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1 <?xml version="1.0"?>
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2 <tool name="BloomTree Manager - Create" id="btman_create" version="1.0.0">
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3 <description>a Sequence Bloom Tree</description>
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4 <macros>
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5 <import>macros.xml</import>
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6 </macros>
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7 <expand macro="requirements" />
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8 <command detect_errors="exit_code">
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9 <![CDATA[
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10 python '$__tool_directory__/create.py'
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11
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12 --explist '${explist}'
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13
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14 --qualitycontrol ${conditional_quality.quality_control}
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15 #if $conditional_quality.quality_control == '0':
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16 --qualitythreshold 0.0
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17 #elif $conditional_quality.quality_control == '1':
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18 --qualitythreshold ${conditional_quality.quality_threshold}
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19 #end if
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20
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21 --klen ${kmer_len}
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22 --minabundance ${min_abundance}
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23
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24 --outfile '${outfile}'
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25 ]]>
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26 </command>
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27 <inputs>
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28 <param format="tabular" name="explist" type="data" label="Select a file with the list of experiments" help="This should be a tabular file with two columns. Take a look at the tool documentation for a detailed explanation about the its content." />
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29
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30 <conditional name="conditional_quality">
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31 <param name="quality_control" type="boolean" checked="false" truevalue="1" falsevalue="0" label="Apply a quality control procedure" />
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32 <when value="1">
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33 <param name="quality_threshold" size="1" type="float" value="0.8" min="0.0" max="1.0" label="Quality threshold" help="If the number of sequences flagged as poor quality on the total number of sequences in a file is less than this threshold, the sequence file will be excluded." />
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34 </when>
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35 </conditional>
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36
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37 <param name="kmer_len" type="integer" value="21" min="0" label="K-mer length" />
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38 <param name="min_abundance" type="integer" value="2" min="0" label="Bloom filter minimum abundance" help="This value is the minimum abundance cutoff for the creation of the Bloom filters. It is worth noting that the same minimum abundance is used for each Bloom filter." />
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39 </inputs>
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40 <outputs>
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41 <data format="txt" name="outfile" label="${tool.name} SBT: Result" from_work_dir="btman.create.txt" />
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42 </outputs>
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43
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44 <help><![CDATA[
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45 This tool is part of the BloomTree Manager Framework that allow to create a Sequence Bloom Tree starting
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46 with a set of FASTA or FASTQ files. It allows also to control the quality of the input dataset and
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47 exclude the files that do not reach a specified quality level.
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48
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49 -----
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50
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51 **Input file**
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52
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53 The input file for this tool must contain two columns with their values delimited by a tab.
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54 The first column contains a list of SRA accessions, and the second column contains a unique identifier
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55 for each set of SRA accessions.
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56
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57 The input file is structured like the example below::
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58
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59 SRR805782 blood
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60 SRR837459 blood
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61 SRR837458 blood
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62 SRR837453 blood
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63 SRR837456 blood
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64 ...
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65 SRR791048 breast
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66 SRR553483 breast
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67 SRR553482 breast
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68 SRR791045 breast
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69 ...
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70 SRR950876 brain
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71 SRR786621 brain
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72
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73 It is worth noting that for each cluster of accessions, every accession should be unique.
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74 It is indeed possible to repeat an accession in multiple clusters.
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75
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76 The tool will create a Sequence Bloom Tree for each cluster of accessions.
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77
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78 -----
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79
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80 **Output**
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81
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82 The tool returns a single text file only. It contains the a tree identifier, one for
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83 each cluster of accessions specified in the input file, that can be used with the
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84 Query tool of the BloomTree Manager Suite to search for the presence of a set of
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85 specific transcripts.
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86
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87 Take a look at the Query tool documentation for a detailed description about how
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88 to query a Sequence Bloom Tree.
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89
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90 -----
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91
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92 .. class:: infomark
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93
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94 **Notes**
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95
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96 This Galaxy tool has been developed by Fabio Cumbo.
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97
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98 Please visit this GithHub_repository_ for more information about the BloomTree Manager
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99
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100 .. _GithHub_repository: https://github.com/fabio-cumbo/bloomtree-manager
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101 ]]></help>
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102
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103 <expand macro="citations" />
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104 </tool>
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