Mercurial > repos > devteam > cuffmerge
view cuffmerge_wrapper.py @ 3:3ed34b8bddfc draft
planemo upload for repository https://github.com/galaxyproject/tools-devteam/tree/master/tool_collections/cufflinks/cuffmerge commit 82ee6fc860c52c531b7a57bbb346ab1a67a434a5
| author | devteam |
|---|---|
| date | Sun, 19 Feb 2017 12:11:53 -0500 |
| parents | 0ed8b7f6d506 |
| children |
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#!/usr/bin/env python import optparse import os import shutil import subprocess import sys import tempfile def stop_err(msg): sys.stderr.write('%s\n' % msg) sys.exit() def __main__(): parser = optparse.OptionParser() parser.add_option('-g', dest='ref_annotation', help='An optional "reference" annotation GTF. Each sample is matched against this file, and sample isoforms are tagged as overlapping, matching, or novel where appropriate. See the refmap and tmap output file descriptions below.') parser.add_option('-s', dest='use_seq_data', action="store_true", help='Causes cuffmerge to look into for fasta files with the underlying genomic sequences (one file per contig) against which your reads were aligned for some optional classification functions. For example, Cufflinks transcripts consisting mostly of lower-case bases are classified as repeats. Note that <seq_dir> must contain one fasta file per reference chromosome, and each file must be named after the chromosome, and have a .fa or .fasta extension.') parser.add_option('-p', '--num-threads', dest='num_threads', help='Use this many threads to align reads. The default is 1.') # Wrapper / Galaxy options. parser.add_option('', '--index', dest='index', help='The path of the reference genome') parser.add_option('', '--ref_file', dest='ref_file', help='The reference dataset from the history') # Outputs. parser.add_option('', '--merged-transcripts', dest='merged_transcripts') parser.add_option('--min-isoform-fraction', dest='min_isoform_fraction') (options, args) = parser.parse_args() # Set/link to sequence file. if options.use_seq_data: if options.ref_file: # Sequence data from history. # Create symbolic link to ref_file so that index will be created in working directory. seq_path = "ref.fa" os.symlink(options.ref_file, seq_path) else: if not os.path.exists(options.index): stop_err('Reference genome %s not present, request it by reporting this error.' % options.index) seq_path = options.index # Build command. # Base. cmd = "cuffmerge -o cm_output " # Add options. if options.num_threads: cmd += (" -p %i " % int(options.num_threads)) if options.ref_annotation: cmd += " -g %s " % options.ref_annotation if options.use_seq_data: cmd += " -s %s " % seq_path if options.min_isoform_fraction: cmd += " --min-isoform-fraction %s " % (options.min_isoform_fraction) # Add input files to a file. with tempfile.NamedTemporaryFile(mode='w', dir=".", delete=False) as inputs_file: for arg in args: inputs_file.write(arg + "\n") cmd += inputs_file.name # Run command. try: with tempfile.NamedTemporaryFile(dir=".") as tmp_stderr: returncode = subprocess.call(args=cmd, stderr=tmp_stderr, shell=True) # Error checking. if returncode != 0: # Get stderr, allowing for case where it's very large. buffsize = 1048576 stderr = '' with open(tmp_stderr.name, 'r') as tmp_stderr2: try: while True: stderr += tmp_stderr2.read(buffsize) if not stderr or len(stderr) % buffsize != 0: break except OverflowError: pass raise Exception(stderr) if len(open("cm_output/merged.gtf", 'r').read().strip()) == 0: raise Exception('The output file is empty, there may be an error with your input file or settings.') # Copy outputs. shutil.move("cm_output/merged.gtf", options.merged_transcripts) except Exception as e: stop_err('Error running cuffmerge: %s' % e) if __name__ == "__main__": __main__()