Mercurial > repos > peterjc > tmhmm_and_signalp
view tools/protein_analysis/signalp3.py @ 10:09ff180d1615 draft
Uploaded v0.1.3 with missing HMM file for RXLR tool included.
author | peterjc |
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date | Wed, 27 Mar 2013 11:21:05 -0400 |
parents | e52220a9ddad |
children | 99b82a2b1272 |
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#!/usr/bin/env python """Wrapper for SignalP v3.0 for use in Galaxy. This script takes exactly five command line arguments: * the organism type (euk, gram+ or gram-) * length to truncate sequences to (integer) * number of threads to use (integer, defaults to one) * an input protein FASTA filename * output tabular filename. There are two further optional arguments * cut type (NN_Cmax, NN_Ymax, NN_Smax or HMM_Cmax) * output GFF3 filename It then calls the standalone SignalP v3.0 program (not the webservice) requesting the short output (one line per protein) using both NN and HMM for predictions. First major feature is cleaning up the output. The raw output from SignalP v3.0 looks like this (21 columns space separated): # SignalP-NN euk predictions # SignalP-HMM euk predictions # name Cmax pos ? Ymax pos ? Smax pos ? Smean ? D ? # name ! Cmax pos ? Sprob ? gi|2781234|pdb|1JLY| 0.061 17 N 0.043 17 N 0.199 1 N 0.067 N 0.055 N gi|2781234|pdb|1JLY|B Q 0.000 17 N 0.000 N gi|4959044|gb|AAD342 0.099 191 N 0.012 38 N 0.023 12 N 0.014 N 0.013 N gi|4959044|gb|AAD34209.1|AF069992_1 Q 0.000 0 N 0.000 N gi|671626|emb|CAA856 0.139 381 N 0.020 8 N 0.121 4 N 0.067 N 0.044 N gi|671626|emb|CAA85685.1| Q 0.000 0 N 0.000 N gi|3298468|dbj|BAA31 0.208 24 N 0.184 38 N 0.980 32 Y 0.613 Y 0.398 N gi|3298468|dbj|BAA31520.1| Q 0.066 24 N 0.139 N In order to make it easier to use in Galaxy, this wrapper script reformats this to use tab separators. Also it removes the redundant truncated name column, and assigns unique column names in the header: #ID NN_Cmax_score NN_Cmax_pos NN_Cmax_pred NN_Ymax_score NN_Ymax_pos NN_Ymax_pred NN_Smax_score NN_Smax_pos NN_Smax_pred NN_Smean_score NN_Smean_pred NN_D_score NN_D_pred HMM_bang HMM_Cmax_score HMM_Cmax_pos HMM_Cmax_pred HMM_Sprob_score HMM_Sprob_pred gi|2781234|pdb|1JLY|B 0.061 17 N 0.043 17 N 0.199 1 N 0.067 N 0.055 N Q 0.000 17 N 0.000 N gi|4959044|gb|AAD34209.1|AF069992_1 0.099 191 N 0.012 38 N 0.023 12 N 0.014 N 0.013 N Q 0.000 0 N 0.000 N gi|671626|emb|CAA85685.1| 0.139 381 N 0.020 8 N 0.121 4 N 0.067 N 0.044 N Q 0.000 0 N 0.000 N gi|3298468|dbj|BAA31520.1| 0.208 24 N 0.184 38 N 0.980 32 Y 0.613 Y 0.398 N Q 0.066 24 N 0.139 N The second major feature is overcoming SignalP's built in limit of 4000 sequences by breaking up the input FASTA file into chunks. This also allows us to pre-trim the sequences since SignalP only needs their starts. The third major feature is taking advantage of multiple cores (since SignalP v3.0 itself is single threaded) by using the individual FASTA input files to run multiple copies of TMHMM in parallel. I would normally use Python's multiprocessing library in this situation but it requires at least Python 2.6 and at the time of writing Galaxy still supports Python 2.4. Note that this is somewhat redundant with job-splitting available in Galaxy itself (see the SignalP XML file for settings). Finally, you can opt to have a GFF3 file produced which will describe the predicted signal peptide and mature peptide for each protein (using one of the predictors which gives a cleavage site). *WORK IN PROGRESS* """ import sys import os import tempfile from seq_analysis_utils import stop_err, split_fasta, fasta_iterator from seq_analysis_utils import run_jobs, thread_count FASTA_CHUNK = 500 MAX_LEN = 6000 #Found by trial and error if len(sys.argv) not in [6,8]: stop_err("Require five (or 7) arguments, organism, truncate, threads, " "input protein FASTA file & output tabular file (plus " "optionally cut method and GFF3 output file). " "Got %i arguments." % (len(sys.argv)-1)) organism = sys.argv[1] if organism not in ["euk", "gram+", "gram-"]: stop_err("Organism argument %s is not one of euk, gram+ or gram-" % organism) try: truncate = int(sys.argv[2]) except: truncate = 0 if truncate < 0: stop_err("Truncate argument %s is not a positive integer (or zero)" % sys.argv[2]) num_threads = thread_count(sys.argv[3], default=4) fasta_file = sys.argv[4] tabular_file = sys.argv[5] if len(sys.argv) == 8: cut_method = sys.argv[6] if cut_method not in ["NN_Cmax", "NN_Ymax", "NN_Smax", "HMM_Cmax"]: stop_err("Invalid cut method %r" % cut_method) gff3_file = sys.argv[7] else: cut_method = None gff3_file = None tmp_dir = tempfile.mkdtemp() def clean_tabular(raw_handle, out_handle, gff_handle=None, cut_method=None): """Clean up SignalP output to make it tabular.""" if cut_method: cut_col = {"NN_Cmax" : 2, "NN_Ymax" : 5, "NN_Smax" : 8, "HMM_Cmax" : 16}[cut_method] else: cut_col = None for line in raw_handle: if not line or line.startswith("#"): continue parts = line.rstrip("\r\n").split() assert len(parts)==21, repr(line) assert parts[14].startswith(parts[0]) #Remove redundant truncated name column (col 0) #and put full name at start (col 14) parts = parts[14:15] + parts[1:14] + parts[15:] out_handle.write("\t".join(parts) + "\n") def make_gff(fasta_file, tabular_file, gff_file, cut_method): cut_col, score_col = {"NN_Cmax" : (2,1), "NN_Ymax" : (5,4), "NN_Smax" : (8,7), "HMM_Cmax" : (16,15), }[cut_method] source = "SignalP" strand = "." #not stranded phase = "." #not phased tags = "Note=%s" % cut_method tab_handle = open(tabular_file) line = tab_handle.readline() assert line.startswith("#ID\t"), line gff_handle = open(gff_file, "w") gff_handle.write("##gff-version 3\n") for (title, seq), line in zip(fasta_iterator(fasta_file), tab_handle): parts = line.rstrip("\n").split("\t") seqid = parts[0] assert title.startswith(seqid), "%s vs %s" % (seqid, title) if len(seq)==0: #Is it possible to have a zero length reference in GFF3? continue cut = int(parts[cut_col]) if cut == 0: assert cut_method == "HMM_Cmax", cut_method #TODO - Why does it do this? cut = 1 assert 1 <= cut <= len(seq), "%i for %s len %i" % (cut, seqid, len(seq)) score = parts[score_col] gff_handle.write("##sequence-region %s %i %i\n" \ % (seqid, 1, len(seq))) #If the cut is at the very begining, there is no signal peptide! if cut > 1: #signal_peptide = SO:0000418 gff_handle.write("%s\t%s\t%s\t%i\t%i\t%s\t%s\t%s\t%s\n" \ % (seqid, source, "signal_peptide", 1, cut-1, score, strand, phase, tags)) #mature_protein_region = SO:0000419 gff_handle.write("%s\t%s\t%s\t%i\t%i\t%s\t%s\t%s\t%s\n" \ % (seqid, source, "mature_protein_region", cut, len(seq), score, strand, phase, tags)) tab_handle.close() gff_handle.close() fasta_files = split_fasta(fasta_file, os.path.join(tmp_dir, "signalp"), n=FASTA_CHUNK, truncate=truncate, max_len=MAX_LEN) temp_files = [f+".out" for f in fasta_files] assert len(fasta_files) == len(temp_files) jobs = ["signalp -short -t %s %s > %s" % (organism, fasta, temp) for (fasta, temp) in zip(fasta_files, temp_files)] assert len(fasta_files) == len(temp_files) == len(jobs) def clean_up(file_list): for f in file_list: if os.path.isfile(f): os.remove(f) try: os.rmdir(tmp_dir) except: pass if len(jobs) > 1 and num_threads > 1: #A small "info" message for Galaxy to show the user. print "Using %i threads for %i tasks" % (min(num_threads, len(jobs)), len(jobs)) results = run_jobs(jobs, num_threads) assert len(fasta_files) == len(temp_files) == len(jobs) for fasta, temp, cmd in zip(fasta_files, temp_files, jobs): error_level = results[cmd] try: output = open(temp).readline() except IOError: output = "(no output)" if error_level or output.lower().startswith("error running"): clean_up(fasta_files + temp_files) stop_err("One or more tasks failed, e.g. %i from %r gave:\n%s" % (error_level, cmd, output), error_level) del results out_handle = open(tabular_file, "w") fields = ["ID"] #NN results: for name in ["Cmax", "Ymax", "Smax"]: fields.extend(["NN_%s_score"%name, "NN_%s_pos"%name, "NN_%s_pred"%name]) fields.extend(["NN_Smean_score", "NN_Smean_pred", "NN_D_score", "NN_D_pred"]) #HMM results: fields.extend(["HMM_type", "HMM_Cmax_score", "HMM_Cmax_pos", "HMM_Cmax_pred", "HMM_Sprob_score", "HMM_Sprob_pred"]) out_handle.write("#" + "\t".join(fields) + "\n") for temp in temp_files: data_handle = open(temp) clean_tabular(data_handle, out_handle) data_handle.close() out_handle.close() #GFF3: if cut_method: make_gff(fasta_file, tabular_file, gff3_file, cut_method) clean_up(fasta_files + temp_files)