Galaxy |

Changeset 0:1d773da0ccf0 (2015-01-27)

Next changeset 1:8ff0ac66f1a3 (2015-05-13)

Commit message:
Uploaded v0.0.2, fixed some error messages

added:
test-data/SRR639755_mito_pairs.fastq.gz
test-data/SRR639755_sample_by_coord.sam
test-data/SRR639755_sample_lax.fastq
test-data/SRR639755_sample_strict.fastq
tools/seq_filter_by_mapping/README.rst
tools/seq_filter_by_mapping/seq_filter_by_mapping.py
tools/seq_filter_by_mapping/seq_filter_by_mapping.xml
tools/seq_filter_by_mapping/tool_dependencies.xml

diff -r 000000000000 -r 1d773da0ccf0 test-data/SRR639755_mito_pairs.fastq.gz

Binary file test-data/SRR639755_mito_pairs.fastq.gz has changed

diff -r 000000000000 -r 1d773da0ccf0 test-data/SRR639755_sample_by_coord.sam
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/test-data/SRR639755_sample_by_coord.sam Tue Jan 27 08:31:13 2015 -0500

@@ -0,0 +1,14 @@
+@HD VN:1.0 SO:coordinate
+@SQ SN:gi|187250362|ref|NC_010642.1| LN:16990
+@PG ID:clc_mapper VN:4.10.86742 CL:clc_mapper -d -z xxx -p fb ss 1 1000 -q yyy -o temp_job.cas --cpus 8
+@RG ID:RG_0 DS:yyy PG:clc_mapper
+SRR639755.6451003 99 gi|187250362|ref|NC_010642.1| 1352 255 7S94M = 1604 353 ATATCTGCAGTTAACATAAAAATATAGCACGAAAGTAACTTTAATATCTCCGACCACACGATAGCTAAGACCCAAACTGGGATTAGATACCCCGCTATGCT <?7A4ADDFHHDHIIBH<HGDHEIG>HBHGGEFH@?D<GDGGHDGGG>DDDFGFHGHGIGB;CEH>A>DEEC?B;;=@CC9;;?CCCCCCC@<9>5<<@A4 RG:Z:RG_0 MD:Z:8G8C22T2T42A7 NM:i:11
+SRR639755.6451003 147 gi|187250362|ref|NC_010642.1| 1604 255 101M = 1352 353 TTCAGCCTACATACCGCCATCTTCAGCAAACCCTAAAAAGGAAGAAAAGTAAGCACAAGTGCCTTAACACAAAAAAGTTAGGTCAAGGTGTAGCCCATGAG >?BA::3B:C?98B@@CC>CA>EEEFFFBCEE>FJJIHC@DDGIIIHF@HFHCFBHD@GGHBFD@HHBDGAFCCEC8HEIHDH>HEHBHHFGHDDD=F@@@ RG:Z:RG_0 MD:Z:9T50AT7T31 NM:i:4
+SRR639755.6035319 137 gi|187250362|ref|NC_010642.1| 9094 255 101M * 0 0 TACTTATGTCTCTCATTTTATTTATTGGGCCAACAAATCTGCTAGGTCTACTACCTCACTCATTTACTCCAACTACGCAATTATCAATAAAACTAGGCATA ?@@FD;:+AHB4<C9F4HEFH@EAA?EE++<<A@FHADDB<?:4D)0*0?D?BFFGIIIDBE:=BDE)=FHGED>;('(5,;;;6;6;>;>(5((5?C(,: RG:Z:RG_0 MD:Z:29T46C14C9 NM:i:3
+SRR639755.2301126 137 gi|187250362|ref|NC_010642.1| 9117 255 101M * 0 0 ATTGGGTCAACAAATCTGCTAGGTCTACTACCTCACTCATTTACTCCAACTACCCAATTATCAATAAACCTAGGCATAGCCATCCCCTTGTGAGCCGGCAC ?@BDB;=AAAAFFDHBGAAHI>;<AFCAF@?GEDEEFHAHFH@<F<D@GGEHIEF@HIE>GH=B@CCGAHC@@DEHHFEHDFFFFDDE>?CCDACCBDB@B RG:Z:RG_0 MD:Z:101 NM:i:0
+SRR639755.6955680 89 gi|187250362|ref|NC_010642.1| 9285 255 97M4S * 0 0 GTCCCCTTAATCCCTATGCTCGTAATTATCGAAACTATCAGCCTTTTTATCCAGCCCGTAGCCCTAGCCGTACGACTCACAGCTAATATTACTGCAGATAT 9<>8CAACC?CBC@DDD@?<8A@>(BBC?DDAB;?C@BFFEEAIIHD@EGF6GGGGAFD?B8GCEJJIIHEIIHEGIHHIJJIEGIGGDHFFC=2FFFBB? RG:Z:RG_0 MD:Z:97 NM:i:0
+SRR639755.7076397 89 gi|187250362|ref|NC_010642.1| 9285 255 97M4S * 0 0 GTCCCCTTAATCCCTATGCTCGTAATTATCGAAACTATCAGCCTTTTTATCCAGCCCGTAGCCCTAGCCGTACGACTCACAGCTAATATTACTGCAGATAT BBDBCDDCDDCDDCDCBDDD@CACC@DFBDDEB>DFFFFFHHHJJJIGGDJIIGJJIIHGIJJJIJIJIIHGIJIJIJJJJJJJJJJJHHHFC=2FFD?@= RG:Z:RG_0 MD:Z:97 NM:i:0
+SRR639755.2301126 69 * 0 255 * gi|187250362|ref|NC_010642.1| 9117 0 ATATCTGCAGTGAGCCTGACTTGGGGCTCGAACTCATGAACCATGAGATCATGACCTGAGCTGAAGTCGTACGGCTAGGGCTACGGGCTGGATAAAAAGGC +1=BDDDDHHHFBF?GDECFGHDEFH@?C:?F@;DH@4B?9)?<BF?=)8C@G=88CC@EHICHH>7=;?;?><A>=A;?(<?9'2-<>B91(>@@CC5?< RG:Z:RG_0
+SRR639755.6035319 69 * 0 255 * gi|187250362|ref|NC_010642.1| 9094 0 ATATCTGCAGTAATATTAGCTGTGAGTCGTACGGCTAGGGCCACGGGCTGGGTAGCAACGATGCTGGGGTGCAGAATTAGGCGGCTGGGCATTAAAGCGAC 1:;44222222<ABDGG@I?4CFD<ACBG?8ACF@0???B9)0)7A0<@8'().()).(,(.5,((-,',,(((,,(((++(0&&0&&(((+((((+()(& RG:Z:RG_0
+SRR639755.6955680 165 * 0 255 * gi|187250362|ref|NC_010642.1| 9285 0 CCGACTGAGCCACCCAGGCGCCCCTAAATTTGCTTTTAATTTTAATGGTGGTTATATTTATTGGGGCAACAAATCTGCTAGGTCTACTACCTCACTCATTT @@BFFADDF?FHHJAE:A@GEHHGHGGIGGE9DCHHHIJIIIG@GGBGHID';=7C==@:=.=CH64<?(;?B>35>@:@>9,::@>;5><A>:<:>9444 RG:Z:RG_0
+SRR639755.7076397 165 * 0 255 * gi|187250362|ref|NC_010642.1| 9285 0 TGACAGCACATTTATTTACAAACTGGTTTGCTGAATATTTTAATCCCACTGTTGAGGCCTACTACCTCACTCATTTACTCCAACTACCCAATTATCAATAA CC@FFFFFHFHHHJJJJJJIJJJJJIFHGIIIJIIGEGIJJJJIJIHIJHIJIIJJIIIJJJJJJJIJJJJIJJJJGHHGHGFFFFFEDCDDDDDD;>;AC RG:Z:RG_0

diff -r 000000000000 -r 1d773da0ccf0 test-data/SRR639755_sample_lax.fastq
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/test-data/SRR639755_sample_lax.fastq Tue Jan 27 08:31:13 2015 -0500

@@ -0,0 +1,40 @@
+@SRR639755.2301126/1
+ATATCTGCAGTGAGCCTGACTTGGGGCTCGAACTCATGAACCATGAGATCATGACCTGAGCTGAAGTCGTACGGCTAGGGCTACGGGCTGGATAAAAAGGC
++
++1=BDDDDHHHFBF?GDECFGHDEFH@?C:?F@;DH@4B?9)?<BF?=)8C@G=88CC@EHICHH>7=;?;?><A>=A;?(<?9'2-<>B91(>@@CC5?<
+@SRR639755.2301126/2
+ATTGGGTCAACAAATCTGCTAGGTCTACTACCTCACTCATTTACTCCAACTACCCAATTATCAATAAACCTAGGCATAGCCATCCCCTTGTGAGCCGGCAC
++
+?@BDB;=AAAAFFDHBGAAHI>;<AFCAF@?GEDEEFHAHFH@<F<D@GGEHIEF@HIE>GH=B@CCGAHC@@DEHHFEHDFFFFDDE>?CCDACCBDB@B
+@SRR639755.6035319/1
+ATATCTGCAGTAATATTAGCTGTGAGTCGTACGGCTAGGGCCACGGGCTGGGTAGCAACGATGCTGGGGTGCAGAATTAGGCGGCTGGGCATTAAAGCGAC
++
+1:;44222222<ABDGG@I?4CFD<ACBG?8ACF@0???B9)0)7A0<@8'().()).(,(.5,((-,',,(((,,(((++(0&&0&&(((+((((+()(&
+@SRR639755.6035319/2
+TACTTATGTCTCTCATTTTATTTATTGGGCCAACAAATCTGCTAGGTCTACTACCTCACTCATTTACTCCAACTACGCAATTATCAATAAAACTAGGCATA
++
+?@@FD;:+AHB4<C9F4HEFH@EAA?EE++<<A@FHADDB<?:4D)0*0?D?BFFGIIIDBE:=BDE)=FHGED>;('(5,;;;6;6;>;>(5((5?C(,:
+@SRR639755.6451003/1
+ATATCTGCAGTTAACATAAAAATATAGCACGAAAGTAACTTTAATATCTCCGACCACACGATAGCTAAGACCCAAACTGGGATTAGATACCCCGCTATGCT
++
+<?7A4ADDFHHDHIIBH<HGDHEIG>HBHGGEFH@?D<GDGGHDGGG>DDDFGFHGHGIGB;CEH>A>DEEC?B;;=@CC9;;?CCCCCCC@<9>5<<@A4
+@SRR639755.6451003/2
+CTCATGGGCTACACCTTGACCTAACTTTTTTGTGTTAAGGCACTTGTGCTTACTTTTCTTCCTTTTTAGGGTTTGCTGAAGATGGCGGTATGTAGGCTGAA
++
+@@@F=DDDHGFHHBHEH>HDHIEH8CECCFAGDBHH@DFBHGG@DHBFCHFH@FHIIIGDD@CHIJJF>EECBFFFEEE>AC>CC@@B89?C:B3::AB?>
+@SRR639755.6955680/1
+ATATCTGCAGTAATATTAGCTGTGAGTCGTACGGCTAGGGCTACGGGCTGGATAAAAAGGCTGATAGTTTCGATAATTACGAGCATAGGGATTAAGGGGAC
++
+?BBFFF2=CFFHDGGIGEIJJIHHIGEHIIEHIIJJECG8B?DFAGGGG6FGE@DHIIAEEFFB@C?;BADD?CBB(>@A8<?@DDD@CBC?CCAAC8><9
+@SRR639755.6955680/2
+CCGACTGAGCCACCCAGGCGCCCCTAAATTTGCTTTTAATTTTAATGGTGGTTATATTTATTGGGGCAACAAATCTGCTAGGTCTACTACCTCACTCATTT
++
+@@BFFADDF?FHHJAE:A@GEHHGHGGIGGE9DCHHHIJIIIG@GGBGHID';=7C==@:=.=CH64<?(;?B>35>@:@>9,::@>;5><A>:<:>9444
+@SRR639755.7076397/1
+ATATCTGCAGTAATATTAGCTGTGAGTCGTACGGCTAGGGCTACGGGCTGGATAAAAAGGCTGATAGTTTCGATAATTACGAGCATAGGGATTAAGGGGAC
++
+=@?DFF2=CFHHHJJJJJJJJJJJIJIJIGHIIJIJIJJJIGHIIJJGIIJDGGIJJJHHHFFFFFD>BEDDBFD@CCAC@DDDBCDCDDCDDCDDCBDBB
+@SRR639755.7076397/2
+TGACAGCACATTTATTTACAAACTGGTTTGCTGAATATTTTAATCCCACTGTTGAGGCCTACTACCTCACTCATTTACTCCAACTACCCAATTATCAATAA
++
+CC@FFFFFHFHHHJJJJJJIJJJJJIFHGIIIJIIGEGIJJJJIJIHIJHIJIIJJIIIJJJJJJJIJJJJIJJJJGHHGHGFFFFFEDCDDDDDD;>;AC

diff -r 000000000000 -r 1d773da0ccf0 test-data/SRR639755_sample_strict.fastq
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/test-data/SRR639755_sample_strict.fastq Tue Jan 27 08:31:13 2015 -0500

@@ -0,0 +1,8 @@
+@SRR639755.6451003/1
+ATATCTGCAGTTAACATAAAAATATAGCACGAAAGTAACTTTAATATCTCCGACCACACGATAGCTAAGACCCAAACTGGGATTAGATACCCCGCTATGCT
++
+<?7A4ADDFHHDHIIBH<HGDHEIG>HBHGGEFH@?D<GDGGHDGGG>DDDFGFHGHGIGB;CEH>A>DEEC?B;;=@CC9;;?CCCCCCC@<9>5<<@A4
+@SRR639755.6451003/2
+CTCATGGGCTACACCTTGACCTAACTTTTTTGTGTTAAGGCACTTGTGCTTACTTTTCTTCCTTTTTAGGGTTTGCTGAAGATGGCGGTATGTAGGCTGAA
++
+@@@F=DDDHGFHHBHEH>HDHIEH8CECCFAGDBHH@DFBHGG@DHBFCHFH@FHIIIGDD@CHIJJF>EECBFFFEEE>AC>CC@@B89?C:B3::AB?>

diff -r 000000000000 -r 1d773da0ccf0 tools/seq_filter_by_mapping/README.rst
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/tools/seq_filter_by_mapping/README.rst Tue Jan 27 08:31:13 2015 -0500

@@ -0,0 +1,114 @@
+Galaxy tool to filter FASTA, FASTQ or SFF sequences by SAM/BAM mapping
+======================================================================
+
+This tool is copyright 2014 by Peter Cock, The James Hutton Institute
+(formerly SCRI, Scottish Crop Research Institute), UK. All rights reserved.
+See the licence text below.
+
+This tool is a short Python script (using Biopython library functions) which
+divides a FASTA, FASTQ, or SFF file in two, those sequences which do or do
+not map according to given SAM/BAM file(s).
+
+Example uses include mapping of FASTQ reads against a known contaminant
+in order to remove reads prior to a de novo assembly.
+
+This tool is available from the Galaxy Tool Shed at:
+
+* http://toolshed.g2.bx.psu.edu/view/peterjc/seq_filter_by_mapping
+
+See also related tools:
+
+* http://toolshed.g2.bx.psu.edu/view/peterjc/seq_filter_by_id
+* http://toolshed.g2.bx.psu.edu/view/peterjc/seq_select_by_id
+* http://toolshed.g2.bx.psu.edu/view/peterjc/seq_rename
+
+
+Automated Installation
+======================
+
+This should be straightforward using the Galaxy Tool Shed, which should be
+able to automatically install the dependency on Biopython and samtools
+and then install this tool and run its unit tests.
+
+
+Manual Installation
+===================
+
+There are just two files to install to use this tool from within Galaxy:
+
+* ``seq_filter_by_mapping.py`` (the Python script)
+* ``seq_filter_by_mapping.xml`` (the Galaxy tool definition)
+
+The suggested location is a dedicated ``tools/seq_filter_by_mapping/`` folder.
+
+You will also need to modify the ``tools_conf.xml`` file to tell Galaxy to offer the
+tool. One suggested location is in the filters section. Simply add the line::
+
+    <tool file="seq_filter_by_mapping/seq_filter_by_mapping.xml" />
+
+If you wish to run the unit tests, also move/copy the ``test-data/`` files
+under Galaxy's ``test-data/`` folder. Then::
+
+    $ ./run_tests.sh -id seq_filter_by_mapping
+
+You will also need to install Biopython 1.54 or later. That's it.
+
+
+History
+=======
+
+======= ======================================================================
+Version Changes
+------- ----------------------------------------------------------------------
+v0.0.1  - Initial version.
+v0.0.2  - Fixed some error messages.
+======= ======================================================================
+
+
+Developers
+==========
+
+Development is on this GitHub repository:
+https://github.com/peterjc/pico_galaxy/tree/master/tools/seq_filter_by_mapping
+
+Much of the code was copied from my older tool:
+https://github.com/peterjc/pico_galaxy/tree/master/tools/seq_filter_by_id
+
+For making the "Galaxy Tool Shed" http://toolshed.g2.bx.psu.edu/ tarball use
+the following command from the Galaxy root folder::
+
+    $ tar -czf seq_filter_by_mapping.tar.gz tools/seq_filter_by_mapping/README.rst tools/seq_filter_by_mapping/seq_filter_by_mapping.py tools/seq_filter_by_mapping/seq_filter_by_mapping.xml tools/seq_filter_by_mapping/tool_dependencies.xml test-data/SRR639755_mito_pairs.fastq.gz test-data/SRR639755_sample_by_coord.sam test-data/SRR639755_sample_strict.fastq test-data/SRR639755_sample_lax.fastq
+
+Check this worked::
+
+    $ tar -tzf seq_filter_by_mapping.tar.gz
+    tools/seq_filter_by_mapping/README.rst
+    tools/seq_filter_by_mapping/seq_filter_by_mapping.py
+    tools/seq_filter_by_mapping/seq_filter_by_mapping.xml
+    tools/seq_filter_by_mapping/tool_dependencies.xml
+    test-data/SRR639755_mito_pairs.fastq.gz
+    test-data/SRR639755_sample_by_coord.sam
+    test-data/SRR639755_sample_strict.fastq
+    test-data/SRR639755_sample_lax.fastq
+
+
+Licence (MIT)
+=============
+
+Permission is hereby granted, free of charge, to any person obtaining a copy
+of this software and associated documentation files (the "Software"), to deal
+in the Software without restriction, including without limitation the rights
+to use, copy, modify, merge, publish, distribute, sublicense, and/or sell
+copies of the Software, and to permit persons to whom the Software is
+furnished to do so, subject to the following conditions:
+
+The above copyright notice and this permission notice shall be included in
+all copies or substantial portions of the Software.
+
+THE SOFTWARE IS PROVIDED "AS IS", WITHOUT WARRANTY OF ANY KIND, EXPRESS OR
+IMPLIED, INCLUDING BUT NOT LIMITED TO THE WARRANTIES OF MERCHANTABILITY,
+FITNESS FOR A PARTICULAR PURPOSE AND NONINFRINGEMENT. IN NO EVENT SHALL THE
+AUTHORS OR COPYRIGHT HOLDERS BE LIABLE FOR ANY CLAIM, DAMAGES OR OTHER
+LIABILITY, WHETHER IN AN ACTION OF CONTRACT, TORT OR OTHERWISE, ARISING FROM,
+OUT OF OR IN CONNECTION WITH THE SOFTWARE OR THE USE OR OTHER DEALINGS IN
+THE SOFTWARE.

diff -r 000000000000 -r 1d773da0ccf0 tools/seq_filter_by_mapping/seq_filter_by_mapping.py
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/tools/seq_filter_by_mapping/seq_filter_by_mapping.py Tue Jan 27 08:31:13 2015 -0500

[

b'@@ -0,0 +1,370 @@\n+#!/usr/bin/env python\n+"""Filter a FASTA, FASTQ or SSF file with SAM/BAM mapping information.\n+\n+When filtering an SFF file, any Roche XML manifest in the input file is\n+preserved in both output files.\n+\n+This tool is a short Python script which requires Biopython 1.54 or later\n+for SFF file support. If you use this tool in scientific work leading to a\n+publication, please cite the Biopython application note:\n+\n+Cock et al 2009. Biopython: freely available Python tools for computational\n+molecular biology and bioinformatics. Bioinformatics 25(11) 1422-3.\n+http://dx.doi.org/10.1093/bioinformatics/btp163 pmid:19304878.\n+\n+This script is copyright 2014 by Peter Cock, The James Hutton Institute\n+(formerly the Scottish Crop Research Institute, SCRI), UK. All rights reserved.\n+See accompanying text file for licence details (MIT license).\n+\n+Use -v or --version to get the version, -h or --help for help.\n+"""\n+import os\n+import sys\n+import re\n+import subprocess\n+from optparse import OptionParser\n+\n+def sys_exit(msg, err=1):\n+ sys.stderr.write(msg.rstrip() + "\\n")\n+ sys.exit(err)\n+\n+#Parse Command Line\n+usage = """Use as follows:\n+\n+$ python seq_filter_by_mapping.py [options] mapping.sam/bam [more mappings]\n+\n+e.g. Positive matches using column one from a single BAM file:\n+\n+$ seq_filter_by_mapping.py -i my_seqs.fastq -f fastq -p matches.fastq mapping.bam\n+\n+Multiple SAM/BAM mapping files may be given.\n+"""\n+parser = OptionParser(usage=usage)\n+parser.add_option(\'-i\', \'--input\', dest=\'input\',\n+ default=None, help=\'Input sequences filename\',\n+ metavar="FILE")\n+parser.add_option(\'-f\', \'--format\', dest=\'format\',\n+ default=None,\n+ help=\'Input sequence format (e.g. fasta, fastq, sff)\')\n+parser.add_option(\'-p\', \'--positive\', dest=\'output_positive\',\n+ default=None,\n+ help=\'Output filename for mapping reads\',\n+ metavar="FILE")\n+parser.add_option(\'-n\', \'--negative\', dest=\'output_negative\',\n+ default=None,\n+ help=\'Output filename for non-mapping reads\',\n+ metavar="FILE")\n+parser.add_option("-m", "--pair-mode", dest="pair_mode",\n+ default="lax",\n+ help="How to treat paired reads (lax or strict, default lax)")\n+parser.add_option("-v", "--version", dest="version",\n+ default=False, action="store_true",\n+ help="Show version and quit")\n+\n+options, args = parser.parse_args()\n+\n+if options.version:\n+ print "v0.0.2"\n+ sys.exit(0)\n+\n+in_file = options.input\n+seq_format = options.format\n+out_positive_file = options.output_positive\n+out_negative_file = options.output_negative\n+pair_mode = options.pair_mode\n+\n+if in_file is None or not os.path.isfile(in_file):\n+ sys_exit("Missing input file: %r" % in_file)\n+if out_positive_file is None and out_negative_file is None:\n+ sys_exit("Neither output file requested")\n+if seq_format is None:\n+ sys_exit("Missing sequence format")\n+if pair_mode not in ["lax", "strict"]:\n+ sys_exit("Pair mode argument should be \'lax\' or \'strict\', not %r" % pair_mode)\n+for mapping in args:\n+ if not os.path.isfile(mapping):\n+ sys_exit("Mapping file %r not found" % mapping)\n+if not args:\n+ sys_exit("At least one SAM/BAM mapping file is required")\n+\n+\n+#Cope with three widely used suffix naming convensions,\n+#Illumina: /1 or /2\n+#Forward/revered: .f or .r\n+#Sanger, e.g. .p1k and .q1k\n+#See http://staden.sourceforge.net/manual/pregap4_unix_50.html\n+#re_f = re.compile(r"(/1|\\.f|\\.[sfp]\\d\\w*)$")\n+#re_r = re.compile(r"(/2|\\.r|\\.[rq]\\d\\w*)$")\n+re_suffix = re.compile(r"(/1|\\.f|\\.[sfp]\\d\\w*|/2|\\.r|\\.[rq]\\d\\w*)$")\n+assert re_suffix.search("demo.f")\n+assert re_suffix.search("demo.s1")\n+assert re_suffix.search("demo.f1k")\n+assert re_suffix.search("demo.p1")\n+assert re_suffix.search("demo.p1k")\n+assert re_suffix.search("demo.p1lk")\n+assert re_suffix.search("demo/'..b'None:\n+ print "Generating two FASTQ files"\n+ positive_handle = open(out_positive_file, "w")\n+ negative_handle = open(out_negative_file, "w")\n+ print in_file\n+ for title, seq, qual in FastqGeneralIterator(handle):\n+ # print("%s --> %s" % (title, clean_name(title.split(None, 1)[0])))\n+ if clean_name(title.split(None, 1)[0]) in ids:\n+ positive_handle.write("@%s\\n%s\\n+\\n%s\\n" % (title, seq, qual))\n+ else:\n+ negative_handle.write("@%s\\n%s\\n+\\n%s\\n" % (title, seq, qual))\n+ positive_handle.close()\n+ negative_handle.close()\n+ elif out_positive_file is not None:\n+ print "Generating matching FASTQ file"\n+ positive_handle = open(out_positive_file, "w")\n+ for title, seq, qual in FastqGeneralIterator(handle):\n+ if clean_name(title.split(None, 1)[0]) in ids:\n+ positive_handle.write("@%s\\n%s\\n+\\n%s\\n" % (title, seq, qual))\n+ positive_handle.close()\n+ elif out_negative_file is not None:\n+ print "Generating non-matching FASTQ file"\n+ negative_handle = open(out_negative_file, "w")\n+ for title, seq, qual in FastqGeneralIterator(handle):\n+ if clean_name(title.split(None, 1)[0]) not in ids:\n+ negative_handle.write("@%s\\n%s\\n+\\n%s\\n" % (title, seq, qual))\n+ negative_handle.close()\n+ handle.close()\n+ # This does not currently bother to record record counts (faster)\n+\n+def sff_filter(in_file, pos_file, neg_file, wanted):\n+ """SFF filter."""\n+ try:\n+ from Bio.SeqIO.SffIO import SffIterator, SffWriter\n+ except ImportError:\n+ sys_exit("SFF filtering requires Biopython 1.54 or later")\n+\n+ try:\n+ from Bio.SeqIO.SffIO import ReadRocheXmlManifest\n+ except ImportError:\n+ #Prior to Biopython 1.56 this was a private function\n+ from Bio.SeqIO.SffIO import _sff_read_roche_index_xml as ReadRocheXmlManifest\n+\n+ in_handle = open(in_file, "rb") #must be binary mode!\n+ try:\n+ manifest = ReadRocheXmlManifest(in_handle)\n+ except ValueError:\n+ manifest = None\n+\n+ #This makes two passes though the SFF file with isn\'t so efficient,\n+ #but this makes the code simple.\n+ pos_count = neg_count = 0\n+ if out_positive_file is not None:\n+ out_handle = open(out_positive_file, "wb")\n+ writer = SffWriter(out_handle, xml=manifest)\n+ in_handle.seek(0) #start again after getting manifest\n+ pos_count = writer.write_file(rec for rec in SffIterator(in_handle) if clean_name(rec.id) in ids)\n+ out_handle.close()\n+ if out_negative_file is not None:\n+ out_handle = open(out_negative_file, "wb")\n+ writer = SffWriter(out_handle, xml=manifest)\n+ in_handle.seek(0) #start again\n+ neg_count = writer.write_file(rec for rec in SffIterator(in_handle) if clean_name(rec.id) not in ids)\n+ out_handle.close()\n+ #And we\'re done\n+ in_handle.close()\n+ return pos_count, neg_count\n+\n+\n+if seq_format.lower()=="sff":\n+ # Now write filtered SFF file based on IDs wanted\n+ pos_count, neg_count = sff_filter(in_file, out_positive_file, out_negative_file, ids)\n+ # At the time of writing, Galaxy doesn\'t show SFF file read counts,\n+ # so it is useful to put them in stdout and thus shown in job info.\n+ print "%i with and %i without specified IDs" % (pos_count, neg_count)\n+elif seq_format.lower()=="fasta":\n+ # Write filtered FASTA file based on IDs from tabular file\n+ pos_count, neg_count = fasta_filter(in_file, out_positive_file, out_negative_file, ids)\n+ print "%i with and %i without specified IDs" % (pos_count, neg_count)\n+elif seq_format.lower().startswith("fastq"):\n+ #Write filtered FASTQ file based on IDs from mapping file\n+ fastq_filter(in_file, out_positive_file, out_negative_file, ids)\n+ # This does not currently track the counts\n+else:\n+ sys_exit("Unsupported file type %r" % seq_format)\n'

diff -r 000000000000 -r 1d773da0ccf0 tools/seq_filter_by_mapping/seq_filter_by_mapping.xml
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/tools/seq_filter_by_mapping/seq_filter_by_mapping.xml Tue Jan 27 08:31:13 2015 -0500

[

@@ -0,0 +1,113 @@
+<tool id="seq_filter_by_mapping" name="Filter sequences by mapping" version="0.0.2">
+    <description>from SAM/BAM file</description>
+    <requirements>
+        <requirement type="package" version="1.64">biopython</requirement>
+        <requirement type="python-module">Bio</requirement>
+        <requirement type="binary">samtools</requirement>
+        <requirement type="package" version="0.1.19">samtools</requirement>
+    </requirements>
+    <version_command interpreter="python">seq_filter_by_mapping.py --version</version_command>
+    <command interpreter="python">
+seq_filter_by_mapping.py -i "$input_file" -f "$input_file.ext" -m $pair_mode
+#if $output_choice_cond.output_choice=="both"
+ -p $output_pos -n $output_neg
+#elif $output_choice_cond.output_choice=="pos"
+ -p $output_pos
+#elif $output_choice_cond.output_choice=="neg"
+ -n $output_neg
+#end if
+## Now loop over all the mapping files
+#for i in $mapping_file#${i} #end for#
+    </command>
+    <stdio>
+        
+        <exit_code range="1:" />
+        <exit_code range=":-1" />
+    </stdio>
+    <inputs>
+        <param name="input_file" type="data" format="fasta,fastq,sff" label="Sequence file to be filtered" help="FASTA, FASTQ, or SFF format." />
+ <param name="mapping_file" type="data" format="sam,bam" multiple="true" label="SAM/BAM mapping of those sequences" help="SAM or BAM format." />
+        <conditional name="output_choice_cond">
+            <param name="output_choice" type="select" label="Output mapped reads, unmapped reads, or both?">
+                <option value="both">Both mapped and unmapped reads, as two files</option>
+                <option value="pos">Just mapped reads, as a single file</option>
+                <option value="neg">Just unmapped reads, as a single file</option>
+            </param>
+            
+            <when value="both" />
+            <when value="pos" />
+            <when value="neg" />
+        </conditional>
+ <param name="pair_mode" type="select" label="Paired read treatment">
+            <option value="lax" selected="true">Treat as a pair, allow either read to be mapped</option>
+     <option value="strict">Treat as a pair, require both reads to be mapped</option>
+     
+        </param>
+    </inputs>
+    <outputs>
+        <data name="output_pos" format="input" metadata_source="input_file" label="$input_file.name (mapped)">
+            <filter>output_choice_cond["output_choice"] != "neg"</filter>
+        </data>
+        <data name="output_neg" format="input" metadata_source="input_file" label="$input_file.name (unmapped)">
+            <filter>output_choice_cond["output_choice"] != "pos"</filter>
+        </data>
+    </outputs>
+    <tests>
+ <test>
+            <param name="input_file" value="SRR639755_mito_pairs.fastq.gz" ftype="fastqsanger" />
+            <param name="mapping_file" value="SRR639755_sample_by_coord.sam" ftype="sam" />
+            <param name="pair_mode" value="lax" />
+            <param name="output_choice" value="pos" />
+            <output name="output_pos" file="SRR639755_sample_lax.fastq" ftype="fastqsanger" />
+        </test>
+ <test>
+            <param name="input_file" value="SRR639755_mito_pairs.fastq.gz" ftype="fastqsanger" />
+            <param name="mapping_file" value="SRR639755_sample_by_coord.sam" ftype="sam" />
+            <param name="pair_mode" value="strict" />
+            <param name="output_choice" value="pos" />
+            <output name="output_pos" file="SRR639755_sample_strict.fastq" ftype="fastqsanger" />
+        </test>
+    </tests>
+    <help>
+**What it does**
+
+By default it divides a FASTA, FASTQ or Standard Flowgram Format (SFF) file in
+two, those sequences (or read pairs) which do or don't map in the provided
+SAM/BAM file. You can opt to have a single output file of just the mapping reads,
+or just the non-mapping ones.
+
+**Example Usage**
+
+You might wish to perform a contamination screan by mapping your reads against
+known contaminant reference sequences, then use this tool to select only the
+unmapped reads for further analysis (e.g. *de novo* assembly).
+
+Similarly you might wish to map your reads against a known bacterial reference,
+then take the non-mapping sequences forward for analysis if looking for novel
+plasmids.
+
+
+**References**
+
+If you use this Galaxy tool in work leading to a scientific publication please
+cite:
+
+Peter J.A. Cock (2014), Galaxy tool for filtering reads by mapping
+http://toolshed.g2.bx.psu.edu/view/peterjc/seq_filter_by_mapping
+
+This tool uses Biopython to read and write SFF files, so you may also wish to
+cite the Biopython application note (and Galaxy too of course):
+
+Cock et al (2009). Biopython: freely available Python tools for computational
+molecular biology and bioinformatics. Bioinformatics 25(11) 1422-3.
+http://dx.doi.org/10.1093/bioinformatics/btp163 pmid:19304878.
+
+This tool is available to install into other Galaxy Instances via the Galaxy
+Tool Shed at http://toolshed.g2.bx.psu.edu/view/peterjc/seq_filter_by_mapping
+    </help>
+    <citations>
+        <citation type="doi">10.1093/bioinformatics/btp163</citation>
+    </citations>
+</tool>

diff -r 000000000000 -r 1d773da0ccf0 tools/seq_filter_by_mapping/tool_dependencies.xml
--- /dev/null Thu Jan 01 00:00:00 1970 +0000
+++ b/tools/seq_filter_by_mapping/tool_dependencies.xml Tue Jan 27 08:31:13 2015 -0500

@@ -0,0 +1,9 @@
+<?xml version="1.0"?>
+<tool_dependency>
+    <package name="biopython" version="1.64">
+        <repository changeset_revision="5477a05cc158" name="package_biopython_1_64" owner="biopython" toolshed="https://toolshed.g2.bx.psu.edu" />
+    </package>
+    <package name="samtools" version="0.1.19">
+        <repository changeset_revision="923adc89c666" name="package_samtools_0_1_19" owner="iuc" toolshed="https://toolshed.g2.bx.psu.edu" />
+    </package>
+</tool_dependency>