Mercurial > repos > devteam > picard
annotate picard_SamToFastq.xml @ 8:3a3234d7a2e8 draft
planemo upload for repository https://github.com/galaxyproject/tools-devteam/tree/master/tools/picard commit 00a7926c285bc4a339bd7deebf40b28f39c7d947-dirty
author | devteam |
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date | Thu, 16 Jul 2015 15:53:10 -0400 |
parents | 3d4f1fa26f0e |
children | 5eaa8a968300 |
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8
3a3234d7a2e8
planemo upload for repository https://github.com/galaxyproject/tools-devteam/tree/master/tools/picard commit 00a7926c285bc4a339bd7deebf40b28f39c7d947-dirty
devteam
parents:
5
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changeset
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1 <tool name="SamToFastq" id="picard_SamToFastq" version="@TOOL_VERSION@.0"> |
5 | 2 <description>extract reads and qualities from SAM/BAM dataset and convert to fastq</description> |
3 <macros> | |
4 <import>picard_macros.xml</import> | |
5 </macros> | |
8
3a3234d7a2e8
planemo upload for repository https://github.com/galaxyproject/tools-devteam/tree/master/tools/picard commit 00a7926c285bc4a339bd7deebf40b28f39c7d947-dirty
devteam
parents:
5
diff
changeset
|
6 <expand macro="requirements" /> |
5 | 7 <command> |
8 | |
9 echo "BAM" > $report && ## This is necessary for output dataset detection (see output tags below) | |
10 | |
11 @java_options@ | |
12 | |
13 java -jar \$JAVA_JAR_PATH/picard.jar | |
14 SamToFastq | |
15 | |
16 INPUT="${inputFile}" | |
17 | |
18 #if str( $output_per_rg ) == "true": | |
19 OUTPUT_PER_RG=true | |
20 OUTPUT_DIR=. | |
21 #elif str( $output_per_rg ) == "false" and str( $interleave ) == "false": | |
22 FASTQ=READ1.fastq | |
23 SECOND_END_FASTQ=READ2.fastq | |
24 UNPAIRED_FASTQ=UNPAIRED_READS.fastq | |
25 #elif str( $output_per_rg ) == "false" and str( $interleave ) == "true": | |
26 FASTQ=INTERLEAVED.fastq | |
27 #end if | |
28 | |
2
9227b8c3093b
Updated command line format per dev team standards.
devteam <devteam@galaxyproject.org>
parents:
0
diff
changeset
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29 RE_REVERSE="${re_reverse}" |
5 | 30 INTERLEAVE="${interleave}" |
2
9227b8c3093b
Updated command line format per dev team standards.
devteam <devteam@galaxyproject.org>
parents:
0
diff
changeset
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31 INCLUDE_NON_PF_READS="${include_non_pf_reads}" |
5 | 32 CLIPPING_ATTRIBUTE="${clipping_attribute}" |
33 CLIPPING_ACTION="${clipping_action}" | |
34 READ1_TRIM="${read1_trim}" | |
35 | |
36 #if int($read1_max_bases_to_write) > -1: | |
37 READ1_MAX_BASES_TO_WRITE="${read1_max_bases_to_write}" | |
0 | 38 #end if |
5 | 39 |
40 READ2_TRIM="${read2_trim}" | |
41 | |
42 #if int($read2_max_bases_to_write) > -1: | |
43 READ2_MAX_BASES_TO_WRITE="${read2_max_bases_to_write}" | |
0 | 44 #end if |
5 | 45 |
2
9227b8c3093b
Updated command line format per dev team standards.
devteam <devteam@galaxyproject.org>
parents:
0
diff
changeset
|
46 INCLUDE_NON_PRIMARY_ALIGNMENTS="${include_non_primary_alignments}" |
0 | 47 |
5 | 48 |
49 VALIDATION_STRINGENCY="${validation_stringency}" | |
50 QUIET=true | |
51 VERBOSITY=ERROR | |
52 | |
0 | 53 </command> |
54 <inputs> | |
55 | |
5 | 56 <param format="sam,bam" name="inputFile" type="data" label="Select SAM/BAM dataset or dataset collection" help="If empty, upload or import a SAM/BAM dataset"/> |
57 <param name="output_per_rg" type="boolean" checked="False" label="Do you want to output a fastq file per read group (two fastq files per read group if the group is paired)" help="OUTPUT_PER_RG; default=False"/> | |
58 <param name="re_reverse" type="boolean" checked="True" label="Re-reverse bases and qualities of reads with negative strand flag set before writing them to fastq" help="RE_REVERSE; default=True"/> | |
59 <param name="interleave" type="boolean" label="Will generate an interleaved fastq if paired, each line will have /1 or /2 to describe which end it came from" help="INTERLEAVE; default=False"/> | |
60 <param name="include_non_pf_reads" type="boolean" label="Include non-PF reads from the SAM/BAM dataset into the output FASTQ" help="INCLUDE_NON_PF_READS; PF means 'passes filtering'. Reads whose 'not passing quality controls' flag is set are non-PF reads; default=False"/> | |
61 <param name="clipping_attribute" type="text" size="4" value="null" label="The attribute that stores the position at which the SAM/BAM record should be clipped" help="CLIPPING_ATTRIBUTE; default=null"/> | |
62 <param name="clipping_action" type="text" size="10" value="null" label="The action that should be taken with clipped reads: 'X' means the reads and qualities should be trimmed at the clipped position; 'N' means the bases should be changed to Ns in the clipped region; and any integer means that the base qualities should be set to that value in the clipped region" help="CLIPPING_ACTION; default=null"/> | |
63 <param name="read1_trim" type="integer" value="0" min="0" label="The number of bases to trim from the beginning of read 1" help="READ1_TRIM; default=0"/> | |
64 <param name="read1_max_bases_to_write" type="integer" value="-1" label="The maximum number of bases to write from read 1 after trimming" help="READ1_MAX_BASES_TO_WRITE; If there are fewer than this many bases left after trimming, all will be written. If this value is null then all bases left after trimming will be written; default=null (-1)"/> | |
65 <param name="read2_trim" type="integer" value="0" min="0" label="The number of bases to trim from the beginning of read 2" help="READ2_TRIM; default=0"/> | |
66 <param name="read2_max_bases_to_write" type="integer" value="-1" label="The maximum number of bases to write from read 2 after trimming" help="READ2_MAX_BASES_TO_WRITE; If there are fewer than this many bases left after trimming, all will be written. If this value is null then all bases left after trimming will be written; default=null (-1)"/> | |
67 <param name="include_non_primary_alignments" type="boolean" label="If true, include non-primary alignments in the output" help="INCLUDE_NON_PRIMARY_ALIGNMENTS; Support of non-primary alignments in SamToFastq is not comprehensive, so there may be exceptions if this is set to true and there are paired reads with non-primary alignments; default=False"/> | |
68 | |
69 <expand macro="VS" /> | |
70 | |
71 </inputs> | |
72 | |
0 | 73 <outputs> |
5 | 74 <!-- here dataset discovery is based on fact that if OUTPUT_PER_RG=true this tool automatically adds .fastq extension to emitted files --> |
75 <data format="txt" name="report" label="SamToFastq run" hidden="true"> | |
76 <discover_datasets pattern="(?P<designation>.+)\.fastq" ext="fastqsanger" visible="true"/> | |
0 | 77 </data> |
78 </outputs> | |
5 | 79 |
0 | 80 <tests> |
5 | 81 <test> |
82 <param name="inputFile" value="picard_SamToFastq.bam" ftype="bam"/> | |
83 <param name="output_per_rg" value="false"/> | |
84 <param name="re_reverse" value="true"/> | |
85 <param name="interleave" value="true"/> | |
86 <param name="include_non_pf_reads" value="false"/> | |
87 <param name="clipping_attribute" value="null" /> | |
88 <param name="clipping_action" value="null" /> | |
89 <param name="read1_trim" value="0" /> | |
90 <param name="read1_max_bases_to_write" value="-1"/> | |
91 <param name="read2_trim" value="0" /> | |
92 <param name="read2_max_bases_to_write" value="-1"/> | |
93 <param name="include_non_primary_alignments" value="false"/> | |
94 <output name="report"> | |
95 <assert_contents> | |
96 <has_line line="BAM" /> | |
97 </assert_contents> | |
98 <discovered_dataset designation="INTERLEAVED" file="picard_SamToFastq_test1.fq" ftype="fastqsanger"/> | |
99 </output> | |
100 </test> | |
0 | 101 </tests> |
5 | 102 |
103 <stdio> | |
104 <exit_code range="1:" level="fatal"/> | |
105 </stdio> | |
106 | |
0 | 107 <help> |
108 | |
5 | 109 **Purpose** |
0 | 110 |
5 | 111 Extracts read sequences and qualities from the input SAM/BAM dataset and outputs them in Sanger fastq format. In the RE_REVERSE=True mode (default behavior), if the read is aligned and the alignment is to the reverse strand on the genome, the read's sequence from input SAM.BAM dataset will be reverse-complemented prior to writing it to fastq in order restore correctly the original read sequence as it was generated by the sequencer. |
0 | 112 |
5 | 113 ----- |
0 | 114 |
5 | 115 .. class:: warningmark |
0 | 116 |
5 | 117 **DANGER: Multiple Outputs** |
0 | 118 |
5 | 119 Generating per readgroup fastq (setting **OUTPUT_PER_RG** to True) may produce very large numbers of outputs. Know what you are doing! |
0 | 120 |
5 | 121 @dataset_collections@ |
0 | 122 |
5 | 123 @description@ |
0 | 124 |
5 | 125 FASTQ=File |
126 F=File Output fastq file (single-end fastq or, if paired, first end of the pair fastq). | |
127 Required. Cannot be used in conjuction with option(s) OUTPUT_PER_RG (OPRG) | |
128 | |
129 SECOND_END_FASTQ=File | |
130 F2=File Output fastq file (if paired, second end of the pair fastq). Default value: null. | |
131 Cannot be used in conjuction with option(s) OUTPUT_PER_RG (OPRG) | |
132 | |
133 UNPAIRED_FASTQ=File | |
134 FU=File Output fastq file for unpaired reads; may only be provided in paired-fastq mode Default | |
135 value: null. Cannot be used in conjuction with option(s) OUTPUT_PER_RG (OPRG) | |
136 | |
137 OUTPUT_PER_RG=Boolean | |
138 OPRG=Boolean Output a fastq file per read group (two fastq files per read group if the group is | |
139 paired). Default value: false. Possible values: {true, false} Cannot be used in | |
140 conjuction with option(s) SECOND_END_FASTQ (F2) UNPAIRED_FASTQ (FU) FASTQ (F) | |
141 | |
142 OUTPUT_DIR=File | |
143 ODIR=File Directory in which to output the fastq file(s). Used only when OUTPUT_PER_RG is true. | |
144 Default value: null. | |
145 | |
146 RE_REVERSE=Boolean | |
147 RC=Boolean Re-reverse bases and qualities of reads with negative strand flag set before writing them | |
148 to fastq Default value: true. Possible values: {true, false} | |
149 | |
150 INTERLEAVE=Boolean | |
151 INTER=Boolean Will generate an interleaved fastq if paired, each line will have /1 or /2 to describe | |
152 which end it came from Default value: false. Possible values: {true, false} | |
153 | |
154 INCLUDE_NON_PF_READS=Boolean | |
155 NON_PF=Boolean Include non-PF reads from the SAM file into the output FASTQ files. PF means 'passes | |
156 filtering'. Reads whose 'not passing quality controls' flag is set are non-PF reads. | |
157 Default value: false. Possible values: {true, false} | |
0 | 158 |
5 | 159 CLIPPING_ATTRIBUTE=String |
160 CLIP_ATTR=String The attribute that stores the position at which the SAM record should be clipped Default | |
161 value: null. | |
162 | |
163 CLIPPING_ACTION=String | |
164 CLIP_ACT=String The action that should be taken with clipped reads: 'X' means the reads and qualities | |
165 should be trimmed at the clipped position; 'N' means the bases should be changed to Ns in | |
166 the clipped region; and any integer means that the base qualities should be set to that | |
167 value in the clipped region. Default value: null. | |
168 | |
169 READ1_TRIM=Integer | |
170 R1_TRIM=Integer The number of bases to trim from the beginning of read 1. Default value: 0. | |
171 | |
172 READ1_MAX_BASES_TO_WRITE=Integer | |
173 R1_MAX_BASES=Integer The maximum number of bases to write from read 1 after trimming. If there are fewer than | |
174 this many bases left after trimming, all will be written. If this value is null then all | |
175 bases left after trimming will be written. Default value: null. | |
176 | |
177 READ2_TRIM=Integer | |
178 R2_TRIM=Integer The number of bases to trim from the beginning of read 2. Default value: 0. | |
179 | |
180 READ2_MAX_BASES_TO_WRITE=Integer | |
181 R2_MAX_BASES=Integer The maximum number of bases to write from read 2 after trimming. If there are fewer than | |
182 this many bases left after trimming, all will be written. If this value is null then all | |
183 bases left after trimming will be written. Default value: null. | |
184 | |
185 INCLUDE_NON_PRIMARY_ALIGNMENTS=Boolean | |
186 If true, include non-primary alignments in the output. Support of non-primary alignments | |
187 in SamToFastq is not comprehensive, so there may be exceptions if this is set to true and | |
188 there are paired reads with non-primary alignments. Default value: false. | |
189 Possible values: {true, false} | |
190 | |
191 @more_info@ | |
0 | 192 |
193 </help> | |
194 </tool> | |
5 | 195 |
196 |