Mercurial > repos > peterjc > fastq_paired_unpaired
annotate tools/fastq/fastq_paired_unpaired.xml @ 3:528ba9c896e0 draft
Uploaded v0.0.8, MIT licence and reST for README, citation information, development moved to GitHub
author | peterjc |
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date | Wed, 18 Sep 2013 06:13:27 -0400 |
parents | 95a632a71951 |
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1 <tool id="fastq_paired_unpaired" name="Divide FASTQ file into paired and unpaired reads" version="0.0.7"> |
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2 <description>using the read name suffices</description> |
2 | 3 <version_command interpreter="python">fastq_paired_unpaired.py --version</version_command> |
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4 <command interpreter="python"> |
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5 fastq_paired_unpaired.py $input_fastq.extension $input_fastq |
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6 #if $output_choice_cond.output_choice=="separate" |
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7 $output_forward $output_reverse |
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8 #elif $output_choice_cond.output_choice=="interleaved" |
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9 $output_paired |
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10 #end if |
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11 $output_singles |
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12 </command> |
2 | 13 <stdio> |
14 <!-- Anything other than zero is an error --> | |
15 <exit_code range="1:" /> | |
16 <exit_code range=":-1" /> | |
17 </stdio> | |
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18 <inputs> |
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19 <param name="input_fastq" type="data" format="fastq" label="FASTQ file to divide into paired and unpaired reads"/> |
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20 <conditional name="output_choice_cond"> |
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21 <param name="output_choice" type="select" label="How to output paired reads?"> |
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22 <option value="separate">Separate (two FASTQ files, for the forward and reverse reads, in matching order).</option> |
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23 <option value="interleaved">Interleaved (one FASTQ file, alternating forward read then partner reverse read).</option> |
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24 </param> |
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25 <!-- Seems need these dummy entries here, compare this to indels/indel_sam2interval.xml --> |
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26 <when value="separate" /> |
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27 <when value="interleaved" /> |
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28 </conditional> |
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29 </inputs> |
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30 <outputs> |
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31 <data name="output_singles" format="input" label="Orphan or single reads"/> |
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32 <data name="output_forward" format="input" label="Forward paired reads"> |
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33 <filter>output_choice_cond["output_choice"] == "separate"</filter> |
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34 </data> |
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35 <data name="output_reverse" format="input" label="Reverse paired reads"> |
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36 <filter>output_choice_cond["output_choice"] == "separate"</filter> |
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37 </data> |
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38 <data name="output_paired" format="input" label="Interleaved paired reads"> |
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39 <filter>output_choice_cond["output_choice"] == "interleaved"</filter> |
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40 </data> |
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41 </outputs> |
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42 <tests> |
2 | 43 <test> |
44 <param name="input_fastq" value="sanger-pairs-mixed.fastq" ftype="fastq"/> | |
45 <param name="output_choice" value="separate"/> | |
46 <output name="output_singles" file="sanger-pairs-singles.fastq" ftype="fastq"/> | |
47 <output name="output_forward" file="sanger-pairs-forward.fastq" ftype="fastq"/> | |
48 <output name="output_reverse" file="sanger-pairs-reverse.fastq" ftype="fastq"/> | |
49 </test> | |
50 <test> | |
51 <param name="input_fastq" value="sanger-pairs-mixed.fastq" ftype="fastq"/> | |
52 <param name="output_choice" value="interleaved"/> | |
53 <output name="output_singles" file="sanger-pairs-singles.fastq" ftype="fastq"/> | |
54 <output name="output_paired" file="sanger-pairs-interleaved.fastq" ftype="fastq"/> | |
55 </test> | |
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56 </tests> |
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57 <help> |
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58 |
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59 **What it does** |
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60 |
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61 Using the common read name suffix conventions, it divides a FASTQ file into |
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62 paired reads, and orphan or single reads. |
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63 |
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64 The input file should be a valid FASTQ file which has been sorted so that |
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65 any partner forward+reverse reads are consecutive. The output files all |
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66 preserve this sort order. Pairing are recognised based on standard name |
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67 suffices. See below or run the tool with no arguments for more details. |
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68 |
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69 Any reads where the forward/reverse naming suffix used is not recognised |
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70 are treated as orphan reads. The tool supports the /1 and /2 convention |
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71 originally used by Illumina, .f and .r convention, the Sanger convention |
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72 (see http://staden.sourceforge.net/manual/pregap4_unix_50.html for details), |
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73 and the current Illumina convention where the reads get the same identifier |
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74 with the fragment number in the description, for example: |
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75 |
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76 * @HWI-ST916:79:D04M5ACXX:1:1101:10000:100326 1:N:0:TGNCCA |
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77 * @HWI-ST916:79:D04M5ACXX:1:1101:10000:100326 2:N:0:TGNCCA |
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78 |
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79 Note that this does support multiple forward and reverse reads per template |
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80 (which is quite common with Sanger sequencing), e.g. this which is sorted |
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81 alphabetically: |
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82 |
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83 * WTSI_1055_4p17.p1kapIBF |
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84 * WTSI_1055_4p17.p1kpIBF |
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85 * WTSI_1055_4p17.q1kapIBR |
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86 * WTSI_1055_4p17.q1kpIBR |
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87 |
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88 or this where the reads already come in pairs: |
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89 |
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90 * WTSI_1055_4p17.p1kapIBF |
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91 * WTSI_1055_4p17.q1kapIBR |
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92 * WTSI_1055_4p17.p1kpIBF |
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93 * WTSI_1055_4p17.q1kpIBR |
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94 |
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95 both become: |
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96 |
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97 * WTSI_1055_4p17.p1kapIBF paired with WTSI_1055_4p17.q1kapIBR |
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98 * WTSI_1055_4p17.p1kpIBF paired with WTSI_1055_4p17.q1kpIBR |
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99 |
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100 **References** |
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101 |
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102 If you use this Galaxy tool in work leading to a scientific publication please |
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103 cite the following paper: |
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104 |
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105 Peter J.A. Cock, Björn A. Grüning, Konrad Paszkiewicz and Leighton Pritchard (2013). |
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106 Galaxy tools and workflows for sequence analysis with applications |
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107 in molecular plant pathology. PeerJ 1:e167 |
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108 http://dx.doi.org/10.7717/peerj.167 |
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109 |
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110 This tool is available to install into other Galaxy Instances via the Galaxy |
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111 Tool Shed at http://toolshed.g2.bx.psu.edu/view/peterjc/fastq_paired_unpaired |
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112 </help> |
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113 </tool> |