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prepDE.py3
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prepDE.py3
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#!/usr/bin/env python3
import re, csv, sys, os, glob, warnings, itertools
from math import ceil
from optparse import OptionParser
from operator import itemgetter
from collections import defaultdict
parser=OptionParser(description='Generates two CSV files containing the count matrices for genes and transcripts, using the coverage values found in the output of `stringtie -e`')
parser.add_option('-i', '--input', '--in', default='.', help="a folder containing all sample sub-directories, or a text file with sample ID and path to its GTF file on each line [default: %default/]")
parser.add_option('-g', default='gene_count_matrix.csv', help="where to output the gene count matrix [default: %default")
parser.add_option('-t', default='transcript_count_matrix.csv', help="where to output the transcript count matrix [default: %default]")
parser.add_option('-l', '--length', default=75, type='int', help="the average read length [default: %default]")
parser.add_option('-p', '--pattern', default=".", help="a regular expression that selects the sample subdirectories")
parser.add_option('-c', '--cluster', action="store_true", help="whether to cluster genes that overlap with different gene IDs, ignoring ones with geneID pattern (see below)")
parser.add_option('-s', '--string', default="MSTRG", help="if a different prefix is used for geneIDs assigned by StringTie [default: %default]")
parser.add_option('-k', '--key', default="prepG", help="if clustering, what prefix to use for geneIDs assigned by this script [default: %default]")
parser.add_option('-v', action="store_true", help="enable verbose processing")
parser.add_option('--legend', default="legend.csv", help="if clustering, where to output the legend file mapping transcripts to assigned geneIDs [default: %default]")
(opts, args)=parser.parse_args()
samples = [] # List of tuples. If sample list, (first column, path). Else, (subdirectory name, path to gtf file in subdirectory)
if (os.path.isfile(opts.input)):
# gtfList = True
try:
fin = open(opts.input, 'r')
for line in fin:
if line[0] != '#':
lineLst = tuple(line.strip().split(None,2))
if (len(lineLst) != 2):
print("Error: line should have a sample ID and a file path:\n%s" % (line.strip()))
exit(1)
if lineLst[0] in samples:
print("Error: non-unique sample ID (%s)" % (lineLst[0]))
exit(1)
if not os.path.isfile(lineLst[1]):
print("Error: GTF file not found (%s)" % (lineLst[1]))
exit(1)
samples.append(lineLst)
except IOError:
print("Error: List of .gtf files, %s, doesn't exist" % (opts.input))
exit(1)
else:
# gtfList = False
## Check that opts.input directory exists
if not os.path.isdir(opts.input):
parser.print_help()
print(" ")
print("Error: sub-directory '%s' not found!" % (opts.input))
sys.exit(1)
#####
## Collect all samples file paths and if empty print help message and quit
#####
samples = []
for i in next(os.walk(opts.input))[1]:
if re.search(opts.pattern,i):
for f in glob.iglob(os.path.join(opts.input,i,"*.gtf")):
samples.append((i,f))
if len(samples) == 0:
parser.print_help()
print(" ")
print("Error: no GTF files found under base directory %s !" % (opts.input))
sys.exit(1)
RE_GENE_ID=re.compile('gene_id "([^"]+)"')
RE_GENE_NAME=re.compile('gene_name "([^"]+)"')
RE_TRANSCRIPT_ID=re.compile('transcript_id "([^"]+)"')
RE_COVERAGE=re.compile('cov "([\-\+\d\.]+)"')
RE_STRING=re.compile(re.escape(opts.string))
RE_GFILE=re.compile('\-G\s*(\S+)') #assume filepath without spaces..
#####
## Sort the sample names by the sample ID
#####
samples.sort()
#if opts.v:
# print "Sample GTFs found:"
# for s in samples:
# print s[1]
#####
## Checks whether a given row is a transcript
## other options: ex. exon, transcript, mRNA, 5'UTR
#####
def is_transcript(x):
return len(x)>2 and x[2]=="transcript"
def getGeneID(s, ctg, tid):
r=RE_GENE_ID.search(s)
#if r: return r.group(1)
rn=RE_GENE_NAME.search(s)
#if rn: return ctg+'|'+rn.group(1)
if r:
if rn:
return r.group(1)+'|'+rn.group(1)
else:
return r.group(1)
return tid
def getCov(s):
r=RE_COVERAGE.search(s)
if r:
v=float(r.group(1))
if v<0.0: v=0.0
return v
return 0.0
def is_overlap(x,y): #NEEDS TO BE INTS!
return x[0]<=y[1] and y[0]<=x[1]
def t_overlap(t1, t2): #from badGenes: chromosome, strand, cluster, start, end, (e1start, e1end)...
if t1[0] != t2[0] or t1[1] != t2[1] or t1[5]<t2[4]: return False
for i in range(6, len(t1)):
for j in range(6, len(t2)):
if is_overlap(t1[i], t2[j]): return True
return False
## Average Readlength
read_len=opts.length
## Variables/Matrices to store t/g_counts
t_count_matrix, g_count_matrix=[],[]
##Get ready for clustering, stuff is once for all samples##
geneIDs=defaultdict(lambda: str) #key=transcript, value=cluster/gene_id
## For each of the sorted sample paths
for s in samples:
badGenes=[] #list of bad genes (just ones that aren't MSTRG)
try:
## opts.input = parent directory of sample subdirectories
## s = sample currently iterating through
## os.path.join(opts.input,s,"*.gtf") path to current sample's GTF
## split = list of lists: [[chromosome, ...],...]
#with open(glob.iglob(os.path.join(opts.input,s,"*.gtf")).next()) as f:
# split=[l.split('\t') for l in f.readlines()]
# if not gtfList:
# f = open(glob.iglob(os.path.join(opts.input,s[1],"*.gtf")).next())
# else:
# f = open(s[1])
with open(s[1]) as f:
split=[l.split('\t') for l in f.readlines()]
## i = numLine; v = corresponding i-th GTF row
for i,v in enumerate(split):
if is_transcript(v):
try:
t_id=RE_TRANSCRIPT_ID.search(v[8]).group(1)
g_id=getGeneID(v[8], v[0], t_id)
except:
print("Problem parsing file %s at line:\n:%s\n" % (s[1], v))
sys.exit(1)
geneIDs[t_id]=g_id
if not RE_STRING.match(g_id):
badGenes.append([v[0],v[6], t_id, g_id, min(int(v[3]),int(v[4])), max(int(v[3]),int(v[4]))]) #chromosome, strand, cluster/transcript id, start, end
j=i+1
while j<len(split) and split[j][2]=="exon":
badGenes[len(badGenes)-1].append((min(int(split[j][3]), int(split[j][4])), max(int(split[j][3]), int(split[j][4]))))
j+=1
except StopIteration:
warnings.warn("Didn't get a GTF in that directory. Looking in another...")
else: #we found the "bad" genes!
break
##THE CLUSTERING BEGINS!##
if opts.cluster and len(badGenes)>0:
clusters=[] #lists of lists (could be sets) or something of transcripts
badGenes.sort(key=itemgetter(3)) #sort by start coord...?
i=0
while i<len(badGenes): #rather un-pythonic
temp_cluster=[badGenes[i]]
k=0
while k<len(temp_cluster):
j=i+1
while j<len(badGenes):
if t_overlap(temp_cluster[k], badGenes[j]):
temp_cluster.append(badGenes[j])
del badGenes[j]
else:
j+=1
k+=1
if len(temp_cluster)>1:
clusters.append([t[2] for t in temp_cluster])
i+=1
print(len(clusters))
for c in clusters:
c.sort()
clusters.sort(key=itemgetter(0))
legend=[]
for u,c in enumerate(clusters):
my_ID=opts.key+str((u+1))
legend.append(list(itertools.chain.from_iterable([[my_ID],c]))) #my_ID, clustered transcript IDs
for t in c:
geneIDs[t]=my_ID
## geneIDs[t]="|".join(c) #duct-tape transcript IDs together, disregarding ref_gene_names and things like that
with open(opts.legend, 'w') as l_file:
my_writer=csv.writer(l_file)
my_writer.writerows(legend)
geneDict=defaultdict(lambda: defaultdict(lambda: 0)) #key=gene/cluster, value=dictionary with key=sample, value=summed counts
t_dict=defaultdict(lambda: defaultdict(lambda: 0))
guidesFile='' # file given with -G for the 1st sample
for q, s in enumerate(samples):
if opts.v:
print(">processing sample %s from file %s" % s)
lno=0
try:
#with open(glob.iglob(os.path.join(opts.input,s,"*.gtf")).next()) as f: #grabs first .gtf file it finds inside the sample subdirectory
# if not gtfList:
# f = open(glob.iglob(os.path.join(opts.input,s[1],"*.gtf")).next())
# else:
f = open(s[1])
transcript_len=0
for l in f:
lno+=1
if l.startswith('#'):
if lno==1:
ei=l.find('-e')
if ei<0:
print("Error: sample file %s was not generated with -e option!" % ( s[1] ))
sys.exit(1)
gf=RE_GFILE.search(l)
if gf:
gfile=gf.group(1)
if guidesFile:
if gfile != guidesFile:
print("Warning: sample file %s generated with a different -G file (%s) than the first sample (%s)" % ( s[1], gfile, guidesFile ))
else:
guidesFile=gfile
else:
print("Error: sample %s was not processed with -G option!" % ( s[1] ))
sys.exit(1)
continue
v=l.split('\t')
if v[2]=="transcript":
if transcript_len>0:
## transcriptList.append((g_id, t_id, int(ceil(coverage*transcript_len/read_len))))
t_dict[t_id][s[0]] = int(ceil(coverage*transcript_len/read_len))
t_id=RE_TRANSCRIPT_ID.search(v[len(v)-1]).group(1)
#g_id=RE_GENE_ID.search(v[len(v)-1]).group(1)
g_id=getGeneID(v[8], v[0], t_id)
#coverage=float(RE_COVERAGE.search(v[len(v)-1]).group(1))
coverage=getCov(v[8])
transcript_len=0
if v[2]=="exon":
transcript_len+=int(v[4])-int(v[3])+1 #because end coordinates are inclusive in GTF
## transcriptList.append((g_id, t_id, int(ceil(coverage*transcript_len/read_len))))
t_dict[t_id][s[0]]=int(ceil(coverage*transcript_len/read_len))
except StopIteration:
# if not gtfList:
# warnings.warn("No GTF file found in " + os.path.join(opts.input,s[1]))
# else:
warnings.warn("No GTF file found in " + s[1])
## transcriptList.sort(key=lambda bla: bla[1]) #gene_id
for i,v in t_dict.items():
## print i,v
try:
geneDict[geneIDs[i]][s[0]]+=v[s[0]]
except KeyError:
print("Error: could not locate transcript %s entry for sample %s" % ( i, s[0] ))
raise
if opts.v:
print("..writing %s " % ( opts.t ))
with open(opts.t, 'w') as csvfile:
my_writer = csv.DictWriter(csvfile, fieldnames = ["transcript_id"] + [x for x,y in samples])
my_writer.writerow(dict((fn,fn) for fn in my_writer.fieldnames))
for i in t_dict:
t_dict[i]["transcript_id"] = i
my_writer.writerow(t_dict[i])
if opts.v:
print("..writing %s " % ( opts.g ))
with open(opts.g, 'w') as csvfile:
my_writer = csv.DictWriter(csvfile, fieldnames = ["gene_id"] + [x for x,y in samples])
## my_writer.writerow([""]+samples)
## my_writer.writerows(geneDict)
my_writer.writerow(dict((fn,fn) for fn in my_writer.fieldnames))
for i in geneDict:
geneDict[i]["gene_id"] = i #add gene_id to row
my_writer.writerow(geneDict[i])
if opts.v:
print("All done.")