Mercurial > repos > bgruening > hicexplorer_hicmergematrixbins
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planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/hicexplorer commit 69bb60ab875c1c1769298678f0890d8b92f1899d
author | iuc |
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date | Thu, 05 Dec 2024 18:29:04 +0000 |
parents | 11fa44ee0603 |
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<tool id="hicexplorer_hicmergematrixbins" name="@BINARY@" version="@TOOL_VERSION@+galaxy@VERSION_SUFFIX@" profile="@PROFILE@"> <description>merge adjacent bins from a Hi-C contact matrix to reduce its resolution</description> <macros> <token name="@BINARY@">hicMergeMatrixBins</token> <import>macros.xml</import> </macros> <expand macro="requirements" /> <command detect_errors="exit_code"><![CDATA[ ln -s '$matrix_h5_cooler' 'matrix.$matrix_h5_cooler.ext' && @BINARY@ --matrix 'matrix.$matrix_h5_cooler.ext' --numBins $numBins $runningWindow --outFileName 'out_matrix.$matrix_h5_cooler.ext' && mv 'out_matrix.$matrix_h5_cooler.ext' matrix ]]> </command> <inputs> <expand macro="matrix_h5_cooler_macro" /> <param argument="--numBins" type="integer" min="1" value="3" label="Number of bins to merge" /> <param argument="--runningWindow" type="boolean" falsevalue="" truevalue="--runningWindow" label="Set to merge for using a running window of length --numBins. Usually not set." /> </inputs> <outputs> <data name="outFileName" from_work_dir="matrix" format="cool"> <change_format> <when input_dataset="matrix_h5_cooler" attribute="ext" value="h5" format="h5" /> </change_format> </data> </outputs> <tests> <test> <param name="matrix_h5_cooler" value="small_test_matrix.h5" /> <param name="numBins" value="5" /> <output name="outFileName" ftype="h5"> <assert_contents> <has_h5_keys keys="intervals,matrix,nan_bins" /> </assert_contents> </output> </test> </tests> <help><![CDATA[ Change matrix resolution ======================== **hicMergeMatrixBins** is used to decrease the resolution of a matrix. With this tool, you can for example create out of a 100 kb contact matrix a 1000 kb one: Number of bins to merge = 10 100 kb * 10 = 1000 kb = 1 Mb Depending on the downstream analyses to perform on a Hi-C matrix generated with HiCExplorer, one might need different bin resolutions. For example using ``hicPlotMatrix`` to display chromatin interactions of a whole chromosome will not produce any meaningful vizualisation if it is performed on a matrix at restriction sites resolution (unmerged). Furthermore, the higher the resolution of a matrix, the more detailed it is, which can make it difficult to interpret, especially if the read depth of the Hi-C data is not high enough. **hicMergeMatrixBins** address these issues by merging a given number of adjacent bins to reduce Hi-C matrices resolution. _________________ Usage ----- To limit the loss of information, it is mandatory to perform **hicMergeMatrixBins** on matrices prior to any correction and any other bin merging (direct output from ``hicBuildMatrix``). After bin merging, ``hicCorrectMatrix`` must be used for downstream analyses requiring corrected matrices. _________________ Output ------ **hicMergeMatrixBins** outputs a Hi-C matrix with reduced resolution. Below, we will develop the example of a Hi-C matrix in *Drosophila melanogaster* that we want to display at the whole X-chromosome scale and at the scale of a 1Mb region of the X chromosome. To do this, we performed two different bin merging using **hicMergeMatrixBins** on an uncorrected matrix built at the restiction sites resolution using ``hicBuildMatrix``. Starting from a matrix with bins of a median length of 529bp (restriction enzyme resolution, here DpnII), running **hicMergeMatrixBins** with a number of bins to merge of 3 produced a matrix with bins of a median length of 1661bp, while **hicMergeMatrixBins** with a number of bins to merge of 50 produced a matrix with bins of a median length of 29798bp. After the correction of these three matrices using ``hicCorrectMatrix``, we plotted them using ``hicPlotMatrix`` at the scale of the whole X-chromosome and at the scale of the X:2000000-3000000 region to see the effect of bin merging on the interactions visualization. - **Effect of bins merging at the scale of a chromosome:** .. image:: $PATH_TO_IMAGES/hicMergeMatrixBins_Xchr.png :width: 60 % When observed altogether, the plots above show that the merging of bins by 50 is the most adequate way to plot interactions for a whole chromosome in *Drosophila melanogaster* when starting from a matrix with bins of a median length of 529bp. - **Effect of bins merging at the scale of a specific region:** .. image:: $PATH_TO_IMAGES/hicMergeMatrixBins_Xregion.png :width: 60 % When observed altogether, the plots above show that the merging of bins by 3 is the most adequate way to plot interactions for a region of 1Mb in Drosophila melanogaster when starting from a matrix with bins of a median length of 529bp. _________________ | For more information about HiCExplorer please consider our documentation on readthedocs.io_ .. _readthedocs.io: http://hicexplorer.readthedocs.io/en/latest/index.html ]]> </help> <expand macro="citations" /> </tool>