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view tools/rgenetics/rgutils.py @ 0:9071e359b9a3
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| author | xuebing |
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| date | Fri, 09 Mar 2012 19:37:19 -0500 |
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# utilities for rgenetics # # copyright 2009 ross lazarus # released under the LGPL # import subprocess, os, sys, time, tempfile,string,plinkbinJZ import datetime galhtmlprefix = """<?xml version="1.0" encoding="utf-8" ?> <!DOCTYPE html PUBLIC "-//W3C//DTD XHTML 1.0 Transitional//EN" "http://www.w3.org/TR/xhtml1/DTD/xhtml1-transitional.dtd"> <html xmlns="http://www.w3.org/1999/xhtml" xml:lang="en" lang="en"> <head> <meta http-equiv="Content-Type" content="text/html; charset=utf-8" /> <meta name="generator" content="Galaxy %s tool output - see http://g2.trac.bx.psu.edu/" /> <title></title> <link rel="stylesheet" href="/static/style/base.css" type="text/css" /> </head> <body> <div class="document"> """ galhtmlattr = """<h3><a href="http://rgenetics.org">Rgenetics</a> tool %s run at %s</h3>""" galhtmlpostfix = """</div></body></html>\n""" plinke = 'plink' # changed jan 2010 - all exes must be on path rexe = 'R' # to avoid cluster/platform dependencies smartpca = 'smartpca.perl' def timenow(): """return current time as a string """ return time.strftime('%d/%m/%Y %H:%M:%S', time.localtime(time.time())) def timestamp(): return datetime.datetime.now().strftime('%Y%m%d%H%M%S') def fail( message ): print >> sys.stderr, message return -1 def whereis(program): for path in os.environ.get('PATH', '').split(':'): if os.path.exists(os.path.join(path, program)) and \ not os.path.isdir(os.path.join(path, program)): return os.path.join(path, program) return None def bedToPicInterval(infile=None): """ Picard tools requiring targets want a sam style header which incidentally, MUST be sorted in natural order - not lexicographic order: @SQ SN:chrM LN:16571 @SQ SN:chr1 LN:247249719 @SQ SN:chr2 LN:242951149 @SQ SN:chr3 LN:199501827 @SQ SN:chr4 LN:191273063 added to the start of what looks like a bed style file chr1 67052400 67052451 - CCDS635.1_cds_0_0_chr1_67052401_r chr1 67060631 67060788 - CCDS635.1_cds_1_0_chr1_67060632_r chr1 67065090 67065317 - CCDS635.1_cds_2_0_chr1_67065091_r chr1 67066082 67066181 - CCDS635.1_cds_3_0_chr1_67066083_r see http://genome.ucsc.edu/FAQ/FAQtracks.html#tracks1 we need to add 1 to start coordinates on the way through - but length calculations are easier """ # bedToPicard.py # ross lazarus October 2010 # LGPL # for Rgenetics def getFlen(bedfname=None): """ find all features in a BED file and sum their lengths """ features = {} try: infile = open(bedfname,'r') except: print '###ERROR: getFlen unable to open bedfile %s' % bedfname sys.exit(1) for i,row in enumerate(infile): if row[0] == '@': # shouldn't happen given a bed file! print 'row %d=%s - should NOT start with @!' % (i,row) sys.exit(1) row = row.strip() if len(row) > 0: srow = row.split('\t') f = srow[0] spos = srow[1] # zero based from UCSC so no need to add 1 - eg 0-100 is 100 bases numbered 0-99 (!) epos = srow[2] # see http://genome.ucsc.edu/FAQ/FAQtracks.html#tracks1 flen = int(epos) - int(spos) features.setdefault(f,0) features[f] += flen infile.close() return features def keynat(string): ''' borrowed from http://code.activestate.com/recipes/285264-natural-string-sorting/ A natural sort helper function for sort() and sorted() without using regular expressions or exceptions. >>> items = ('Z', 'a', '10th', '1st', '9') >>> sorted(items) ['10th', '1st', '9', 'Z', 'a'] >>> sorted(items, key=keynat) ['1st', '9', '10th', 'a', 'Z'] ''' it = type(1) r = [] for c in string: if c.isdigit(): d = int(c) if r and type( r[-1] ) == it: r[-1] = r[-1] * 10 + d else: r.append(d) else: r.append(c.lower()) return r def writePic(outfname=None,bedfname=None): """ collect header info and rewrite bed with header for picard """ featlen = getFlen(bedfname=bedfname) try: outf = open(outfname,'w') except: print '###ERROR: writePic unable to open output picard file %s' % outfname sys.exit(1) infile = open(bedfname,'r') # already tested in getFlen k = featlen.keys() fk = sorted(k, key=keynat) header = ['@SQ\tSN:%s\tLN:%d' % (x,featlen[x]) for x in fk] outf.write('\n'.join(header)) outf.write('\n') for row in infile: row = row.strip() if len(row) > 0: # convert zero based start coordinate to 1 based srow = row.split('\t') srow[1] = '%d' % (int(srow[1])+1) # see http://genome.ucsc.edu/FAQ/FAQtracks.html#tracks1 outf.write('\t'.join(srow)) outf.write('\n') outf.close() infile.close() # bedToPicInterval starts here fd,outf = tempfile.mkstemp(prefix='rgPicardHsMetrics') writePic(outfname=outf,bedfname=infile) return outf def getFileString(fpath, outpath): """ format a nice file size string """ size = '' fp = os.path.join(outpath, fpath) s = '? ?' if os.path.isfile(fp): n = float(os.path.getsize(fp)) if n > 2**20: size = ' (%1.1f MB)' % (n/2**20) elif n > 2**10: size = ' (%1.1f KB)' % (n/2**10) elif n > 0: size = ' (%d B)' % (int(n)) s = '%s %s' % (fpath, size) return s def fixPicardOutputs(tempout=None,output_dir=None,log_file=None,html_output=None,progname=None,cl=[],transpose=True): """ picard produces long hard to read tab header files make them available but present them transposed for readability """ rstyle="""<style type="text/css"> tr.d0 td {background-color: oldlace; color: black;} tr.d1 td {background-color: aliceblue; color: black;} </style>""" cruft = [] dat = [] try: r = open(tempout,'r').readlines() except: r = [] for row in r: if row.strip() > '': srow = row.split('\t') if row[0] == '#': cruft.append(row.strip()) # want strings else: dat.append(srow) # want lists res = [rstyle,] res.append(galhtmlprefix % progname) res.append(galhtmlattr % (progname,timenow())) flist = os.listdir(output_dir) pdflist = [x for x in flist if os.path.splitext(x)[-1].lower() == '.pdf'] if len(pdflist) > 0: # assumes all pdfs come with thumbnail .jpgs for p in pdflist: imghref = '%s.jpg' % os.path.splitext(p)[0] # removes .pdf res.append('<table cellpadding="10"><tr><td>\n') res.append('<a href="%s"><img src="%s" alt="Click thumbnail to download %s" hspace="10" align="middle"></a>\n' % (p,imghref,p)) res.append('</tr></td></table>\n') res.append('<b>Your job produced the following output files.</b><hr/>\n') res.append('<table>\n') for i,f in enumerate(flist): fn = os.path.split(f)[-1] res.append('<tr><td><a href="%s">%s</a></td></tr>\n' % (fn,fn)) res.append('</table><p/>\n') if len(cruft) + len(dat) > 0: res.append('<b>Picard on line resources</b><ul>\n') res.append('<li><a href="http://picard.sourceforge.net/index.shtml">Click here for Picard Documentation</a></li>\n') res.append('<li><a href="http://picard.sourceforge.net/picard-metric-definitions.shtml">Click here for Picard Metrics definitions</a></li></ul><hr/>\n') if transpose: res.append('<b>Picard output (transposed for readability)</b><hr/>\n') else: res.append('<b>Picard output</b><hr/>\n') res.append('<table cellpadding="3" >\n') if len(cruft) > 0: cres = ['<tr class="d%d"><td>%s</td></tr>' % (i % 2,x) for i,x in enumerate(cruft)] res += cres if len(dat) > 0: maxrows = 100 if transpose: tdat = map(None,*dat) # transpose an arbitrary list of lists missing = len(tdat) - maxrows tdat = ['<tr class="d%d"><td>%s</td><td>%s</td></tr>\n' % ((i+len(cruft)) % 2,x[0],x[1]) for i,x in enumerate(tdat) if i < maxrows] if len(tdat) > maxrows: tdat.append('<tr><td colspan="2">...WARNING: %d rows deleted for sanity...see raw files for all rows</td></tr>' % missing) else: tdat = ['<tr class="d%d"><td>%s</td></tr>\n' % ((i+len(cruft)) % 2,x) for i,x in enumerate(dat) if i < maxrows] if len(dat) > maxrows: missing = len(dat) - maxrows tdat.append('<tr><td>...WARNING: %d rows deleted for sanity...see raw files for all rows</td></tr>' % missing) res += tdat res.append('</table>\n') else: res.append('<b>No Picard output found - please consult the Picard log above for an explanation</b>') l = open(log_file,'r').readlines() if len(l) > 0: res.append('<b>Picard log</b><hr/>\n') rlog = ['<pre>',] rlog += l rlog.append('</pre>') res += rlog else: res.append("Odd, Picard left no log file %s - must have really barfed badly?" % log_file) res.append('<hr/>The freely available <a href="http://picard.sourceforge.net/command-line-overview.shtml">Picard software</a> \n') res.append( 'generated all outputs reported here, using this command line:<br/>\n<pre>%s</pre>\n' % ''.join(cl)) res.append(galhtmlpostfix) outf = open(html_output,'w') outf.write(''.join(res)) outf.write('\n') outf.close() def keynat(string): ''' borrowed from http://code.activestate.com/recipes/285264-natural-string-sorting/ A natural sort helper function for sort() and sorted() without using regular expressions or exceptions. >>> items = ('Z', 'a', '10th', '1st', '9') >>> sorted(items) ['10th', '1st', '9', 'Z', 'a'] >>> sorted(items, key=keynat) ['1st', '9', '10th', 'a', 'Z'] ''' it = type(1) r = [] for c in string: if c.isdigit(): d = int(c) if r and type( r[-1] ) == it: r[-1] = r[-1] * 10 + d else: r.append(d) else: r.append(c.lower()) return r def getFlen(bedfname=None): """ find all features in a BED file and sum their lengths """ features = {} otherHeaders = [] try: infile = open(bedfname,'r') except: print '###ERROR: getFlen unable to open bedfile %s' % bedfname sys.exit(1) for i,row in enumerate(infile): if row.startswith('@'): # add to headers if not @SQ if not row.startswith('@SQ'): otherHeaders.append(row) else: row = row.strip() if row.startswith('#') or row.lower().startswith('browser') or row.lower().startswith('track'): continue # ignore headers srow = row.split('\t') if len(srow) > 3: srow = row.split('\t') f = srow[0] spos = srow[1] # zero based from UCSC so no need to add 1 - eg 0-100 is 100 bases numbered 0-99 (!) epos = srow[2] # see http://genome.ucsc.edu/FAQ/FAQtracks.html#tracks1 flen = int(epos) - int(spos) features.setdefault(f,0) features[f] += flen infile.close() fk = features.keys() fk = sorted(fk, key=keynat) return features,fk,otherHeaders def bedToPicInterval(infile=None,outfile=None): """ Picard tools requiring targets want a sam style header which incidentally, MUST be sorted in natural order - not lexicographic order: @SQ SN:chrM LN:16571 @SQ SN:chr1 LN:247249719 @SQ SN:chr2 LN:242951149 @SQ SN:chr3 LN:199501827 @SQ SN:chr4 LN:191273063 added to the start of what looks like a bed style file chr1 67052400 67052451 - CCDS635.1_cds_0_0_chr1_67052401_r chr1 67060631 67060788 - CCDS635.1_cds_1_0_chr1_67060632_r chr1 67065090 67065317 - CCDS635.1_cds_2_0_chr1_67065091_r chr1 67066082 67066181 - CCDS635.1_cds_3_0_chr1_67066083_r see http://genome.ucsc.edu/FAQ/FAQtracks.html#tracks1 we need to add 1 to start coordinates on the way through - but length calculations are easier """ # bedToPicard.py # ross lazarus October 2010 # LGPL # for Rgenetics """ collect header info and rewrite bed with header for picard """ featlen,fk,otherHeaders = getFlen(bedfname=infile) try: outf = open(outfile,'w') except: print '###ERROR: writePic unable to open output picard file %s' % outfile sys.exit(1) inf = open(infile,'r') # already tested in getFlen header = ['@SQ\tSN:%s\tLN:%d' % (x,featlen[x]) for x in fk] if len(otherHeaders) > 0: header += otherHeaders outf.write('\n'.join(header)) outf.write('\n') for row in inf: row = row.strip() if len(row) > 0: # convert zero based start coordinate to 1 based if row.startswith('@'): continue else: srow = row.split('\t') srow[1] = '%d' % (int(srow[1])+1) # see http://genome.ucsc.edu/FAQ/FAQtracks.html#tracks1 outf.write('\t'.join(srow)) outf.write('\n') outf.close() inf.close() def oRRun(rcmd=[],outdir=None,title='myR',rexe='R'): """ run an r script, lines in rcmd, in a temporary directory move everything, r script and all back to outdir which will be an html file # test RRun(rcmd=['print("hello cruel world")','q()'],title='test') """ rlog = [] print '### rexe = %s' % rexe assert os.path.isfile(rexe) rname = '%s.R' % title stoname = '%s.R.log' % title rfname = rname stofname = stoname if outdir: # want a specific path rfname = os.path.join(outdir,rname) stofname = os.path.join(outdir,stoname) try: os.makedirs(outdir) # might not be there yet... except: pass else: outdir = tempfile.mkdtemp(prefix=title) rfname = os.path.join(outdir,rname) stofname = os.path.join(outdir,stoname) rmoutdir = True f = open(rfname,'w') if type(rcmd) == type([]): f.write('\n'.join(rcmd)) else: # string f.write(rcmd) f.write('\n') f.close() sto = file(stofname,'w') vcl = [rexe,"--vanilla --slave", '<', rfname ] x = subprocess.Popen(' '.join(vcl),shell=True,stderr=sto,stdout=sto,cwd=outdir) retval = x.wait() sto.close() rlog = file(stofname,'r').readlines() rlog.insert(0,'## found R at %s' % rexe) if outdir <> None: flist = os.listdir(outdir) else: flist = os.listdir('.') flist.sort flist = [(x,x) for x in flist] for i,x in enumerate(flist): if x == rname: flist[i] = (x,'R script for %s' % title) elif x == stoname: flist[i] = (x,'R log for %s' % title) if False and rmoutdir: os.removedirs(outdir) return rlog,flist # for html layout def RRun(rcmd=[],outdir=None,title='myR',tidy=True): """ run an r script, lines in rcmd, in a temporary directory move everything, r script and all back to outdir which will be an html file # test RRun(rcmd=['print("hello cruel world")','q()'],title='test') echo "a <- c(5, 5); b <- c(0.5, 0.5)" | cat - RScript.R | R --slave \ --vanilla suggested by http://tolstoy.newcastle.edu.au/R/devel/05/09/2448.html """ killme = string.punctuation + string.whitespace trantab = string.maketrans(killme,'_'*len(killme)) title = title.translate(trantab) rlog = [] tempout=False rname = '%s.R' % title stoname = '%s.R.log' % title cwd = os.getcwd() if outdir: # want a specific path try: os.makedirs(outdir) # might not be there yet... except: pass os.chdir(outdir) if type(rcmd) == type([]): script = '\n'.join(rcmd) else: # string script = rcmd sto = file(stoname,'w') rscript = file(rname,'w') rscript.write(script) rscript.write('\n#R script autogenerated by rgenetics/rgutils.py on %s\n' % timenow()) rscript.close() vcl = '%s --slave --vanilla < %s' % (rexe,rname) if outdir: x = subprocess.Popen(vcl,shell=True,stderr=sto,stdout=sto,cwd=outdir) else: x = subprocess.Popen(vcl,shell=True,stderr=sto,stdout=sto) retval = x.wait() sto.close() rlog = file(stoname,'r').readlines() if retval <> 0: rlog.insert(0,'Nonzero exit code = %d' % retval) # indicate failure if outdir: flist = os.listdir(outdir) else: flist = os.listdir(os.getcwd()) flist.sort flist = [(x,x) for x in flist] for i,x in enumerate(flist): if x == rname: flist[i] = (x,'R script for %s' % title) elif x == stoname: flist[i] = (x,'R log for %s' % title) if outdir: os.chdir(cwd) return rlog,flist # for html layout def runPlink(bfn='bar',ofn='foo',logf=None,plinktasks=[],cd='./',vclbase = []): """run a series of plink tasks and append log results to stdout vcl has a list of parameters for the spawnv common settings can all go in the vclbase list and are added to each plinktask """ # root for all fplog,plog = tempfile.mkstemp() if type(logf) == type(' '): # open otherwise assume is file - ugh I'm in a hurry mylog = file(logf,'a+') else: mylog = logf mylog.write('## Rgenetics: http://rgenetics.org Galaxy Tools rgQC.py Plink runner\n') for task in plinktasks: # each is a list vcl = vclbase + task sto = file(plog,'w') x = subprocess.Popen(' '.join(vcl),shell=True,stdout=sto,stderr=sto,cwd=cd) retval = x.wait() sto.close() try: lplog = file(plog,'r').read() mylog.write(lplog) os.unlink(plog) # no longer needed except: mylog.write('### %s Strange - no std out from plink when running command line\n%s' % (timenow(),' '.join(vcl))) def pruneLD(plinktasks=[],cd='./',vclbase = []): """ plink blathers when doing pruning - ignore Linkage disequilibrium based SNP pruning if a million snps in 3 billion base pairs, have mean 3k spacing assume 40-60k of ld in ceu, a window of 120k width is about 40 snps so lots more is perhaps less efficient - each window computational cost is ON^2 unless the code is smart enough to avoid unecessary computation where allele frequencies make it impossible to see ld > the r^2 cutoff threshold So, do a window and move forward 20? The fine Plink docs at http://pngu.mgh.harvard.edu/~purcell/plink/summary.shtml#prune reproduced below Sometimes it is useful to generate a pruned subset of SNPs that are in approximate linkage equilibrium with each other. This can be achieved via two commands: --indep which prunes based on the variance inflation factor (VIF), which recursively removes SNPs within a sliding window; second, --indep-pairwise which is similar, except it is based only on pairwise genotypic correlation. Hint The output of either of these commands is two lists of SNPs: those that are pruned out and those that are not. A separate command using the --extract or --exclude option is necessary to actually perform the pruning. The VIF pruning routine is performed: plink --file data --indep 50 5 2 will create files plink.prune.in plink.prune.out Each is a simlpe list of SNP IDs; both these files can subsequently be specified as the argument for a --extract or --exclude command. The parameters for --indep are: window size in SNPs (e.g. 50), the number of SNPs to shift the window at each step (e.g. 5), the VIF threshold. The VIF is 1/(1-R^2) where R^2 is the multiple correlation coefficient for a SNP being regressed on all other SNPs simultaneously. That is, this considers the correlations between SNPs but also between linear combinations of SNPs. A VIF of 10 is often taken to represent near collinearity problems in standard multiple regression analyses (i.e. implies R^2 of 0.9). A VIF of 1 would imply that the SNP is completely independent of all other SNPs. Practically, values between 1.5 and 2 should probably be used; particularly in small samples, if this threshold is too low and/or the window size is too large, too many SNPs may be removed. The second procedure is performed: plink --file data --indep-pairwise 50 5 0.5 This generates the same output files as the first version; the only difference is that a simple pairwise threshold is used. The first two parameters (50 and 5) are the same as above (window size and step); the third parameter represents the r^2 threshold. Note: this represents the pairwise SNP-SNP metric now, not the multiple correlation coefficient; also note, this is based on the genotypic correlation, i.e. it does not involve phasing. To give a concrete example: the command above that specifies 50 5 0.5 would a) consider a window of 50 SNPs, b) calculate LD between each pair of SNPs in the window, b) remove one of a pair of SNPs if the LD is greater than 0.5, c) shift the window 5 SNPs forward and repeat the procedure. To make a new, pruned file, then use something like (in this example, we also convert the standard PED fileset to a binary one): plink --file data --extract plink.prune.in --make-bed --out pruneddata """ fplog,plog = tempfile.mkstemp() alog = [] alog.append('## Rgenetics: http://rgenetics.org Galaxy Tools rgQC.py Plink pruneLD runner\n') for task in plinktasks: # each is a list vcl = vclbase + task sto = file(plog,'w') x = subprocess.Popen(' '.join(vcl),shell=True,stdout=sto,stderr=sto,cwd=cd) retval = x.wait() sto.close() try: lplog = file(plog,'r').readlines() lplog = [x for x in lplog if x.find('Pruning SNP') == -1] alog += lplog alog.append('\n') os.unlink(plog) # no longer needed except: alog.append('### %s Strange - no std out from plink when running command line\n%s\n' % (timenow(),' '.join(vcl))) return alog def readMap(mapfile=None,allmarkers=False,rsdict={},c=None,spos=None,epos=None): """abstract out - keeps reappearing """ mfile = open(mapfile, 'r') markers = [] snpcols = {} snpIndex = 0 # in case empty or comment lines for rownum,row in enumerate(mfile): line = row.strip() if not line or line[0]=='#': continue chrom, snp, genpos, abspos = line.split()[:4] # just in case more cols try: abspos = int(abspos) except: abspos = 0 # stupid framingham data grumble grumble if allmarkers or rsdict.get(snp,None) or (chrom == c and (spos <= abspos <= epos)): markers.append((chrom,abspos,snp)) # decorate for sort into genomic snpcols[snp] = snpIndex # so we know which col to find genos for this marker snpIndex += 1 markers.sort() rslist = [x[2] for x in markers] # drop decoration rsdict = dict(zip(rslist,rslist)) mfile.close() return markers,snpcols,rslist,rsdict