annotate hd.xml @ 20:b084b6a8e3ac draft

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author mheinzl
date Fri, 14 Dec 2018 04:31:21 -0500
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1 <?xml version="1.0" encoding="UTF-8"?>
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2 <tool id="hd" name="HD:" version="1.0.0">
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3 <description>hamming distance analysis of duplex tags</description>
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4 <requirements>
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5 <requirement type="package" version="2.7">python</requirement>
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6 <requirement type="package" version="1.4.0">matplotlib</requirement>
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7 </requirements>
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8 <command>
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9 python2 '$__tool_directory__/hd.py' --inputFile '$inputFile' --inputName1 '$inputFile.name' --sample_size $sampleSize --subset_tag $subsetTag --nproc $nproc $onlyDCS --minFS $minFS --maxFS $maxFS
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10 $nr_above_bars --output_pdf $output_pdf --output_tabular $output_tabular
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11 </command>
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12 <inputs>
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13 <param name="inputFile" type="data" format="tabular" label="Dataset 1: input tags" optional="false" help="Input in tabular format with the family size, tag and the direction of the strand ('ab' or 'ba') for each family."/>
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14 <param name="sampleSize" type="integer" label="number of tags in the sample" value="1000" min="0" help="specifies the number of tags in one analysis. If sample size is 0, all tags of the dataset are compared against all tags."/>
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15 <param name="minFS" type="integer" label="minimum family size of the tags" min="1" value="1" help="filters the tags after their family size: Families with a smaller size are skipped. Default: min. family size = 1."/>
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16 <param name="maxFS" type="integer" label="max family size of the tags" min="0" value="0" help="filters the tags after their family size: Families with a larger size are skipped. If max. family size is 0, no upper bound is defined and the maximum family size in the analysis will be the maximum family size of the whole dataset. Default: max. family size = 0."/>
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17 <param name="onlyDCS" type="boolean" label="only DCS in the analysis?" truevalue="" falsevalue="--only_DCS" checked="False" help="Only tags, which have a partner tag (ab and ba) in the dataset, are included in the analysis."/>
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18 <param name="subsetTag" type="integer" label="shorten tag in the analysis?" value="0" help="By this parameter an analysis with shorter tag length is simulated. If this parameter is 0 (by default), the tags with its original length are used in the analysis."/>
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19 <param name="nproc" type="integer" label="number of processors" value="8" help="Number of processor used for computing."/>
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20 <param name="nr_above_bars" type="boolean" label="include numbers above bars?" truevalue="--nr_above_bars" falsevalue="" checked="True" help="The absolute and relative values of the data can be included or removed from the plots. "/>
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21
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22 </inputs>
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23 <outputs>
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24 <data name="output_tabular" format="tabular"/>
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25 <data name="output_pdf" format="pdf" />
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26 </outputs>
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27 <tests>
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28 <test>
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29 <param name="inputFile" value="Test_data.tabular"/>
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30 <param name="sampleSize" value="0"/>
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31 <output name="output_pdf" file="output_file.pdf" lines_diff="6"/>
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32 <output name="output_tabular" file="output_file.tabular"/>
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33 </test>
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34 </tests>
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35 <help> <![CDATA[
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36 **What it does**
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37
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38 This tool calculates the Hamming distance for the tags by comparing them to all tags in the dataset and finally searches for the minimum Hamming distance.
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39 The Hamming distance is shown in a histogram separated by the family sizes or in a family size distribution separated by the Hamming distances.
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40 This similarity measure was calculated for each tag to distinguish whether similar tags truly stem from different molecules or occured due to sequencing or PCR errros.
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41 In addition, the tags of chimeric reads can be identified by calculating the Hamming distance for each half of the tag.
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42 This analysis can be performed on only a sample (by default: sample size=1000) or on the whole dataset (sample size=0).
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43 It is also possible to select on only those tags, which have a partner tag (ab and ba) in the dataset (DCSs) or to filter the dataset after the tag's family size.
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44
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45 **Input**
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46
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47 This tools expects a tabular file with the tags of all families, their sizes and information about forward (ab) and reverse (ba) strands::
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48
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49 1 AAAAAAAAAAAATGTTGGAATCTT ba
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50 10 AAAAAAAAAAAGGCGGTCCACCCC ab
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51 28 AAAAAAAAAAATGGTATGGACCGA ab
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53 **How to generate the input**
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55 The first step of the `Du Novo Analysis Pipeline <https://doi.org/10.1186/s13059-016-1039-4>`_ is the **Make Families** tool that produces output in this form::
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57 1 2 3 4
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58 ------------------------------------------------------
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59 AAAAAAAAAAAAAAATAGCTCGAT ba read1 CGCTACGTGACTGGGTCATG
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60 AAAAAAAAAAAAAAATAGCTCGAT ba read2 CGCTACGTGACTGGGTCATG
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61 AAAAAAAAAAAAAAATAGCTCGAT ba read3 CGCTACGTGACTGGGTCATG
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63 we only need columns 1 and 2. These two columns can be extracted from this dataset using **Cut** tool::
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65 1 2
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66 ---------------------------
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67 AAAAAAAAAAAAAAATAGCTCGAT ba
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68 AAAAAAAAAAAAAAATAGCTCGAT ba
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69 AAAAAAAAAAAAAAATAGCTCGAT ba
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71 now one needs to count the number of unique occurencies of each tag. This is done using **Unique lines** tool, which would add an additional column containg counts (column 1)::
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74 1 2 3
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75 -----------------------------
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76 3 AAAAAAAAAAAAAAATAGCTCGAT ba
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78 these data can now be used in this tool.
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81 **Output**
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82
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83 The output is one PDF file with the plots of the Hamming distance and a tabular file with the data of the plot for each dataset.
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84
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85
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86 **About Author**
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87
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88 Author: Monika Heinzl
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89
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90 Department: Institute of Bioinformatics, Johannes Kepler University Linz, Austria
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91
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92 Contact: monika.heinzl@edumail.at
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93
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94 ]]>
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95
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96 </help>
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97 <citations>
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98 <citation type="bibtex">
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99 @misc{duplex,
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100 author = {Heinzl, Monika},
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101 year = {2018},
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102 title = {Development of algorithms for the analysis of duplex sequencing data}
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103 }
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104 </citation>
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105 </citations>
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106 </tool>