comparison picard_ReorderSam.xml @ 0:1cd7f3b42609

Uploaded tool.
author devteam
date Tue, 23 Oct 2012 13:14:29 -0400
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children 9227b8c3093b
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-1:000000000000 0:1cd7f3b42609
1 <tool name="Reorder SAM/BAM" id="picard_ReorderSam" version="1.56.0">
2 <requirements><requirement type="package" version="1.56.0">picard</requirement></requirements>
3 <command interpreter="python">
4 picard_wrapper.py
5 --input=$inputFile
6 #if $source.indexSource == "built-in"
7 --ref="${source.ref.fields.path}"
8 #else
9 --ref-file=$refFile
10 --species-name=$source.speciesName
11 --build-name=$source.buildName
12 --trunc-names=$source.truncateSeqNames
13 #end if
14 --allow-inc-dict-concord=$allowIncDictConcord
15 --allow-contig-len-discord=$allowContigLenDiscord
16 --output-format=$outputFormat
17 --output=$outFile
18 --tmpdir "${__new_file_path__}"
19 -j "\$JAVA_JAR_PATH/ReorderSam.jar"
20 </command>
21 <inputs>
22 <param format="bam,sam" name="inputFile" type="data" label="SAM/BAM dataset to be reordered"
23 help="If empty, upload or import a SAM/BAM dataset." />
24 <conditional name="source">
25 <param name="indexSource" type="select" label="Select Reference Genome" help="This tool will re-order SAM/BAM in the same order as reference selected below.">
26 <option value="built-in">Locally cached</option>
27 <option value="history">History</option>
28 </param>
29 <when value="built-in">
30 <param name="ref" type="select" label="Select a reference genome">
31 <options from_data_table="picard_indexes" />
32 </param>
33 </when>
34 <when value="history">
35 <param name="refFile" type="data" format="fasta" metadata_name="dbkey" label="Using reference file" />
36 <param name="speciesName" type="text" value="" label="Species name" />
37 <param name="buildName" type="text" value="" label="Build name" />
38 <param name="truncateSeqNames" type="boolean" checked="False" truevalue="true" falsevalue="false" label="Truncate sequence names after first whitespace" />
39 </when>
40 </conditional>
41 <param name="allowIncDictConcord" type="boolean" checked="False" truevalue="true" falsevalue="false" label="Allow incomplete dict concordance?" help="Allows a partial overlap of the BAM contigs with the new reference sequence contigs." />
42 <param name="allowContigLenDiscord" type="boolean" checked="False" truevalue="true" falsevalue="false" label="Allow contig length discordance?" help="This is dangerous--don't check it unless you know exactly what you're doing!" />
43 <param name="outputFormat" type="boolean" checked="True" truevalue="bam" falsevalue="sam" label="Output BAM instead of SAM" help="Uncheck for SAM output" />
44 </inputs>
45 <outputs>
46 <data name="outFile" format="bam" label="${tool.name} on ${on_string}: reordered ${outputFormat}">
47 <change_format>
48 <when input="outputFormat" value="sam" format="sam" />
49 </change_format>
50 </data>
51 </outputs>
52 <tests>
53 <test>
54 <!-- Commands:
55 cp test-data/phiX.fasta .
56 samtools faidx phiX.fasta
57 java -jar CreateSequenceDictionary.jar R=phiX.fasta O=phiX.dict URI=phiX.fasta TRUNCATE_NAMES_AT_WHITESPACE=false SPECIES=phiX174
58 java -jar ReorderSam.jar VALIDATION_STRINGENCY=LENIENT I=test-data/picard_RS_input1.bam O=picard_RS_output1.bam REFERENCE=phiX.fasta ALLOW_INCOMPLETE_DICT_CONCORDANCE=false ALLOW_CONTIG_LENGTH_DISCORDANCE=false
59 -->
60 <param name="inputFile" value="picard_RS_input1.bam" />
61 <param name="indexSource" value="history" />
62 <param name="refFile" value="phiX.fasta" />
63 <param name="speciesName" value="phiX174" />
64 <param name="buildName" value="" />
65 <param name="truncateSeqNames" value="false" />
66 <param name="allowIncDictConcord" value="false" />
67 <param name="allowContigLenDiscord" value="false" />
68 <param name="outputFormat" value="True" />
69 <output name="outFile" file="picard_RS_output1.bam" ftype="bam" lines_diff="4" compare="contains" />
70 </test>
71 <test>
72 <!-- Command:
73 java -jar ReorderSam.jar VALIDATION_STRINGENCY=LENIENT I=test-data/picard_RS_input2.sam O=picard_RS_output2.sam REFERENCE=/path/to/phiX/picard_index/phiX.fa ALLOW_INCOMPLETE_DICT_CONCORDANCE=false ALLOW_CONTIG_LENGTH_DISCORDANCE=false
74 /path/to/phiX/srma_index/phiX.fa is path to phiX.fa, phiX.fa.fai, and phiX.dict
75 -->
76 <param name="inputFile" value="picard_RS_input2.sam" />
77 <param name="indexSource" value="built-in" />
78 <param name="ref" value="phiX" />
79 <param name="allowIncDictConcord" value="false" />
80 <param name="allowContigLenDiscord" value="false" />
81 <param name="outputFormat" value="False" />
82 <output name="outFile" file="picard_RS_output2.sam" ftype="sam" lines_diff="4" sort="True" />
83 </test>
84 <test>
85 <!-- Commands:
86 cp test-data/picard_RS_input4.fasta .
87 samtools faidx picard_RS_input4.fasta
88 java -jar CreateSequenceDictionary.jar R=picard_RS_input4.fasta O=picard_RS_input4.dict URI=picard_RS_input4.fasta TRUNCATE_NAMES_AT_WHITESPACE=true SPECIES=phiX174 GENOME_ASSEMBLY=phiX_buildBlah1.1
89 java -jar ReorderSam.jar VALIDATION_STRINGENCY=LENIENT I=test-data/picard_RS_input3.bam O=picard_RS_output3.sam REFERENCE=picard_RS_input4.fasta ALLOW_INCOMPLETE_DICT_CONCORDANCE=true ALLOW_CONTIG_LENGTH_DISCORDANCE=false
90 picard_RS_input3.bam can be made from picard_RS_input3.sam
91 -->
92 <param name="inputFile" value="picard_RS_input3.bam" />
93 <param name="indexSource" value="history" />
94 <param name="refFile" value="picard_RS_input4.fasta" />
95 <param name="speciesName" value="phiX174" />
96 <param name="buildName" value="phiX_buildBlah1.1" />
97 <param name="truncateSeqNames" value="true" />
98 <param name="allowIncDictConcord" value="true" />
99 <param name="allowContigLenDiscord" value="false" />
100 <param name="outputFormat" value="False" />
101 <output name="outFile" file="picard_RS_output3.sam" ftype="sam" lines_diff="12" sort="True" />
102 </test>
103 </tests>
104 <help>
105
106 .. class:: infomark
107
108 **Purpose**
109
110 Reorder SAM/BAM to match contig ordering in a particular reference file. Note that this is
111 not the same as sorting as done by the SortSam tool, which sorts by either coordinate
112 values or query name. The ordering in ReorderSam is based on exact name matching of
113 contigs/chromosomes. Reads that are mapped to a contig that is not in the new reference file are
114 not included in the output.
115
116 **Picard documentation**
117
118 This is a Galaxy wrapper for ReorderSam, a part of the external package Picard-tools_.
119
120 .. _Picard-tools: http://www.google.com/search?q=picard+samtools
121
122 ------
123
124 .. class:: infomark
125
126 **Inputs, outputs, and parameters**
127
128 For the file that needs to be reordered, either a sam file or a bam file must be supplied.
129 If a bam file is used, it must be coordinate-sorted. A reference file is also required,
130 so either a fasta file should be supplied or a built-in reference can be selected.
131
132 The output contains the same reads as the input file but the reads have been rearranged so
133 they appear in the same order as the provided reference file. The tool will output either
134 bam (the default) or sam, according to user selection. Bam is recommended since it is smaller.
135
136 The only extra parameters that can be set are flags for allowing incomplete dict concordance
137 and allowing contig length discordance. If incomplete dict concordance is allowed, only a
138 partial overlap of the bam contigs with the new reference sequence contigs is required. By
139 default it is off, requiring a corresponding contig in the new reference for each read contig.
140 If contig length discordance is allowed, contig names that are the same between a read and the
141 new reference contig are allowed even if they have different lengths. This is usually not a
142 good idea, unless you know exactly what you're doing. It's off by default.
143
144 .. class:: warningmark
145
146 **Warning on SAM/BAM quality**
147
148 Many SAM/BAM files produced externally and uploaded to Galaxy do not fully conform to SAM/BAM specifications. Galaxy deals with this by using the **LENIENT**
149 flag when it runs Picard, which allows reads to be discarded if they're empty or don't map. This appears
150 to be the only way to deal with SAM/BAM that cannot be parsed.
151
152
153 </help>
154 </tool>
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