# HG changeset patch # User peterjc # Date 1307481848 14400 # Node ID d570cc3247797f5f1b5d807680c374ac145214d4 # Parent b79caa511ba269343a0a6d63826ba6380782e7f7 Migrated tool version 0.0.4 from old tool shed archive to new tool shed repository diff -r b79caa511ba2 -r d570cc324779 tools/fastq/fastq_filter_by_id.py --- a/tools/fastq/fastq_filter_by_id.py Tue Jun 07 17:23:49 2011 -0400 +++ b/tools/fastq/fastq_filter_by_id.py Tue Jun 07 17:24:08 2011 -0400 @@ -1,6 +1,9 @@ #!/usr/bin/env python """Filter a FASTQ file with IDs from a tabular file, e.g. from BLAST. +NOTE - This script is now OBSOLETE, having been replaced by a new verion +which handles FASTA, FASTQ and SFF all in one. + Takes five command line options, tabular filename, ID column numbers (comma separated list using one based counting), input FASTA filename, and two output FASTA filenames (for records with and without the given IDs). @@ -13,10 +16,10 @@ in column one, and the ID of the match from the database is in column two. Here sensible values for the column numbers would therefore be "1" or "2". -This script is copyright 2010 by Peter Cock, SCRI, UK. All rights reserved. +This script is copyright 2010-2011 by Peter Cock, SCRI, UK. All rights reserved. See accompanying text file for licence details (MIT/BSD style). -This is version 0.0.2 of the script. +This is version 0.0.4 of the script. """ import sys from galaxy_utils.sequence.fastq import fastqReader, fastqWriter @@ -86,7 +89,6 @@ #The [1:] is because the fastaReader leaves the @ on the identifer. if not record.identifier or record.identifier.split()[0][1:] not in ids: negative_writer.write(record) - positive_writer.close() negative_writer.close() else: stop_err("Neither output file requested") diff -r b79caa511ba2 -r d570cc324779 tools/fastq/fastq_filter_by_id.txt --- a/tools/fastq/fastq_filter_by_id.txt Tue Jun 07 17:23:49 2011 -0400 +++ b/tools/fastq/fastq_filter_by_id.txt Tue Jun 07 17:24:08 2011 -0400 @@ -1,3 +1,11 @@ +Obsolete +======== + +This tool is now obsolete, having been replaced by a more general version +covering the FASTA, FASTQ and SFF sequence formats in a single tool. You +should only install this tool if you need to support existing workflows +which used it. + Galaxy tool to filter FASTQ sequences by ID =========================================== @@ -33,13 +41,17 @@ v0.0.1 - Initial verion (not publicly released) v0.0.2 - Allow both, just pos or just neg output files - Preserve the FASTQ variant in the XML wrapper +v0.0.3 - Fixed bug when generating non-matching FASTQ file only +v0.0.4 - Deprecated, marked as hidden in the XML Developers ========== -This script and similar versions for FASTA and SFF files are currently being -developed on the following hg branch: +This script and related tools are being developed on the following hg branch: +http://bitbucket.org/peterjc/galaxy-central/src/tools + +This incorporates the previously used hg branch: http://bitbucket.org/peterjc/galaxy-central/src/fasta_filter For making the "Galaxy Tool Shed" http://community.g2.bx.psu.edu/ tarball use diff -r b79caa511ba2 -r d570cc324779 tools/fastq/fastq_filter_by_id.xml --- a/tools/fastq/fastq_filter_by_id.xml Tue Jun 07 17:23:49 2011 -0400 +++ b/tools/fastq/fastq_filter_by_id.xml Tue Jun 07 17:24:08 2011 -0400 @@ -1,4 +1,4 @@ - +