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| author | spanish_national_institue_of_bioinformatics |
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| date | Fri, 12 Apr 2019 05:28:43 -0400 |
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<tool id="nucleR" name="NucleR" version="0.1"> <description>: analyze aligned BAM files from MNAse (in RData format)</description> <requirements> <requirement type="binary">docker</requirement> </requirements> <command> <![CDATA[ docker run -v $__root_dir__/database/files:$__root_dir__/database/files -v /tmp:/tmp -u `id -u`:`id -g` mmbirb/nucleosome-dynamics nucleR --input $rdata_file --output $output_gff_file --type $seq_type --width $width --minoverlap $minoverlap --dyad_length $dyad_length --hthresh $hthres --wthresh $wthres --pcKeepComp $pcKeepComp --fdrOverAmp $fdrOverAmp --trim $trim --fragmentLen $fragmentLen #if $threshold.is == "absolute": --thresholdValue ${threshold.thresholdValue} #else if $threshold.is == "percentage": --thresholdPercentage ${threshold.thresholdPercentage} #end if #if $chr --chr $chr #end if #if $start --start $start #end if #if $end --end $end #end if #if $comp --components $comp #end if ]]> </command> <inputs> <param name="rdata_file" type="data" format="rdata" label="Input MNase-seq/ATAC-seq reads (RData)" help="Input BAM file in RData format as generated by readBAM."/> <param name="seq_type" type="select" label="Type of sequence reads"> <option value="paired">Paired</option> <option value="single">Single</option> </param> <param name="width" size="4" type="integer" value="147" label="Width (bp)" help="Size of each nucleosome."/> <param name="minoverlap" type="integer" value="80" label="Minimum Overlap (bp)" help="Minimum overlap between two nucleosomes for merging them."/> <param name="dyad_length" type="integer" value="50" label="Dyad length (bp)" help="Lenght of the reads that should be used for nucleosome calling to define the dyad of the nucleosomes keeping the number of bases around the center of the read."/> <param name="fragmentLen" type="integer" value="170" label="Fragment Length (bp)" help="Maximum fragment length allowed (bp)" optional="True" /> <param name="chr" type="text" value="" label="Chromosome" optional="True" help="Chromosome to consider for the analysis in the given input file."/> <param name="start" type="integer" value="" label="Start" optional="True" help="Start genomic position to consider for the analysis in the given input file."/> <param name="end" type="integer" value="" label="End" optional="True" help="End genomic position to consider for the analysis in the given input file."/> <param name="comp" type="integer" value="1" label="Components" optional="True" help="Number of negative binomials that will be used to filter duplicated reads."/> <conditional name="threshold"> <param name="is" type="select" label="Background threshold" help="Minimum number of reads (Coverage) to call a nucleosome. Can be given as a percentage, or an absolute number of reads."> <option value="percentage" selected="True">use a percentage</option> <option value="absolute">use a number of reads</option> </param> <when value="absolute"> <param name="thresholdValue" type="integer" value="10" label="Bakground level (reads)" help="Absolute value to filter out nucleosome calls. It is the minimum number of reads (coverage) in a nucleosome call expressed as reads per million of mapped reads."/> </when> <when value="percentage"> <param name="thresholdPercentage" type="float" value="35" label="Background level (%)" help="Percentile of coverage in the experiment used as threshold to filter out nucleosome calls (i.e., 25% would mean that only peaks with coverage in the 1st quantile would be considered)"/> </when> </conditional> <param name="hthres" type="float" value="0.4" label="Height Threshold" help="Height threshold (between 0 and 1) to classify a nucleosome as fuzzy (class=F) or well-positioned ( class=W) according to the number of reads at the dyad. Nucleosomes below this value will be defined as fuzzy."/> <param name="wthres" type="float" value="0.6" label="Width Threshold" help="Width threshold (between 0 and 1) to classify a nucleosome as fuzzy (class=F) or well-positioned (class=W) according to the dispersion of the reads around the dyad."/> <param name="fdrOverAmp" type="float" value="0.05" label="fdrOverAmp" help="Threshold to filter over-amplified reads , as defined in filterDuplReads function of htSetqTools R package."/> <param name="pcKeepComp" type="float" value="0.02" label="Coverage Smoothing" help="Parameter used in the smoothing when Fourier transformation is applied. Number of components to select with respect to the total size of the sample. Allowed values are numeric (in range 0:1) for manual setting, or auto for automatic detection."/> <param name="trim" type="integer" value="50" label="Trim" help="Number of basepairs to keep from each read (or to extend in case it is larger than the read width)."/> </inputs> <outputs> <data format="gff" name="output_gff_file" label="NR__${os.path.splitext(($rdata_file.name.split('__'))[1])[0]}.gff" /> </outputs> <tests> <test> <param name="rdata_file" value="readBAM__cellcycleM_chrII.RData" /> <param name="seq_type" value="paired" /> <param name="width" value="147" /> <param name="minoverlap" value="80" /> <param name="dyad_length" value="50" /> <param name="thresholdPercentage" value="35" /> <param name="hthres" value="0.4" /> <param name="wthres" value="0.6" /> <param name="pcKeepComp" value="0.02" /> <output name="output_gff_file" file="NR__cellcycleM_chrII.gff" /> </test> </tests> <help> .. image:: ${static_path}/images/NucleosomeDynamicsLogo.png :height: 80 :width: 200 ----- Nucleosome Dynamics is a set of tools that take MNase-seq and ATAC-seq aligned reads and performs a serie of nucleosome-related analyses on them. .. class:: infomark Visit the documentation of the original application for learning more about the accepted values and formats. http://mmb.irbbarcelona.org/NucleosomeDynamics/help/usage/nucleosome-dynamics </help> <citations> <citation type="bibtex"> @misc{github, author = {Buitrago D}, year = {2019}, title = {Nucleosome Dynamics suite: containerized installation}, publisher = {Github}, journal = {GitHub repository}, url = {https://github.com/nucleosome-dynamics/nucleosome_dynamics}, }</citation> </citations> </tool>