks on maximum tag overlap and calculates focus ratios) + -nfr (Centers peaks on most likely nucleosome free region [works best with mnase data]) + (-center and -nfr can be performed later with "getPeakTags" + + Peak Filtering options: (set -F/-L/-C to 0 to skip) + -F <#> (fold enrichment over input tag count, default: 4.0) + -P <#> (poisson p-value threshold relative to input tag count, default: 0.0001) + -L <#> (fold enrichment over local tag count, default: 4.0) + -LP <#> (poisson p-value threshold relative to local tag count, default: 0.0001) + -C <#> (fold enrichment limit of expected unique tag positions, default: 2.0) + -localSize <#> (region to check for local tag enrichment, default: 10000) + -inputSize <#> (Size of region to search for control tags, default: 2x peak size) + -fdr <#> (False discovery rate, default = 0.001) + -poisson <#> (Set poisson p-value cutoff, default: uses fdr) + -tagThreshold <#> (Set # of tags to define a peak, default: 25) + -ntagThreshold <#> (Set # of normalized tags to define a peak, by default uses 1e7 for norm) + -minTagThreshold <#> (Absolute minimum tags per peak, default: expected tags per peak) + + GroSeq Options: (Need to specify "-style groseq"): + -tssSize <#> (size of region for initiation detection/artifact size, default: 250) + -minBodySize <#> (size of regoin for transcript body detection, default: 1000) + -maxBodySize <#> (size of regoin for transcript body detection, default: 10000) + -tssFold <#> (fold enrichment for new initiation dectection, default: 4.0) + -bodyFold <#> (fold enrichment for new transcript dectection, default: 4.0) + -endFold <#> (end transcript when levels are this much less than the start, default: 10.0) + -fragLength <#> (Approximate fragment length, default: 150) + -uniqmap <directory> (directory of binary files specifying uniquely mappable locations) + Download from http://biowhat.ucsd.edu/homer/groseq/ + -confPvalue <#> (confidence p-value: 1.00e-05) + -minReadDepth <#> (Minimum initial read depth for transcripts, default: auto) + -pseudoCount <#> (Pseudo tag count, default: 2.0) + -gtf <filename> (Output de novo transcripts in GTF format) + "-o auto" will produce <dir>/transcripts.txt and <dir>/transcripts.gtf + </help> +</tool> +