annotate repex_tarean.xml @ 3:c0ae68651c11 draft

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author petr-novak
date Mon, 06 Jan 2020 04:00:31 -0500
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1 <tool id="tareanx" name="Tandem Repeat Analyzer" version="2.3.6" >
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2 <stdio>
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3 <regex match="Traceback" source="stderr" level="fatal" description="Unknown error" />
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4 <regex match="error" source="stderr" level="fatal" description="Unknown error" />
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5 <regex match="warning" source="stderr" level="warning" description="Unknown warning" />
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6 <exit_code range="1:" level="fatal" description="Error" />
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7 </stdio>
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8 <description>Identification of genomic tandem repeats from NGS data</description>
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9 <requirements>
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10 <requirement type="package" version="3.7">python</requirement>
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11 <requirement type="package" version="0.9.1" >pyrserve</requirement>
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12 <requirement type="package">last</requirement>
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13 <requirement type="package">mafft</requirement>
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14 <requirement type="package">imagemagick</requirement>
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15 <requirement type="package">blast</requirement>
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16 <requirement type="package">diamond</requirement>
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17 <requirement type="package">blast-legacy</requirement>
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18 <requirement type="package">r-igraph</requirement>
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19 <requirement type="package">r-data.tree</requirement>
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20 <requirement type="package">r-stringr</requirement>
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21 <requirement type="package">r-r2html</requirement>
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22 <requirement type="package">r-hwriter</requirement>
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23 <requirement type="package">r-dt</requirement>
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24 <requirement type="package">r-scales</requirement>
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25 <requirement type="package">r-plotrix</requirement>
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26 <requirement type="package">r-png</requirement>
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27 <requirement type="package">r-plyr</requirement>
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28 <requirement type="package">r-dplyr</requirement>
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29 <requirement type="package">r-optparse</requirement>
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30 <requirement type="package">r-dbi</requirement>
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31 <requirement type="package">r-rsqlite</requirement>
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32 <requirement type="package">r-rserve</requirement>
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33 <requirement type="package">bioconductor-biostrings</requirement>
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34 <requirement type="package" version="1.0">repex_tarean</requirement>
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35 <requirement type="set_environment">REPEX</requirement>
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36 </requirements>
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37 <command detect_errors="exit_code">
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38 export PYTHONHASHSEED=0;
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39 \${REPEX}/seqclust --paired --sample ${sample} --output_dir=tarean_output --logfile=${log} --cleanup --tarean_mode
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40 #if $advanced_options.advanced:
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41 --mincl $advanced_options.size_threshold $advanced_options.keep_names $advanced_options.automatic_filtering -M $advanced_options.merging
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42 #if $advanced_options.custom_library.options_custom_library :
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43 -d $advanced_options.custom_library.library extra_database
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44 #end if
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45 #if $advanced_options.options.options:
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46 -opt $advanced_options.options.options
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47 #end if
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48 #else:
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49 -M 0.2
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50
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51 #end if
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52 ${FastaFile} >stdout.log 2> stderr.log ;
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53 echo "STDOUT CONTENT:" >> ${log} ;
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54 cat stdout.log >> ${log} ;
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55 echo "STDERR CONTENT:" >> ${log} ;
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56 cat stderr.log >> ${log} &amp;&amp;
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57 ${__tool_directory__}/stderr_filter.py stderr.log &amp;&amp;
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58 cd tarean_output &amp;&amp;
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59 zip -r ${ReportArchive}.zip * &amp;&amp;
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60 mv ${ReportArchive}.zip ${ReportArchive} &amp;&amp;
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61 cp index.html ${ReportFile} &amp;&amp;
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62 mkdir ${ReportFile.files_path} &amp;&amp;
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63 cp -r --parents libdir ${ReportFile.files_path} &amp;&amp;
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64 cp -r --parents seqclust/clustering/superclusters ${ReportFile.files_path} &amp;&amp;
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65 cp -r --parents seqclust/clustering/clusters ${ReportFile.files_path} &amp;&amp;
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66 cp seqclust/clustering/hitsort.cls ${ReportFile.files_path}/seqclust/clustering/hitsort.cls &amp;&amp;
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67 cp *.png ${ReportFile.files_path}/ &amp;&amp;
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68 cp *.csv ${ReportFile.files_path}/ &amp;&amp;
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69 cp *.html ${ReportFile.files_path}/ &amp;&amp;
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70 cp *.css ${ReportFile.files_path}/ &amp;&amp;
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71 cp *.fasta ${ReportFile.files_path}/ 2>>$log &amp;&amp; rm -r ../tarean_output || :
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72
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73
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74 </command>
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75
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76 <inputs>
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77 <param name="FastaFile" label="paired-end NGS reads" type="data" format="fasta"
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78 help="Input file must contain fasta-formatted interlaced read pairs from paired-end sequencing. All pairs must be complete. Example of input data format is provided in the help below."/>
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79 <param name="sample" label="Sample size" type="integer" value="500000" min="10000"/>
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80
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81 <conditional name="advanced_options">
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82 <param name="advanced" type="boolean" truevalue="true" falsevalue="false" checked="False" label="Advanced options" />
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83 <when value="false">
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84 <!-- pass -->
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85 </when>
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86 <when value="true">
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87 <param name="merging" type="boolean" truevalue="0.2" falsevalue="0" checked="True" label="Perform cluster merging" help="By default, clusters connected through paired-end reads are merged"/>
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88 <conditional name="custom_library">
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89 <param name="options_custom_library" type="boolean" truevalue="true" falsevalue="false" checked="False" label="Use custom repeat database"/>
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90 <when value="false">
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91 <!-- do nothing here -->
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92 </when>
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93 <when value="true">
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94 <param name="library" format="fasta" type="data" label="Use custom repeat database" help="Perform additional similarity search to user-provided repeat database. The database should contain FASTA-formatted DNA sequences with headers (sequence names) in the format: '>reapeatname#class/subclass'"/>
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95 </when>
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96 </conditional>
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97 <param name="size_threshold" label="Cluster size threshold for detailed analysis" type="float" value="0.01" min="0.0001" max="100" help ="Minimal size (as percentage of input reads) of the smallest cluster which is analyzed, cluster with less than 20 reads are not considered at all."/>
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98 <param name="automatic_filtering" label="Perform automatic filtering of abundant satellite repeats" type="boolean" truevalue="--automatic_filtering" falsevalue="" checked="false"/>
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99 <param name="keep_names" label="Keep original sequences names" type="boolean" truevalue="--keep_names" falsevalue="" checked="false" help="By default sequence are relabeled using integers. If you want to keep original names, use this option."/>
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100 <conditional name="options">
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101 <param name="options" type="select" label="Similarity search options" help="Different similarity search parameters are used depending on the used input data to adjust search to differences in length and error rate">
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102 <option value="ILLUMINA" selected="true">Illumina reads, read length 100nt or more </option>
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103 <option value="ILLUMINA_SHORT" selected="false">Illumina reads, shorter than 100nt (Do not use reads shorter than 50nt!) </option>
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104 <option value="ILLUMINA_DUST_OFF" selected="false">Illumina reads, no masking of low complexity repeats </option>
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105 </param>
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106 </conditional>
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107 </when>
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108 </conditional>
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109
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110 </inputs>
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111 <outputs>
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112 <data name="log" format="txt" label="TAREAN log file"/>
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113 <data name="ReportArchive" format="zip" label="TAREAN Archive with HTML report from data ${FastaFile.hid}"/>
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114 <data name="ReportFile" format="html" label="TAREAN HTML report from data ${FastaFile.hid}"/>
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115 </outputs>
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116
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117 <help>
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118 **HELP**
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119
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120 TAREAN - TAndem REpeat ANalyzer is a computational pipeline for
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121 **unsupervised identification of satellite repeats** from unassembled
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122 sequence reads. The pipeline uses low-pass paired-end whole genome
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123 sequence reads and performs graph-based clustering. The resulting
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124 clusters, representing all types of repeats present in the genome, are
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125 then examined to identify those containing circular structures indicative
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126 of tandem repeats. A poster summarizing TAREAN principles and
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127 implementation can be found `here.`__
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128
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129
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130 .. __: http://w3lamc.umbr.cas.cz/lamc/?page_id=312
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131
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132 **Input data**
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133
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134
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135 The analysis requires **paired-end reads** generated by whole genome
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136 shotgun sequencing. The data should be provided as a single input file in
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137 fasta format with the reads interlaced (see example below). All the pairs
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138 must be complete, i.e. both "forward" and "reverse" sequence reads must be
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139 present. The reads should all be trimmed to the same length. The optimal
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140 size range is between 100 and 200 nucleotides. The number of reads to be
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141 analyzed should not exceed 1x coverage of the genome. Genome coverage
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142 between 0.01 and 0.5x is recommended. The reads should be filtered for
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143 quality. The recommended quality filtering is as follows: each read should
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144 have a quality score >=10 for 95% of the bases, i.e. if your reads are 100
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145 base pairs long, then a read only passes this quality threshold if 95
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146 bases have a quality of 10 or higher. Additionally, any reads containing
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147 indeterminate base pairs (indicated as N in the reads) should be removed.
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148 Finally, if either one of the reads in a pair fails to meet the
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149 aforementioned thresholds, **both** sequences should be removed.
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150 example of interlaced input format::
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151
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152 >0001_f
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153 CGTAATATACATACTTGCTAGCTAGTTGGATGCATCCAACTTGCAAGCTAGTTTGATG
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154 >0001_r
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155 GATTTGACGGACACACTAACTAGCTAGTTGCATCTAAGCGGGCACACTAACTAACTAT
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156 >0002_f
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157 ACTCATTTGGACTTAACTTTGATAATAAAAACTTAAAAAGGTTTCTGCACATGAATCG
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158 >0002_r
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159 TATGTTGAAAAATTGAATTTCGGGACGAAACAGCGTCTATCGTCACGACATAGTGCTC
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160 >0003_f
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161 TGACATTTGTGAACGTTAATGTTCAACAAATCTTTCCAATGTCTTTTTATCTTATCAT
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162 >0003_r
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163 TATTGAAATACTGGACACAAATTGGAAATGAAACCTTGTGAGTTATTCAATTTATGTT
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164 ...
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165
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166
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167 To perform the quality filtering on your fastQ formatted data as described
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168 above, and to interlace your paired-end sequence reads,
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169 please use the `Preprocessing of paired-reads`__ tool.
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170
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171 .. __: tool_runner?tool_id=paired_fastq_filtering
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172
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173
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174 **Additional parameters**
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175
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176 **Sample size** defines how many reads will be used during the computation.
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177 The default setting of 500,000 reads will enable detection of high copy
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178 number satellites within several hours. For higher
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179 sensitivity the sample size can be increased. Since the sample size affects
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180 memory usage, this parameter may be automatically adjusted to a lower value
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181 during the run. The maximum sample size which can be processed depends on the
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182 repetitiveness of the analyzed genome. This significantly limits the number of reads
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183 that can be analyzed with the TAREAN pipeline.
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184
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185 **Perform cluster merging**. Families of repetitive elements are
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186 frequently split into multiple clusters rather than being represented as a
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187 single one. If you do not want to merge clusters based on the presence
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188 of broken read pairs, disable this option.
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189
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190 **Use custom repeat database**. This option allows users to perform similarity
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191 comparison of identified repeats to their custom databases. The repeat class should
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192 be encoded in FASTA headers of database entries in order to allow correct
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193 parsing of similarity hits.
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194
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195 **Similarity search options** By default sequence reads are compared using
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196 mgblast program. Default threshold is explicitly set to 90% sequence
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197 similarity spanning at least 55% of the read length (in the case of reads
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198 differing in length it applies to the longer one). Additionally, sequence
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199 overlap must be at least 55 nt. If you select option for shorter reads
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200 than 100 nt, minimum overlap 55 nt is not required.
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201
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202 By default,
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203 mgblast search use DUST program to filter out
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204 low-complexity sequences. If you want
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205 to increase sensitivity of detection of satellites with shorter monomer
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206 use option with '*no masking of low complexity repeats*'. Note that omitting
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207 DUST filtering will significantly increase running times
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208
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209 **Output**
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210
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211 A list of clusters identified as putative satellite repeats, their genomic
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212 abundance and various cluster characteristics are provided. Length and
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213 consensus sequences of reconstructed monomers are also shown and
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214 accompanied by a detailed output from kmer-based reconstruction including
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215 sequences and sequence logos of alternative variants of monomer sequences.
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216
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217 The output includes an **HTML summary** with a table listing all analyzed
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218 clusters. More detailed information about clusters is provided in
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219 additional files and directories. All results are also provided as a
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220 downloadable **zip archive**. Since read clustering results in
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221 thousands of clusters, the search for satellite repeats is limited to
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222 a subset of the largest ones corresponding to the most abundant genomic
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223 repeats. The default setting of the pipeline is to analyze all clusters containing at least
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224 0.01% of the input reads. Besides the satellite repeats, three other
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225 groups of clusters are reported in the output (1) LTR-retrotransposons,
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226 (2) 45S and 5S rDNA and (3) all remaining clusters passing the size
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227 threshold. As (1) and (2) contain sequences with circular
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228 graphs, their consensus is calculated in the same way as for satellite
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229 repeats. Additionally a **log file** reporting the progress of the
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230 computational pipeline is provided.
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231
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232
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233 </help>
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234
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235 </tool>