Mercurial > repos > galaxyp > translate_bed_sequences
view translate_bed_sequences.py @ 0:d723eb657f1d draft
planemo upload for repository https://github.com/galaxyproteomics/tools-galaxyp/tree/master/tools/translate_bed_sequences commit e04ed4b4960d6109a85c1cc68a2bf4931c8751ef-dirty
| author | galaxyp |
|---|---|
| date | Mon, 25 Jan 2016 12:21:21 -0500 |
| parents | |
| children | 4221664a2bd0 |
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#!/usr/bin/env python """ # #------------------------------------------------------------------------------ # University of Minnesota # Copyright 2014, Regents of the University of Minnesota #------------------------------------------------------------------------------ # Author: # # James E Johnson # #------------------------------------------------------------------------------ """ """ Input: BED file (12 column) + 13th sequence column appended by extract_genomic_dna Output: Fasta of 3-frame translations of the spliced sequence """ import sys,re,os.path import tempfile import optparse from optparse import OptionParser from Bio.Seq import reverse_complement, transcribe, back_transcribe, translate class BedEntry( object ): def __init__(self, line): self.line = line try: fields = line.rstrip('\r\n').split('\t') (chrom,chromStart,chromEnd,name,score,strand,thickStart,thickEnd,itemRgb,blockCount,blockSizes,blockStarts) = fields[0:12] seq = fields[12] if len(fields) > 12 else None self.chrom = chrom self.chromStart = int(chromStart) self.chromEnd = int(chromEnd) self.name = name self.score = int(score) self.strand = strand self.thickStart = int(thickStart) self.thickEnd = int(thickEnd) self.itemRgb = itemRgb self.blockCount = int(blockCount) self.blockSizes = [int(x) for x in blockSizes.split(',')] self.blockStarts = [int(x) for x in blockStarts.split(',')] self.seq = seq except Exception, e: print >> sys.stderr, "Unable to read Bed entry" % e exit(1) def __str__(self): return '%s\t%d\t%d\t%s\t%d\t%s\t%d\t%d\t%s\t%d\t%s\t%s%s' % ( self.chrom, self.chromStart, self.chromEnd, self.name, self.score, self.strand, self.thickStart, self.thickEnd, self.itemRgb, self.blockCount, ','.join([str(x) for x in self.blockSizes]), ','.join([str(x) for x in self.blockStarts]), '\t%s' % self.seq if self.seq else '') def get_splice_junctions(self): splice_juncs = [] for i in range(self.blockCount - 1): splice_junc = "%s:%d_%d" % (self.chrom, self.chromStart + self.blockSizes[i], self.chromStart + self.blockStarts[i+1]) splice_juncs.append(splice_junc) return splice_juncs def get_exon_seqs(self): exons = [] for i in range(self.blockCount): # splice_junc = "%s:%d_%d" % (self.chrom, self.chromStart + self.blockSizes[i], self.chromStart + self.blockStarts[i+1]) exons.append(self.seq[self.blockStarts[i]:self.blockStarts[i] + self.blockSizes[i]]) if self.strand == '-': #reverse complement exons.reverse() for i,s in enumerate(exons): exons[i] = reverse_complement(s) return exons def get_spliced_seq(self): seq = ''.join(self.get_exon_seqs()) return seq def get_translation(self,sequence=None): translation = None seq = sequence if sequence else self.get_spliced_seq() if seq: seqlen = len(seq) / 3 * 3; if seqlen >= 3: translation = translate(seq[:seqlen]) return translation def get_translations(self): translations = [] seq = self.get_spliced_seq() if seq: for i in range(3): translation = self.get_translation(sequence=seq[i:]) if translation: translations.append(translation) return translations ## (start,end) def get_subrange(self,tstart,tstop): chromStart = self.chromStart chromEnd = self.chromEnd r = range(self.blockCount) if self.strand == '-': r.reverse() bStart = 0 for x in r: bEnd = bStart + self.blockSizes[x] if bStart <= tstart < bEnd: if self.strand == '+': chromStart = self.chromStart + self.blockStarts[x] + (tstart - bStart) else: chromEnd = self.chromStart + self.blockStarts[x] + (tstart - bStart) if bStart <= tstop < bEnd: if self.strand == '+': chromEnd = self.chromStart + self.blockStarts[x] + (tstop - bStart) else: chromStart = self.chromStart + self.blockStarts[x] + self.blockSizes[x] - (tstop - bStart) bStart += self.blockSizes[x] return(chromStart,chromEnd) #get the blocks for sub range def get_blocks(self,chromStart,chromEnd): tblockCount = 0 tblockSizes = [] tblockStarts = [] for x in range(self.blockCount): bStart = self.chromStart + self.blockStarts[x] bEnd = bStart + self.blockSizes[x] if bStart > chromEnd: break if bEnd < chromStart: continue cStart = max(chromStart,bStart) tblockStarts.append(cStart - chromStart) tblockSizes.append(min(chromEnd,bEnd) - cStart) tblockCount += 1 ## print >> sys.stderr, "tblockCount: %d tblockStarts: %s tblockSizes: %s" % (tblockCount,tblockStarts,tblockSizes) return (tblockCount,tblockSizes,tblockStarts) ## [(start,end,seq,blockCount,blockSizes,blockStarts),(start,end,seq,blockCount,blockSizes,blockStarts),(start,end,seq,blockCount,blockSizes,blockStarts)] ## filter: ignore translation if stop codon in first exon after ignore_left_bp def get_filterd_translations(self,untrimmed=False,filtering=True,ignore_left_bp=0,ignore_right_bp=0,debug=False): translations = [None,None,None,None,None,None] seq = self.get_spliced_seq() ignore = (ignore_left_bp if self.strand == '+' else ignore_right_bp) / 3 block_sum = sum(self.blockSizes) exon_sizes = [x for x in self.blockSizes] if self.strand == '-': exon_sizes.reverse() splice_sites = [sum(exon_sizes[:x]) / 3 for x in range(1,len(exon_sizes))] if debug: print >> sys.stderr, "splice_sites: %s" % splice_sites junc = splice_sites[0] if len(splice_sites) > 0 else exon_sizes[0] if seq: for i in range(3): translation = self.get_translation(sequence=seq[i:]) if translation: tstart = 0 tstop = len(translation) offset = (block_sum - i) % 3 if debug: print >> sys.stderr, "frame: %d\ttstart: %d tstop: %d offset: %d\t%s" % (i,tstart,tstop,offset,translation) if not untrimmed: tstart = translation.rfind('*',0,junc) + 1 stop = translation.find('*',junc) tstop = stop if stop >= 0 else len(translation) offset = (block_sum - i) % 3 trimmed = translation[tstart:tstop] if debug: print >> sys.stderr, "frame: %d\ttstart: %d tstop: %d offset: %d\t%s" % (i,tstart,tstop,offset,trimmed) if filtering and tstart > ignore: continue #get genomic locations for start and end if self.strand == '+': chromStart = self.chromStart + i + (tstart * 3) chromEnd = self.chromEnd - offset - (len(translation) - tstop) * 3 else: chromStart = self.chromStart + offset + (len(translation) - tstop) * 3 chromEnd = self.chromEnd - i - (tstart * 3) #get the blocks for this translation (tblockCount,tblockSizes,tblockStarts) = self.get_blocks(chromStart,chromEnd) translations[i] = (chromStart,chromEnd,trimmed,tblockCount,tblockSizes,tblockStarts) if debug: print >> sys.stderr, "tblockCount: %d tblockStarts: %s tblockSizes: %s" % (tblockCount,tblockStarts,tblockSizes) # translations[i] = (chromStart,chromEnd,trimmed,tblockCount,tblockSizes,tblockStarts) return translations def get_seq_id(self,seqtype='unk:unk',reference='',frame=None): ## Ensembl fasta ID format # >ID SEQTYPE:STATUS LOCATION GENE TRANSCRIPT # >ENSP00000328693 pep:splice chromosome:NCBI35:1:904515:910768:1 gene:ENSG00000158815:transcript:ENST00000328693 gene_biotype:protein_coding transcript_biotype:protein_coding frame_name = '' chromStart = self.chromStart chromEnd = self.chromEnd strand = 1 if self.strand == '+' else -1 if frame != None: block_sum = sum(self.blockSizes) offset = (block_sum - frame) % 3 frame_name = '_' + str(frame + 1) if self.strand == '+': chromStart += frame chromEnd -= offset else: chromStart += offset chromEnd -= frame location = "chromosome:%s:%s:%s:%s:%s" % (reference,self.chrom,chromStart,chromEnd,strand) seq_id = "%s%s %s %s" % (self.name,frame_name,seqtype,location) return seq_id def get_line(self, start_offset = 0, end_offset = 0): if start_offset or end_offset: s_offset = start_offset if start_offset else 0 e_offset = end_offset if end_offset else 0 if s_offset > self.chromStart: s_offset = self.chromStart chrStart = self.chromStart - s_offset chrEnd = self.chromEnd + e_offset blkSizes = self.blockSizes blkSizes[0] += s_offset blkSizes[-1] += e_offset blkStarts = self.blockStarts for i in range(1,self.blockCount): blkStarts[i] += s_offset items = [str(x) for x in [self.chrom,chrStart,chrEnd,self.name,self.score,self.strand,self.thickStart,self.thickEnd,self.itemRgb,self.blockCount,','.join([str(x) for x in blkSizes]),','.join([str(x) for x in blkStarts])]] return '\t'.join(items) + '\n' return self.line def __main__(): #Parse Command Line parser = optparse.OptionParser() parser.add_option( '-i', '--input', dest='input', help='BED file (tophat junctions.bed) with sequence column added' ) parser.add_option( '-o', '--output', dest='output', help='Translations of spliced sequence') parser.add_option( '-b', '--bed_format', dest='bed_format', action='store_true', default=False, help='Append translations to bed file instead of fasta' ) parser.add_option( '-D', '--fa_db', dest='fa_db', default=None, help='Prefix DB identifier for fasta ID line, e.g. generic' ) parser.add_option( '-s', '--fa_sep', dest='fa_sep', default='|', help='fasta ID separator defaults to pipe char, e.g. generic|ProtID|description' ) parser.add_option( '-B', '--bed', dest='bed', default=None, help='Output a bed file with added 13th column having translation' ) parser.add_option( '-G', '--gff3', dest='gff', default=None, help='Output translations to a GFF3 file' ) parser.add_option( '-S', '--seqtype', dest='seqtype', default='pep:splice', help='SEQTYPE:STATUS for fasta ID line' ) parser.add_option( '-P', '--id_prefix', dest='id_prefix', default='', help='prefix for the sequence ID' ) parser.add_option( '-R', '--reference', dest='reference', default=None, help='Genome Reference Name for fasta ID location ' ) parser.add_option( '-r', '--refsource', dest='refsource', default=None, help='Source for Genome Reference, e.g. Ensembl, UCSC, or NCBI' ) parser.add_option( '-Q', '--score_name', dest='score_name', default=None, help='include in the fasta ID line score_name:score ' ) parser.add_option( '-l', '--leading_bp', dest='leading_bp', type='int', default=None, help='leading number of base pairs to ignore when filtering' ) parser.add_option( '-t', '--trailing_bp', dest='trailing_bp', type='int', default=None, help='trailing number of base pairs to ignore when filtering' ) parser.add_option( '-U', '--unfiltered', dest='filtering', action='store_false', default=True, help='Do NOT filterout translation with stop codon in the first exon' ) parser.add_option( '-u', '--untrimmed', dest='untrimmed', action='store_true', default=False, help='Do NOT trim from splice site to stop codon' ) parser.add_option( '-L', '--min_length', dest='min_length', type='int', default=None, help='Minimun length (to first stop codon)' ) parser.add_option( '-M', '--max_stop_codons', dest='max_stop_codons', type='int', default=None, help='Filter out translations with more than max_stop_codons' ) parser.add_option( '-d', '--debug', dest='debug', action='store_true', default=False, help='Turn on wrapper debugging to stdout' ) (options, args) = parser.parse_args() # Input files if options.input != None: try: inputPath = os.path.abspath(options.input) inputFile = open(inputPath, 'r') except Exception, e: print >> sys.stderr, "failed: %s" % e exit(2) else: inputFile = sys.stdin # Output files bed_fh = None gff_fh = None gff_fa_file = None gff_fa = None outFile = None if options.output == None: #write to stdout outFile = sys.stdout if options.gff: gff_fa_file = tempfile.NamedTemporaryFile(prefix='gff_fasta_',suffix=".fa",dir=os.getcwd()).name gff_fa = open(gff_fa_file,'w') else: try: outPath = os.path.abspath(options.output) outFile = open(outPath, 'w') except Exception, e: print >> sys.stderr, "failed: %s" % e exit(3) if options.gff: gff_fa_file = outPath if options.bed: bed_fh = open(options.bed,'w') bed_fh.write('track name="%s" description="%s" \n' % ('novel_junctioni_translations','test')) if options.gff: gff_fh = open(options.gff,'w') gff_fh.write("##gff-version 3.2.1\n") if options.reference: gff_fh.write("##genome-build %s %s\n" % (options.refsource if options.refsource else 'unknown', options.reference)) leading_bp = 0 trailing_bp = 0 if options.leading_bp: if options.leading_bp >= 0: leading_bp = options.leading_bp else: print >> sys.stderr, "failed: leading_bp must be positive" exit(5) if options.trailing_bp: if options.trailing_bp >= 0: trailing_bp = options.trailing_bp else: print >> sys.stderr, "failed: trailing_bp must be positive" exit(5) # Scan bed file try: for i, line in enumerate( inputFile ): if line.startswith('track'): if outFile and options.bed_format: outFile.write(line) continue entry = BedEntry(line) strand = 1 if entry.strand == '+' else -1 translations = entry.get_translations() if options.debug: exon_seqs = entry.get_exon_seqs() exon_sizes = [len(seq) for seq in exon_seqs] splice_sites = [sum(exon_sizes[:x]) / 3 for x in range(1,len(exon_sizes))] print >> sys.stderr, entry.name print >> sys.stderr, line.rstrip('\r\n') print >> sys.stderr, "exons: %s" % exon_seqs print >> sys.stderr, "%s" % splice_sites for i,translation in enumerate(translations): print >> sys.stderr, "frame %d: %s" % (i+1,translation) print >> sys.stderr, "splice: %s" % (''.join(['^' if (((j*3)+i)/3) in splice_sites else '-' for j in range(len(translation))])) print >> sys.stderr, "" if options.bed_format: tx_entry = "%s\t%s\n" % (line.rstrip('\r\n'),'\t'.join(translations)) outFile.write(tx_entry) else: translations = entry.get_filterd_translations(untrimmed=options.untrimmed,filtering=options.filtering,ignore_left_bp=leading_bp,ignore_right_bp=trailing_bp,debug=options.debug) for i,tx in enumerate(translations): if tx: (chromStart,chromEnd,translation,blockCount,blockSizes,blockStarts) = tx if options.min_length != None and len(translation) < options.min_length: continue if options.max_stop_codons != None and translation.count('*') > options.max_stop_codons: continue frame_name = '_%s' % (i + 1) pep_id = "%s%s%s" % (options.id_prefix,entry.name,frame_name) if bed_fh: bed_fh.write('%s\t%d\t%d\t%s\t%d\t%s\t%d\t%d\t%s\t%d\t%s\t%s\t%s\n' % (str(entry.chrom),chromStart,chromEnd,pep_id,entry.score,entry.strand,chromStart,chromEnd,entry.itemRgb,blockCount,','.join([str(x) for x in blockSizes]),','.join([str(x) for x in blockStarts]),translation)) location = "chromosome:%s:%s:%s:%s:%s" % (options.reference,entry.chrom,chromStart,chromEnd,strand) score = " %s:%s" % (options.score_name,entry.score) if options.score_name else '' seq_description = "%s %s%s" % (options.seqtype, location, score) seq_id = "%s " % pep_id if options.fa_db: seq_id = "%s%s%s%s" % (options.fa_db,options.fa_sep,pep_id,options.fa_sep) fa_id = "%s%s" % (seq_id,seq_description) fa_entry = ">%s\n%s\n" % (fa_id,translation) outFile.write(fa_entry) if gff_fh: if gff_fa: gff_fa.write(fa_entry) gff_fh.write("##sequence-region %s %d %d\n" % (entry.chrom,chromStart + 1,chromEnd - 1)) gff_fh.write("%s\t%s\t%s\t%s\t%s\t%s\t%s\t%d\tID=%s\n" % (entry.chrom,'splice_junc','gene',chromStart + 1,chromEnd - 1,entry.score,entry.strand,0,pep_id)) for x in range(blockCount): start = chromStart+blockStarts[x] + 1 end = start + blockSizes[x] - 1 phase = (3 - sum(blockSizes[:x]) % 3) % 3 gff_fh.write("%s\t%s\t%s\t%s\t%s\t%s\t%s\t%d\tParent=%s;ID=%s_%d\n" % (entry.chrom,'splice_junc','CDS',start,end,entry.score,entry.strand,phase,pep_id,pep_id,x)) """ ##gff-version 3 ##sequence-region 19 1 287484 19 MassSpec peptide 282299 287484 10.0 - 0 ID=TEARLSFYSGHSSFGMYCMVFLALYVQ 19 MassSpec CDS 287474 287484 . - 0 Parent=TEARLSFYSGHSSFGMYCMVFLALYVQ;transcript_id=ENST00000269812 19 MassSpec CDS 282752 282809 . - 1 Parent=TEARLSFYSGHSSFGMYCMVFLALYVQ;transcript_id=ENST00000269812 19 MassSpec CDS 282299 282310 . - 0 Parent=TEARLSFYSGHSSFGMYCMVFLALYVQ;transcript_id=ENST00000269812 """ if bed_fh: bed_fh.close() if gff_fh: if gff_fa: gff_fa.close() else: outFile.close() gff_fa = open(gff_fa_file,'r') gff_fh.write("##FASTA\n") for i, line in enumerate(gff_fa): gff_fh.write(line) gff_fh.close() except Exception, e: print >> sys.stderr, "failed: Error reading %s - %s" % (options.input if options.input else 'stdin',e) if __name__ == "__main__" : __main__()