comparison fasterq_dump.xml @ 15:f5ea3ce9b9b0 draft

"planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/sra-tools commit fe3f54a0d3edb83fcf6752e3b1524c582b4febd5"
author iuc
date Tue, 10 Sep 2019 11:35:35 -0400
parents
children aad3885b3216
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14:1790dcf3c32d 15:f5ea3ce9b9b0
1 <tool id="fasterq_dump" name="Faster Download and Extract Reads in FASTQ" version="@VERSION@.4" profile="16.01">
2 <description>format from NCBI SRA</description>
3 <macros>
4 <import>sra_macros.xml</import>
5 </macros>
6 <expand macro="requirements"/>
7 <version_command>fasterq-dump --version</version_command>
8 <command detect_errors="exit_code"><![CDATA[
9
10 @SET_ACCESSIONS@
11 #if $input.input_select == "file":
12 acc='${input.file.name}' &&
13 ln -s '${input.file}' "\$acc" &&
14 #end if
15
16 fasterq-dump "\$acc" -e \${GALAXY_SLOTS:-1}
17 $adv.split
18 #if str( $adv.minlen ) != "":
19 --min-read-len "$adv.minlen"
20 #end if
21 $adv.skip_technical >> $log 2>&1
22 &&
23 mkdir -p output &&
24 mkdir -p outputOther &&
25 count=`ls *.fastq | wc -l` &&
26 echo "There are \$count fastq" &&
27 data=(\$(ls *.fastq)) &&
28 if [ "\$count" -eq 1 ]; then
29 gzip -c "\${data[0]}" > output/"\${acc}"__single.fastqsanger.gz &&
30 rm "\${data[0]}";
31 elif [ "$adv.split" = "--split-3" ]; then
32 if [ -e "\${acc}".fastq ]; then
33 gzip -c "\${acc}".fastq > outputOther/"\${acc}"__single.fastqsanger.gz;
34 fi &&
35 gzip -c "\${acc}"_1.fastq > output/"\${acc}"_forward.fastqsanger.gz &&
36 gzip -c "\${acc}"_2.fastq > output/"\${acc}"_reverse.fastqsanger.gz &&
37 rm "\${acc}"*.fastq;
38 elif [ "\$count" -eq 2 ]; then
39 #if $adv.skip_technical:
40 gzip -c "\${data[0]}" > output/"\${acc}"_forward.fastqsanger.gz &&
41 gzip -c "\${data[1]}" > output/"\${acc}"_reverse.fastqsanger.gz &&
42 #else
43 gzip -c "\${data[0]}" > outputOther/"\${data[0]}"sanger.gz &&
44 gzip -c "\${data[1]}" > outputOther/"\${data[1]}"sanger.gz &&
45 #end if
46 rm "\${data[0]}" &&
47 rm "\${data[1]}";
48 else
49 for file in \${data[*]}; do
50 gzip -c "\$file" > outputOther/"\$file"sanger.gz &&
51 rm "\$file";
52 done;
53 fi;
54 #if $input.input_select=="file_list":
55 ) ; done
56
57 ;
58 #elif $input.input_select=="accession_number":
59 );
60 #end if
61 ]]>
62 </command>
63 <inputs>
64 <expand macro="input_conditional"/>
65 <section name="adv" title="Advanced Options" expanded="False">
66 <param name="minlen" type="integer" label="Minimum read length" optional="true" help="Filter by sequence length. Will dump only reads longer or equal to this value." argument="--min-read-len"/>
67 <param name="split" type="select" display="radio" label="Select how to split the spots" help="This option will only be used when there are multiple reads per spot (for example paired-end).">
68 <option value="--split-3">--split-3: write properly paired biological reads into different files and single reads in another file</option>
69 <option value="--split-files">--split-files: write reads into different files (forward and reverse may not match if one read is empty)</option>
70 <option value="--split-spot">--split-spot: split spots into reads (only one output file)</option>
71 <option value="--concatenate-reads">--concatenate-reads: writes whole spots into one file</option>
72 </param>
73 <param name="skip_technical" type="boolean" truevalue="--skip-technical" falsevalue="--include-technical" checked="True" label="Dump only biological reads" help="Will not be used if --split-3 is selected." argument="--skip-technical/--include-technical"/>
74 </section>
75 </inputs>
76 <outputs>
77 <data name="log" format="txt" label="fasterq-dump log"/>
78 <collection name="list_paired" type="list:paired" label="Pair-end data (fasterq-dump)">
79
80 <!-- Use named regex group to grab pattern
81 <identifier_0>_<identifier_1>.fq. Here identifier_0 is the list
82 identifier in the nested collection and identifier_1 is either
83 forward or reverse (for instance samp1_forward.fq).
84 -->
85
86 <discover_datasets pattern="(?P&lt;identifier_0&gt;[^_]+)_(?P&lt;identifier_1&gt;[^_]+)\.fastqsanger.gz" directory="output" ext="fastqsanger.gz" />
87 </collection>
88 <collection name="output_collection" type='list' label="Single-end data (fasterq-dump)">
89 <discover_datasets pattern="(?P&lt;designation&gt;.+)__single\.fastqsanger.gz" directory="output" ext='fastqsanger.gz'/>
90 </collection>
91 <collection name="output_collection_other" type='list' label="Other data (fasterq-dump)">
92 <discover_datasets pattern="(?P&lt;designation&gt;.+)\.fastqsanger\.gz" directory="outputOther" format="fastqsanger.gz"/>
93 </collection>
94 </outputs>
95 <tests>
96 <test>
97 <param name="input_select" value="accession_number"/>
98 <param name="accession" value="ERR086330"/>
99 <output_collection name="list_paired" type="list:paired">
100 <element name="ERR086330">
101 <element name="forward" file="ERR086330_1.fastq.gz" decompress="True">
102 </element>
103 <element name="reverse" file="ERR086330_2.fastq.gz" decompress="True">
104 </element>
105 </element>
106 </output_collection>
107 </test>
108 <test>
109 <param name="input_select" value="accession_number"/>
110 <param name="accession" value="SRR002702"/>
111 <param name="split" value="--split-files"/>
112 <param name="skip_technical" value="False"/>
113 <output_collection name="output_collection_other" type="list">
114 <element name="SRR002702_1" file="SRR002702_1.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
115 <element name="SRR002702_2" file="SRR002702_2.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
116 </output_collection>
117 </test>
118 <test>
119 <param name="input_select" value="file"/>
120 <param name="file" value="SRR522874.sra"/>
121 <param name="split" value="--split-files"/>
122 <param name="skip_technical" value="True"/>
123 <output_collection name="list_paired" type="list:paired">
124 <element name="SRR522874.sra">
125 <element name="forward" file="SRR522874.sra_2.fastq.gz" decompress="True">
126 </element>
127 <element name="reverse" file="SRR522874.sra_4.fastq.gz" decompress="True">
128 </element>
129 </element>
130 </output_collection>
131 </test>
132 <test>
133 <param name="input_select" value="file"/>
134 <param name="file" value="SRR522874.sra"/>
135 <param name="split" value="--split-files"/>
136 <param name="skip_technical" value="False"/>
137 <output_collection name="output_collection_other" type="list">
138 <element name="SRR522874.sra_1" file="SRR522874.sra_1.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
139 <element name="SRR522874.sra_2" file="SRR522874.sra_2.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
140 <element name="SRR522874.sra_3" file="SRR522874.sra_3.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
141 <element name="SRR522874.sra_4" file="SRR522874.sra_4.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
142 </output_collection>
143 </test>
144 <test>
145 <param name="input_select" value="file_list"/>
146 <param name="file_list" value="list_sra"/>
147 <param name="minlen" value="21"/>
148 <output_collection name="output_collection_other" type="list">
149 <element name="SRR522874__single" file="SRR522874.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
150 </output_collection>
151 <output_collection name="list_paired" type="list:paired">
152 <element name="SRR522874">
153 <element name="forward" file="SRR522874_1.fastq.gz" decompress="True">
154 </element>
155 <element name="reverse" file="SRR522874_2.fastq.gz" decompress="True">
156 </element>
157 </element>
158 </output_collection>
159 <output_collection name="output_collection" type="list">
160 <element name="SRR002702" file="SRR002702_2.fastq.gz" ftype="fastqsanger.gz" decompress="True"/>
161 </output_collection>
162 </test>
163 </tests>
164 <help><![CDATA[
165 **What it does?**
166
167 This tool extracts data (in fastq_ format) from the Short Read Archive (SRA) at the National Center for Biotechnology Information (NCBI). It is based on the fasterq-dump_ utility of the SRA Toolkit.
168
169 **How to use it?**
170
171 There are three ways in which you can download data:
172
173 1. Data for single accession
174 2. Multiple datasets using a list of accessions
175 3. Extract data from already uploaded SRA dataset
176
177 Below we discuss each in detail.
178
179 ------
180
181 **Uploading data for a single accession**
182
183 When you type a single accession number (e.g., `SRR1582967`) into **Accession** box and click **Execute** the tool will fetch data for you.
184
185 -----
186
187 **Uploading multiple datasets using a list of accessions**
188
189 A more realistic scenario is when you want to upload a number of datasets at once. To do this you need a list of accession, where there is only one accession per line (see below for information on how to generate such a file). Once you have this file:
190
191 1. Upload it into your history using Galaxy's upload tool
192 2. Once the list of accessions is uploaded choose *List of SRA accessions, one per line* from **select input type** dropdown
193 3. Choose uploaded file within the **sra accession list** field
194 4. Click **Execute**
195
196 -----
197
198 **Extract data from already uploaded SRA dataset**
199
200 If a SRA dataset is present in the history, it can be converted into fastq dataset by setting **select input type** drop-down to *SRA archive in current history*. Just like in the case of extracting data for single accession number the following applies:
201
202 - if data is paired-ended (or mate-pair) the tool will generate a single *interleaved* dataset, in which forward and reverse mates are alternating (see example below).
203 - if data is single ended, a standard fastq dataset will be produced
204
205 -----
206
207 **Output**
208
209 In every case, fastq datasets produced will be saved in Galaxy's history as a collection_ - a single history element containing multiple datasets.
210 In fact, three collections will be produced: one containing paired-end data, another containing single-end data, and a third one which contains reads which could not be classified.
211 Some collections may be empty if the accessions provided in the list does not contain one of the type of data.
212
213 .. class:: warningmark
214
215 When you decide to dump technical reads (in Advanced Options Dump only biological reads is set to No), you will probably find your PAIRED data in the other data collection as it is impossible to determine if it was 2 biological reads or one biological and one technical.
216
217 .. class:: warningmark
218
219 By default, only biological reads are dumped and in case of PAIRED dataset only the spots which have both reads will be in the paired-end collection. The remaining single reads will be in the other colletion.
220 To keep all reads, and maybe do not have the same number of reads in forward and reverse use the --split-files option in Advanced Options, Select how to split the spots.
221
222 @ACCESSION_LIST_HOWTO@
223
224 -----
225
226
227 .. _fastq: https://en.wikipedia.org/wiki/FASTQ_format
228 .. _fastq-dump: https://ncbi.github.io/sra-tools/fastq-dump.html
229 .. _fasterq-dump: https://github.com/ncbi/sra-tools/wiki/HowTo:-fasterq-dump
230 .. _collection: https://galaxyproject.org/tutorials/collections/
231 .. _link: http://www.ncbi.nlm.nih.gov/Traces/sra/sra.cgi?view=studies
232
233 @SRATOOLS_ATTRRIBUTION@
234
235 ]]>
236 </help>
237 <expand macro="citation"/>
238 </tool>