annotate computeGCBias.xml @ 17:1795fdfc23b8 draft

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1 <tool id="deeptools_compute_gc_bias" name="computeGCBias" version="@WRAPPER_VERSION@.0">
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2 <description>Determine the GC bias of your sequenced reads</description>
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3 <macros>
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4 <token name="@BINARY@">computeGCBias</token>
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5 <import>deepTools_macros.xml</import>
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6 </macros>
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7 <expand macro="requirements" />
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8 <command>
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9 <![CDATA[
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10 ln -s "$bamInput" "local_bamInput.bam" &&
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11 #if $bamInput.ext == 'bam':
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12 ln -s '${bamInput.metadata.bam_index}' local_bamInput.bam.bai &&
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13 #else:
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14 ln -s '${bamInput.metadata.cram_index}' local_bamInput.bam.crai &&
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15 #end if
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17 @BINARY@
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18 @THREADS@
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19 --bamfile local_bamInput.bam
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20 --GCbiasFrequenciesFile $outFileName
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22 #if $fragmentLength != "":
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23 --fragmentLength $fragmentLength
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24 #end if
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26 @reference_genome_source@
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28 #if $effectiveGenomeSize.effectiveGenomeSize_opt == "specific":
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29 --effectiveGenomeSize $effectiveGenomeSize.effectiveGenomeSize
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30 #else:
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31 --effectiveGenomeSize $effectiveGenomeSize.effectiveGenomeSize_opt
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32 #end if
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34 #if str($region).strip() != '':
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35 --region '$region'
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36 #end if
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38 #if $advancedOpt.showAdvancedOpt == "yes":
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39 --sampleSize '$advancedOpt.sampleSize'
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40 --regionSize '$advancedOpt.regionSize'
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42 #if $advancedOpt.extraSampling:
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43 --extraSampling $advancedOpt.extraSampling
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44 #end if
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46 @blacklist@
0
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47 #end if
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48
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49 #if str($image_format) != 'none':
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50 --biasPlot $outImageName
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51 --plotFileFormat $image_format
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52 #end if
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53 ]]>
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54 </command>
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55 <inputs>
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56 <param name="bamInput" format="bam,cram" type="data" label="BAM file"
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57 help=""/>
0
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58
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59 <expand macro="reference_genome_source" />
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60 <expand macro="effectiveGenomeSize" />
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61 <expand macro="fragmentLength" />
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62 <expand macro="region_limit_operation" />
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63
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64 <conditional name="advancedOpt">
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65 <param name="showAdvancedOpt" type="select" label="Show advanced options" >
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66 <option value="no" selected="true">no</option>
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67 <option value="yes">yes</option>
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68 </param>
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69 <when value="no" />
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70 <when value="yes">
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71 <param name="sampleSize" type="integer" value="50000000" min="1"
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72 label="Number of sampling points to consider" help="(--sampleSize)" />
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73 <param name="regionSize" type="integer" value="300" min="1"
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74 label="Region size"
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75 help ="To plot the reads per GC over a region, the size of the region is
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76 required (see below for more details about the method). By default, the bin size
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77 is set to 300 bases, which is close to the standard fragment size of many sequencing
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78 applications. However, if the depth of sequencing is low, a larger bin size will
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79 be required, otherwise many bins will not overlap with any read. (--regionSize)"/>
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80 <param name="extraSampling" type="data" format="bed" optional="true"
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81 label="BED file containing genomic regions for which extra sampling is required because they are underrepresented in the genome"
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82 help="(--extraSampling)" />
8
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83 <expand macro="blacklist" />
0
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84 </when>
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85 </conditional>
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86 <param name="image_format" type="select"
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87 label="GC bias plot"
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88 help="If given, a diagnostic image summarizing the GC bias found on the sample will be created. (--plotFileFormat)">
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89 <option value="none">No image</option>
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90 <option value="png" selected="true">Image in png format</option>
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91 <option value="pdf">Image in pdf format</option>
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92 <option value="svg">Image in svg format</option>
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93 <option value="eps">Image in eps format</option>
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94 <option value="plotly">HTML page rendered with plotly</option>
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95 </param>
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96 </inputs>
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97 <outputs>
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98 <data name="outFileName" format="tabular" />
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99 <data name="outImageName" format="png" label="${tool.name} GC-bias Plot">
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100 <filter>
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101 ((
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102 image_format != 'none'
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103 ))
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104 </filter>
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105 <change_format>
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106 <when input="image_format" value="pdf" format="pdf" />
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107 <when input="image_format" value="svg" format="svg" />
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108 <when input="image_format" value="eps" format="eps" />
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109 <when input="image_format" value="plotly" format="html" />
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110 </change_format>
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111 </data>
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112 </outputs>
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113 <tests>
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114 <test>
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115 <param name="bamInput" value="paired_chr2L.bam" ftype="bam" />
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116 <param name="image_format" value="png" />
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117 <param name="showAdvancedOpt" value="yes" />
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118 <param name="regionSize" value="1" />
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119 <param name="ref_source" value="history" />
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120 <param name="input1" value="sequence.2bit" />
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121 <param name="sampleSize" value="10" />
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122 <param name="effectiveGenomeSize_opt" value="specific" />
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123 <param name="effectiveGenomeSize" value="10050" />
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124 <param name="region" value="chr2L" />
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125 <param name="image_format" value="none" />
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126 <param name="fragmentLength" value="300" />
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127 <output name="outFileName" file="computeGCBias_result1.tabular" ftype="tabular" />
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128 </test>
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129 </tests>
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130 <help>
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131 <![CDATA[
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132 What it does
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133 ------------
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134
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135 This tool computes the GC bias using the method proposed in Benjamini and Speed (2012) Nucleic Acids Res. (see below for further details).
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136 The output is used to plot the results and can also be used later on to correct the bias with the tool ``correctGCbias``.
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137 There are two plots produced by the tool: a boxplot showing the absolute read numbers per GC-content bin and an x-y plot depicting the ratio of observed/expected reads per GC-content bin.
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138
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139 Output files
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140 ------------
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141
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142 - Diagnostic plots:
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143 - box plot of absolute read numbers per GC-content bin
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144 - x-y plot of observed/expected read ratios per GC-content bin
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145
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146 - Tabular file: to be used for GC correction with ``correctGCbias``
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147
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148 .. image:: $PATH_TO_IMAGES/computeGCBias_output.png
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149 :width: 600
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150 :height: 455
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151
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152 -----
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153
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154 Theoretical Background
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155 ----------------------
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156
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157 ``computeGCBias`` is based on a paper by `Benjamini and Speed <http://nar.oxfordjournals.org/content/40/10/e72>`_.
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158 The basic assumption of the GC bias diagnosis is that an ideal sample should show a uniform distribution of sequenced reads across the genome, i.e. all regions of the genome should have similar numbers of reads, regardless of their base-pair composition.
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159 In reality, the DNA polymerases used for PCR-based amplifications during the library preparation of the sequencing protocols prefer GC-rich regions. This will influence the outcome of the sequencing as there will be more reads for GC-rich regions just because of the DNA polymerase's preference.
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161 ``computeGCbias`` will first calculate the **expected GC profile** by counting the number of DNA fragments of a fixed size per GC fraction where GC fraction is defined as the number of G's or C's in a genome region of a given length.
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162 The result is basically a histogram depicting the frequency of DNA fragments for each type of genome region with a GC fraction between 0 to 100 percent. This will be different for each reference genome, but is independent of the actual sequencing experiment.
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163
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164 The profile of the expected DNA fragment distribution is then compared to the **observed GC profile**, which is generated by counting the number of sequenced reads per GC fraction.
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165
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166 In an ideal experiment, the observed GC profile would, of course, look like the expected profile.
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167 This is indeed the case when applying ``computeGCBias`` to simulated reads.
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168
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169 .. _computeGCBias_example_image:
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171 .. image:: $PATH_TO_IMAGES/GC_bias_simulated_reads_2L.png
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173 As you can see, both plots based on **simulated reads** do not show enrichments or depletions for specific GC content bins, there is an almost flat line around the log2ratio of 0 (= ratio(observed/expected) of 1). The fluctuations on the ends of the x axis are due to the fact that only very, very few regions in the *Drosophila* genome have such extreme GC fractions so that the number of fragments that are picked up in the random sampling can vary.
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175 Now, let's have a look at **real-life data** from genomic DNA sequencing. Panels A and B can be clearly distinguished and the major change that took place between the experiments underlying the plots was that the samples in panel A were prepared with too many PCR cycles and a standard polymerase whereas the samples of panel B were subjected to very few rounds of amplification using a high fidelity DNA polymerase.
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176
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177 .. image:: $PATH_TO_IMAGES/QC_GCplots_input.png
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178 :width: 600
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179 :height: 452
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181 **Note:** The expected GC profile depends on the reference genome as different organisms have very different GC contents. For example, one would expect more fragments with GC fractions between 30% to 60% in mouse samples (average GC content of the mouse genome: 45 %) than for genome fragments from, for example, *Plasmodium falciparum* (average genome GC content *P. falciparum*: 20%).
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183 For more details, for example about when to exclude regions from the read distribution calculation, go `here <http://deeptools.readthedocs.org/en/latest/content/tools/computeGCBias.html#excluding-regions-from-the-read-distribution-calculation>`_
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186 -----
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188 @REFERENCES@
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189 ]]>
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190 </help>
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191 <expand macro="citations" />
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192 </tool>