Mercurial > repos > modencode-dcc > spp_package
view run_spp.R @ 12:d063cc917090 draft
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author | modencode-dcc |
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date | Thu, 07 Feb 2013 23:42:12 -0500 |
parents | 495a6d033ca1 |
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# run_spp.R # ============= # Author: Anshul Kundaje, Computer Science Dept., Stanford University # Email: akundaje@stanford.edu # Last updated: Oct 8, 2010 # ============= # MANDATORY ARGUMENTS # -c=<ChIP_tagAlign/BAMFile>, full path and name of tagAlign/BAM file (can be gzipped) (FILE EXTENSION MUST BE tagAlign.gz, tagAlign, bam or bam.gz) # MANDATORY ARGUMENT FOR PEAK CALLING # -i=<Input_tagAlign/BAMFile>, full path and name of tagAlign/BAM file (can be gzipped) (FILE EXTENSION MUST BE tagAlign.gz, tagAlign, bam or bam.gz) # OPTIONAL ARGUMENTS # -s=<min>:<step>:<max> , strand shifts at which cross-correlation is evaluated, default=-100:5:600 # -speak=<strPeak>, user-defined cross-correlation peak strandshift # -x=<min>:<max>, strand shifts to exclude (This is mainly to avoid phantom peaks) default=10:(readlen+10) # -p=<nodes> , number of parallel processing nodes, default=NULL # -fdr=<falseDisoveryRate> , false discovery rate threshold for peak calling # -npeak=<numPeaks>, threshold on number of peaks to call # -tmpdir=<tempdir> , Temporary directory (if not specified R function tempdir() is used) # -filtchr=<chrnamePattern> , Pattern to use to remove tags that map to specific chromosomes e.g. _ will remove all tags that map to chromosomes with _ in their name # OUTPUT PARAMETERS # -odir=<outputDirectory> name of output directory (If not set same as ChIP file directory is used) # -savn=<narrowpeakfilename> OR -savn NarrowPeak file name # -savr=<regionpeakfilename> OR -savr RegionPeak file name # -savd=<rdatafile> OR -savd , save Rdata file # -savp=<plotdatafile> OR -savp , save cross-correlation plot # -out=<resultfile>, append peakshift result to a file # format:Filename<tab>numReads<tab>estFragLen<tab>corr_estFragLen<tab>PhantomPeak<tab>corr_phantomPeak<tab>argmin_corr<tab>min_corr<tab>phantomPeakCoef<tab>relPhantomPeakCoef<tab>QualityTag # -rf , if plot or rdata or narrowPeak file exists replace it. If not used then the run is aborted if the plot or Rdata or narrowPeak file exists # -clean, if present will remove the original chip and control files after reading them in. CAUTION: Use only if the script calling run_spp.R is creating temporary files args <- commandArgs(trailingOnly=TRUE); # Read Arguments from command line nargs = length(args); # number of arguments # ########################################################################### # AUXILIARY FUNCTIONS # ########################################################################### print.usage <- function() { # =================================== # Function will print function usage # =================================== cat('Usage: Rscript run_spp.R <options>\n',file=stderr()) cat('MANDATORY ARGUMENTS\n',file=stderr()) cat('-c=<ChIP_alignFile>, full path and name (or URL) of tagAlign/BAM file (can be gzipped)(FILE EXTENSION MUST BE tagAlign.gz, tagAlign, bam or bam.gz) \n',file=stderr()) cat('MANDATORY ARGUMENTS FOR PEAK CALLING\n',file=stderr()) cat('-i=<Input_alignFile>, full path and name (or URL) of tagAlign/BAM file (can be gzipped) (FILE EXTENSION MUST BE tagAlign.gz, tagAlign, bam or bam.gz) \n',file=stderr()) cat('OPTIONAL ARGUMENTS\n',file=stderr()) cat('-s=<min>:<step>:<max> , strand shifts at which cross-correlation is evaluated, default=-100:5:600\n',file=stderr()) cat('-speak=<strPeak>, user-defined cross-correlation peak strandshift\n',file=stderr()) cat('-x=<min>:<max>, strand shifts to exclude (This is mainly to avoid region around phantom peak) default=10:(readlen+10)\n',file=stderr()) cat('-p=<nodes> , number of parallel processing nodes, default=0\n',file=stderr()) cat('-fdr=<falseDisoveryRate> , false discovery rate threshold for peak calling\n',file=stderr()) cat('-npeak=<numPeaks>, threshold on number of peaks to call\n',file=stderr()) cat('-tmpdir=<tempdir> , Temporary directory (if not specified R function tempdir() is used)\n',file=stderr()) cat('-filtchr=<chrnamePattern> , Pattern to use to remove tags that map to specific chromosomes e.g. _ will remove all tags that map to chromosomes with _ in their name\n',file=stderr()) cat('OUTPUT ARGUMENTS\n',file=stderr()) cat('-odir=<outputDirectory> name of output directory (If not set same as ChIP file directory is used)\n',file=stderr()) cat('-savn=<narrowpeakfilename> OR -savn NarrowPeak file name (fixed width peaks)\n',file=stderr()) cat('-savr=<regionpeakfilename> OR -savr RegionPeak file name (variable width peaks with regions of enrichment)\n',file=stderr()) cat('-savd=<rdatafile> OR -savd, save Rdata file\n',file=stderr()) cat('-savp=<plotdatafile> OR -savp, save cross-correlation plot\n',file=stderr()) cat('-out=<resultfile>, append peakshift/phantomPeak results to a file\n',file=stderr()) cat(' format:Filename<tab>numReads<tab>estFragLen<tab>corr_estFragLen<tab>PhantomPeak<tab>corr_phantomPeak<tab>argmin_corr<tab>min_corr<tab>phantomPeakCoef<tab>relPhantomPeakCoef<tab>QualityTag)\n',file=stderr()) cat('-rf, if plot or rdata or narrowPeak file exists replace it. If not used then the run is aborted if the plot or Rdata or narrowPeak file exists\n',file=stderr()) cat('-clean, if present will remove the original chip and control files after reading them in. CAUTION: Use only if the script calling run_spp.R is creating temporary files\n',file=stderr()) } # end: print.usage() get.file.parts <- function(file.fullpath) { # =================================== # Function will take a file name with path and split the file name into # path, fullname, name and ext # =================================== if (! is.character(file.fullpath)) { stop('File name must be a string') } file.parts <- strsplit(as.character(file.fullpath), .Platform$file.sep, fixed=TRUE)[[1]] # split on file separator if (length(file.parts) == 0) { # if empty file name return(list(path='', fullname='', name='', ext='') ) } else { if (length(file.parts) == 1) { # if no path then just the file name itself file.path <- '.' file.fullname <- file.parts } else { file.path <- paste(file.parts[1:(length(file.parts)-1)], collapse=.Platform$file.sep) # 1:last-1 token is path file.fullname <- file.parts[length(file.parts)] # last token is filename } file.fullname.parts <- strsplit(file.fullname,'.',fixed=TRUE)[[1]] # split on . if (length(file.fullname.parts) == 1) { # if no extension file.ext <- '' file.name <- file.fullname.parts } else { file.ext <- paste('.', file.fullname.parts[length(file.fullname.parts)], sep="") # add the . to the last token file.name <- paste(file.fullname.parts[1:(length(file.fullname.parts)-1)], collapse=".") } return(list(path=file.path, fullname=file.fullname, name=file.name, ext=file.ext)) } } # end: get.file.parts() parse.arguments <- function(args) { # =================================== # Function will parse arguments # =================================== # Set arguments to default values chip.file <- NA # main ChIP tagAlign/BAM file name isurl.chip.file <- FALSE # flag indicating whether ChIP file is a URL control.file <- NA # control tagAlign/BAM file name isurl.control.file <- FALSE # flag indicating whether control file is a URL sep.min <- -100 # min strand shift sep.max <- 600 # max strand shift sep.bin <- 5 # increment for strand shift sep.peak <- NA # user-defined peak shift exclude.min <- 10 # lowerbound of strand shift exclusion region exclude.max <- NaN # upperbound of strand shift exclusion region n.nodes <- NA # number of parallel processing nodes fdr <- 0.01 # false discovery rate threshold for peak calling npeak <- NA # threshold on number of peaks to call temp.dir <- tempdir() # temporary directory chrname.rm.pattern <- NA # chromosome name pattern used to remove tags output.odir <- NA # Output directory name output.npeak.file <- NA # Output narrowPeak file name output.rpeak.file <- NA # Output regionPeak file name output.rdata.file <- NA # Rdata file output.plot.file <- NA # cross correlation plot file output.result.file <- NA # result file replace.flag <- FALSE # replace file flag clean.files.flag <- FALSE # file deletion flag # Parse arguments for (each.arg in args) { if (grepl('^-c=',each.arg)) { #-c=<chip.file> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { chip.file <- arg.split[2] # second part is chip.file } else { stop('No tagAlign/BAM file name provided for parameter -c=') } } else if (grepl('^-i=',each.arg)) { #-i=<control.file> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { control.file <- arg.split[2] # second part is control.file } else { stop('No tagAlign/BAM file name provided for parameter -i=') } } else if (grepl('^-s=',each.arg)) { #-s=<sep.min>:<sep.bin>:<sep.max> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { sep.vals <- arg.split[2] # second part is sepmin:sepbin:sepmax sep.vals.split <- strsplit(sep.vals,':',fixed=TRUE)[[1]] # split on : if (length(sep.vals.split) != 3) { # must have 3 parts stop('Strand shift limits must be specified as -s=sepmin:sepbin:sepmax') } else { if (any(is.na(as.numeric(sep.vals.split)))) { # check that sep vals are numeric stop('Strand shift limits must be numeric values') } sep.min <- round(as.numeric(sep.vals.split[1])) sep.bin <- round(as.numeric(sep.vals.split[2])) sep.max <- round(as.numeric(sep.vals.split[3])) if ((sep.min > sep.max) || (sep.bin > (sep.max - sep.min)) || (sep.bin < 0)) { stop('Illegal separation values -s=sepmin:sepbin:sepmax') } } } else { stop('Strand shift limits must be specified as -s=sepmin:sepbin:sepmax') } } else if (grepl('^-speak=',each.arg)) { #-speak=<sep.peak> , user-defined cross-correlation peak strandshift arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { sep.peak <- arg.split[2] # second part is <sep.peak> if (is.na(as.numeric(sep.peak))) { # check that sep.peak is numeric stop('-speak=<sep.peak>: User defined peak shift must be numeric') } sep.peak <- as.numeric(sep.peak) } else { stop('User defined peak shift must be provided as -speak=<sep.peak>') } } else if (grepl('^-x=',each.arg)) { #-x=<exclude.min>:<exclude.max> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { exclude.vals <- arg.split[2] # second part is excludemin:excludemax exclude.vals.split <- strsplit(exclude.vals,':',fixed=TRUE)[[1]] # split on : if (length(exclude.vals.split) != 2) { # must have 2 parts stop('Exclusion limits must be specified as -x=excludemin:excludemax') } else { if (any(is.na(as.numeric(exclude.vals.split)))) { # check that exclude vals are numeric stop('Exclusion limits must be numeric values') } exclude.min <- round(as.numeric(exclude.vals.split[1])) exclude.max <- round(as.numeric(exclude.vals.split[2])) if (exclude.min > exclude.max) { stop('Illegal exclusion limits -x=excludemin:excludemax') } } } else { stop('Exclusion limits must be specified as -x=excludemin:excludemax') } } else if (grepl('^-p=',each.arg)) { #-p=<n.nodes> , number of parallel processing nodes, default=NULL arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { n.nodes <- arg.split[2] # second part is numnodes if (is.na(as.numeric(n.nodes))) { # check that n.nodes is numeric stop('-p=<numnodes>: numnodes must be numeric') } n.nodes <- round(as.numeric(n.nodes)) } else { stop('Number of parallel nodes must be provided as -p=<numnodes>') } } else if (grepl('^-fdr=',each.arg)) { #-fdr=<fdr> , false discovery rate, default=0.01 arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { fdr <- arg.split[2] # second part is fdr if (is.na(as.numeric(fdr))) { # check that fdr is numeric stop('-fdr=<falseDiscoveryRate>: false discovery rate must be numeric') } fdr <- as.numeric(fdr) } else { stop('False discovery rate must be provided as -fdr=<fdr>') } } else if (grepl('^-npeak=',each.arg)) { #-npeak=<numPeaks> , number of peaks threshold, default=NA arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { npeak <- arg.split[2] # second part is npeak if (is.na(as.numeric(npeak))) { # check that npeak is numeric stop('-npeak=<numPeaks>: threshold on number of peaks must be numeric') } npeak <- round(as.numeric(npeak)) } else { stop('Threshold on number of peaks must be provided as -npeak=<numPeaks>') } } else if (grepl('^-tmpdir=',each.arg)) { #-tmpdir=<temp.dir> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { temp.dir <- arg.split[2] # second part is temp.dir } else { stop('No temporary directory provided for parameter -tmpdir=') } } else if (grepl('^-filtchr=',each.arg)) { #-filtchr=<chrname.rm.pattern> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { chrname.rm.pattern <- arg.split[2] # second part is chrname.rm.pattern } else { stop('No pattern provided for parameter -filtchr=') } } else if (grepl('^-odir=',each.arg)) { #-odir=<output.odir> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { output.odir <- arg.split[2] # second part is output.odir } else { stop('No output directory provided for parameter -odir=') } } else if (grepl('^-savn',each.arg)) { # -savn=<output.npeak.file> OR -savn , save narrowpeak arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2])) { output.npeak.file <- arg.split[2] #-savn= } else if (each.arg=='-savn') { output.npeak.file <- NULL # NULL indicates get the name from the main file name } else { stop('Argument for saving narrowPeak file must be -savn or -savn=<filename>') } } else if (grepl('^-savr',each.arg)) { # -savr=<output.rpeak.file> OR -savr , save regionpeak arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2])) { output.rpeak.file <- arg.split[2] #-savr= } else if (each.arg=='-savr') { output.rpeak.file <- NULL # NULL indicates get the name from the main file name } else { stop('Argument for saving regionPeak file must be -savr or -savr=<filename>') } } else if (grepl('^-savd',each.arg)) { # -savd=<output.rdata.file> OR -savd , save Rdata file arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2])) { output.rdata.file <- arg.split[2] #-savd= } else if (each.arg=='-savd') { output.rdata.file <- NULL # NULL indicates get the name from the main file name } else { stop('Argument for saving Rdata file must be -savd or -savd=<filename>') } } else if (grepl('^-savp',each.arg)) { # -savp=<output.plot.file> OR -savp , save cross-correlation plot arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2])) { output.plot.file <- arg.split[2] #-savp= } else if (each.arg=='-savp') { output.plot.file <- NULL # NULL indicates get the name from the main file name } else { stop('Argument for saving Rdata file must be -savp or -savp=<filename>') } } else if (grepl('^-out=',each.arg)) { #-out=<output.result.file> arg.split <- strsplit(each.arg,'=',fixed=TRUE)[[1]] # split on = if (! is.na(arg.split[2]) ) { output.result.file <- arg.split[2] # second part is output.result.file } else { stop('No result file provided for parameter -out=') } } else if (each.arg == '-rf') { replace.flag <- TRUE } else if (each.arg == '-clean') { clean.files.flag <- TRUE } else { stop('Illegal argument ',each.arg) } } # End: for loop # Check mandatory arguments if (is.na(chip.file)) { stop('-c=<tagAlign/BAMFileName> is a mandatory argument') } if (is.na(control.file) && ! is.na(output.npeak.file)) { stop('-i=<tagAlign/BAMFileName> is required for peak calling') } # Check if ChIP and control files are URLs if (grepl('^http://',chip.file)) { isurl.chip.file <- TRUE } if (grepl('^http://',control.file)) { isurl.control.file <- TRUE } # If ChIP file is a URL output.odir MUST be specified if (isurl.chip.file && is.na(output.odir)) { stop('If ChIP file is a URL, then output directory MUST be specified') } # Check that ChIP and control files exist if (isurl.chip.file) { if (system(paste('wget -q --spider',chip.file)) != 0) { stop('ChIP file URL not valid: ',chip.file) } } else if (!file.exists(chip.file)) { stop('ChIP File:',chip.file,' does not exist') } if (!is.na(control.file)) { if (isurl.control.file) { if (system(paste('wget -q --spider',control.file)) != 0) { stop('Control file URL not valid: ',control.file) } } else if (!file.exists(control.file)) { stop('Control File:',control.file,' does not exist') } } # Correct other arguments if (is.na(output.odir)) { # Reconstruct output.odir if not provided output.odir <- get.file.parts(chip.file)$path } if (is.null(output.npeak.file)) { # Reconstruct output.npeak.file if NULL output.npeak.file <- file.path(output.odir, paste(get.file.parts(chip.file)$name, '_VS_', get.file.parts(control.file)$name,'.narrowPeak', sep="")) } if (is.null(output.rpeak.file)) { # Reconstruct output.rpeak.file if NULL output.rpeak.file <- file.path(output.odir, paste(get.file.parts(chip.file)$name, '_VS_', get.file.parts(control.file)$name,'.regionPeak', sep="")) } if (is.null(output.rdata.file)) { # Reconstruct output.rdata.file if NULL output.rdata.file <- file.path(output.odir, paste(get.file.parts(chip.file)$name, '.Rdata', sep="")) } if (is.null(output.plot.file)) { # Reconstruct output.plot.file if NULL output.plot.file <- file.path(output.odir, paste(get.file.parts(chip.file)$name, '.pdf', sep="")) } return(list(chip.file=chip.file, isurl.chip.file=isurl.chip.file, control.file=control.file, isurl.control.file=isurl.control.file, sep.range=c(sep.min,sep.bin,sep.max), sep.peak=sep.peak, ex.range=c(exclude.min,exclude.max), n.nodes=n.nodes, fdr=fdr, npeak=npeak, temp.dir=temp.dir, chrname.rm.pattern=chrname.rm.pattern, output.odir=output.odir, output.npeak.file=output.npeak.file, output.rpeak.file=output.rpeak.file, output.rdata.file=output.rdata.file, output.plot.file=output.plot.file, output.result.file=output.result.file, replace.flag=replace.flag, clean.files.flag=clean.files.flag)) } # end: parse.arguments() read.align <- function(align.filename) { # =================================== # Function will read a tagAlign or BAM file # =================================== if (grepl('(\\.bam)?.*(\\.tagAlign)',align.filename)) { # if tagalign file chip.data <- read.tagalign.tags(align.filename) # get readlength info tmpDataRows <- read.table(align.filename,nrows=500) chip.data$read.length <- round(median(tmpDataRows$V3 - tmpDataRows$V2)) } else if (grepl('(\\.tagAlign)?.*(\\.bam)',align.filename)) { # if bam file # create BAM file name bam2align.filename <- sub('\\.bam','.tagAlign',align.filename) # generate command to convert bam to tagalign command <- vector(length=2) command[1] <- sprintf("samtools view -F 0x0204 -o - %s",align.filename) command[2] <- paste("awk 'BEGIN{FS=" , '"\t"' , ";OFS=", '"\t"} {if (and($2,16) > 0) {print $3,($4-1),($4-1+length($10)),"N","1000","-"} else {print $3,($4-1),($4-1+length($10)),"N","1000","+"}}', "' 1> ", bam2align.filename, sep="") # command[2] <- paste("awk 'BEGIN{OFS=", '"\t"} {if (and($2,16) > 0) {print $3,($4-1),($4-1+length($10)),"N","1000","-"} else {print $3,($4-1),($4-1+length($10)),"N","1000","+"}}', "' 1> ", bam2align.filename, sep="") command <- paste(command,collapse=" | ") # Run command status <- system(command,intern=FALSE,ignore.stderr=FALSE) if ((status != 0) || !file.exists(bam2align.filename)) { cat(sprintf("Error converting BAM to tagalign file: %s\n",align.filename),file=stderr()) q(save="no",status=1) } # read converted BAM file chip.data <- read.tagalign.tags(bam2align.filename) # get readlength info tmpDataRows <- read.table(bam2align.filename,nrows=500) chip.data$read.length <- round(median(tmpDataRows$V3 - tmpDataRows$V2)) # delete temporary tagalign file file.remove(bam2align.filename) } else { cat(sprintf("Error:Unknown file format for file:%s\n",align.fname),file=stderr()) q(save="no",status=1) } return(chip.data) } # end: read.align() print.run.params <- function(params){ # =================================== # Output run parameters # =================================== cat('################\n',file=stdout()) cat(iparams$chip.file, iparams$control.file, iparams$sep.range, iparams$sep.peak, iparams$ex.range, iparams$n.nodes, iparams$fdr, iparams$npeak, iparams$output.odir, iparams$output.npeak.file, iparams$output.rpeak.file, iparams$output.rdata.file, iparams$output.plot.file, iparams$output.result.file, iparams$replace.flag, labels=c('ChIP data:','Control data:', 'strandshift(min):','strandshift(step):','strandshift(max)','user-defined peak shift', 'exclusion(min):','exclusion(max):','num parallel nodes:','FDR threshold:','NumPeaks Threshold:','Output Directory:', 'narrowPeak output file name:', 'regionPeak output file name:', 'Rdata filename:', 'plot pdf filename:','result filename:','Overwrite files?:'), fill=18, file=stdout()) cat('\n',file=stdout()) } # end: print.run.parameters() check.replace.flag <- function(params){ # =================================== # Check if files exist # =================================== # If replace.flag is NOT set, check if output files exist and abort if necessary if (! iparams$replace.flag) { if (! is.na(iparams$output.npeak.file)) { if (file.exists(iparams$output.npeak.file)) { cat('narrowPeak file already exists. Aborting Run. Use -rf if you want to overwrite\n',file=stderr()) q(save="no",status=1) } } if (! is.na(iparams$output.rpeak.file)) { if (file.exists(iparams$output.rpeak.file)) { cat('regionPeak file already exists. Aborting Run. Use -rf if you want to overwrite\n',file=stderr()) q(save="no",status=1) } } if (! is.na(iparams$output.plot.file)) { if (file.exists(iparams$output.plot.file)) { cat('Plot file already exists. Aborting Run. Use -rf if you want to overwrite\n',file=stderr()) q(save="no",status=1) } } if (! is.na(iparams$output.rdata.file)) { if (file.exists(iparams$output.rdata.file)) { cat('Rdata file already exists. Aborting Run. Use -rf if you want to overwrite\n',file=stderr()) q(save="no",status=1) } } } } # ############################################################################# # MAIN FUNCTION # ############################################################################# # Check number of arguments minargs = 1; maxargs = 17; if (nargs < minargs | nargs > maxargs) { print.usage() q(save="no",status=1) } # Parse arguments # iparams$chip.file # iparams$isurl.chip.file # iparams$control.file # iparams$isurl.control.file # iparams$sep.range # iparams$sep.peak # iparams$ex.range # iparams$n.nodes # iparams$fdr # iparams$npeak # iparams$temp.dir # iparams$output.odir # iparams$output.npeak.file # iparams$output.rpeak.file # iparams$output.rdata.file # iparams$output.plot.file # iparams$output.result.file # iparams$replace.flag # iparams$clean.files.flag iparams <- parse.arguments(args) # Print run parameters print.run.params(iparams) # Check if output files exist check.replace.flag(iparams) # curr.chip.file and curr.control.file always point to the original ChIP and control files on disk # ta.chip.filename & ta.control.filename always point to the final but temporary versions of the ChIP and control files that will be passed to read.align # Download ChIP and control files if necessary to temp.dir if (iparams$isurl.chip.file) { curr.chip.file <- file.path(iparams$temp.dir, get.file.parts(iparams$chip.file)$fullname) # file is downloaded to temp.dir. Has same name as URL suffix cat('Downloading ChIP file:',iparams$chip.file,"\n",file=stdout()) if (system(paste('wget -N -q -P',iparams$temp.dir,iparams$chip.file)) != 0) { stop('Error downloading ChIP file:',iparams$chip.file) } } else { curr.chip.file <- iparams$chip.file # file is in original directory } if (iparams$isurl.control.file) { curr.control.file <- file.path(iparams$temp.dir, get.file.parts(iparams$control.file)$fullname) # file is downloaded to temp.dir. Has same name as URL suffix cat('Downloading control file:',iparams$control.file,"\n",file=stdout()) if (system(paste('wget -N -q -P',iparams$temp.dir,iparams$control.file)) != 0) { stop('Error downloading Control file:',iparams$control.file) } } else { curr.control.file <- iparams$control.file # file is in original directory } # unzip ChIP and input files if required AND copy to temp directory if (get.file.parts(curr.chip.file)$ext == '.gz') { ta.chip.filename <- tempfile(get.file.parts(curr.chip.file)$name, tmpdir=iparams$temp.dir) # unzip file to temp.dir/[filename with .gz removed][randsuffix] cat('Decompressing ChIP file\n',file=stdout()) if (system(paste("gunzip -c",curr.chip.file,">",ta.chip.filename)) != 0) { stop('Unable to decompress file:', iparams$chip.file) } if (iparams$clean.files.flag) { # Remove original file if clean.files.flag is set file.remove(curr.chip.file) } } else { ta.chip.filename <- tempfile(get.file.parts(curr.chip.file)$fullname, tmpdir=iparams$temp.dir) if (iparams$clean.files.flag) { file.rename(curr.chip.file,ta.chip.filename) # move file to temp.dir/[filename][randsuffix] } else { file.copy(curr.chip.file,ta.chip.filename) # copy file to temp.dir/[filename][randsuffix] } } if (! is.na(iparams$control.file)) { if (get.file.parts(curr.control.file)$ext == '.gz') { ta.control.filename <- tempfile(get.file.parts(curr.control.file)$name, tmpdir=iparams$temp.dir) # unzip file to temp.dir/[filename with .gz removed][randsuffix] cat('Decompressing control file\n',file=stdout()) if (system(paste("gunzip -c",curr.control.file,">",ta.control.filename)) != 0) { stop('Unable to decompress file:', iparams$control.file) } if (iparams$clean.files.flag) { # Remove original file if clean.files.flag is set file.remove(curr.control.file) } } else { ta.control.filename <- tempfile(get.file.parts(curr.control.file)$fullname, tmpdir=iparams$temp.dir) # copy file to temp.dir/[filename][randsuffix] if (iparams$clean.files.flag) { file.rename(curr.control.file,ta.control.filename) # move file to temp.dir/[filename][randsuffix] } else { file.copy(curr.control.file,ta.control.filename) # copy file to temp.dir/[filename][randsuffix] } } } # Remove downloaded files if (iparams$isurl.chip.file & file.exists(curr.chip.file)) { file.remove(curr.chip.file) } if (! is.na(iparams$control.file)) { if (iparams$isurl.control.file & file.exists(curr.control.file)) { file.remove(curr.control.file) } } # Load SPP library library(spp) # Read ChIP tagAlign/BAM files cat("Reading ChIP tagAlign/BAM file",iparams$chip.file,"\n",file=stdout()) chip.data <- read.align(ta.chip.filename) cat("ChIP data read length",chip.data$read.length,"\n",file=stdout()) file.remove(ta.chip.filename) # Delete temporary file if (length(chip.data$tags)==0) { stop('Error in ChIP file format:', iparams$chip.file) } # Remove illegal chromosome names if (! is.na(iparams$chrname.rm.pattern)) { selectidx <- which(grepl(iparams$chrname.rm.pattern,names(chip.data$tags))==FALSE) chip.data$tags <- chip.data$tags[selectidx] chip.data$quality <- chip.data$quality[selectidx] } chip.data$num.tags <- sum(unlist(lapply(chip.data$tags,function(d) length(d)))) # Read Control tagAlign/BAM files if (! is.na(iparams$control.file)) { cat("Reading Control tagAlign/BAM file",iparams$control.file,"\n",file=stdout()) control.data <- read.align(ta.control.filename) file.remove(ta.control.filename) # Delete temporary file if (length(control.data$tags)==0) { stop('Error in control file format:', iparams$chip.file) } cat("Control data read length",control.data$read.length,"\n",file=stdout()) # Remove illegal chromosome names if (! is.na(iparams$chrname.rm.pattern)) { selectidx <- which(grepl(iparams$chrname.rm.pattern,names(control.data$tags))==FALSE) control.data$tags <- control.data$tags[selectidx] control.data$quality <- control.data$quality[selectidx] } control.data$num.tags <- sum(unlist(lapply(control.data$tags,function(d) length(d)))) } # Open multiple processes if required if (is.na(iparams$n.nodes)) { cluster.nodes <- NULL } else { library(snow) cluster.nodes <- makeCluster(iparams$n.nodes) } # ################################# # Calculate cross-correlation for various strand shifts # ################################# cat("Calculating peak characteristics\n",file=stdout()) # crosscorr # $cross.correlation : Cross-correlation profile as an $x/$y data.frame # $peak : Position ($x) and height ($y) of automatically detected cross-correlation peak. # $whs: Optimized window half-size for binding detection (based on the width of the cross-correlation peak) crosscorr <- get.binding.characteristics(chip.data, srange=iparams$sep.range[c(1,3)], bin=iparams$sep.range[2], accept.all.tags=T, cluster=cluster.nodes) if (!is.na(iparams$n.nodes)) { stopCluster(cluster.nodes) } # Smooth the cross-correlation curve if required cc <- crosscorr$cross.correlation crosscorr$min.cc <- crosscorr$cross.correlation[ which.min(crosscorr$cross.correlation$y) , ] # minimum value and shift of cross-correlation cat("Minimum cross-correlation value", crosscorr$min.cc$y,"\n",file=stdout()) cat("Minimum cross-correlation shift", crosscorr$min.cc$x,"\n",file=stdout()) sbw <- 2*floor(ceiling(5/iparams$sep.range[2]) / 2) + 1 # smoothing bandwidth cc$y <- runmean(cc$y,sbw,alg="fast") # Compute cross-correlation peak bw <- ceiling(2/iparams$sep.range[2]) # crosscorr[i] is compared to crosscorr[i+/-bw] to find peaks peakidx <- (diff(cc$y,bw)>=0) # cc[i] > cc[i-bw] peakidx <- diff(peakidx,bw) peakidx <- which(peakidx==-1) + bw # exclude peaks from the excluded region if ( is.nan(iparams$ex.range[2]) ) { iparams$ex.range[2] <- chip.data$read.length+10 } peakidx <- peakidx[(cc$x[peakidx] < iparams$ex.range[1]) | (cc$x[peakidx] > iparams$ex.range[2])] cc <- cc[peakidx,] # Find max peak position and other peaks within 0.9*max_peakvalue that are further away from maxpeakposition maxpeakidx <- which.max(cc$y) maxpeakshift <- cc$x[maxpeakidx] maxpeakval <- cc$y[maxpeakidx] peakidx <-which((cc$y >= 0.9*maxpeakval) & (cc$x >= maxpeakshift)) cc <- cc[peakidx,] # sort the peaks and get the top 3 sortidx <- order(cc$y,decreasing=TRUE) sortidx <- sortidx[c(1:min(3,length(sortidx)))] cc.peak <- cc[sortidx,] # Override peak shift if user supplies peak shift if (! is.na(iparams$sep.peak)) { cc.peak <- approx(crosscorr$cross.correlation$x,crosscorr$cross.correlation$y,iparams$sep.peak,rule=2) } cat("Peak cross-correlation value", paste(cc.peak$y,collapse=","),"\n",file=stdout()) cat("Peak strand shift",paste(cc.peak$x,collapse=","),"\n",file=stdout()) # Reset values in crosscorr crosscorr$peak$x <- cc.peak$x[1] crosscorr$peak$y <- cc.peak$y[1] # Compute window half size whs.thresh <- crosscorr$min.cc$y + (crosscorr$peak$y - crosscorr$min.cc$y)/3 crosscorr$whs <- max(crosscorr$cross.correlation$x[crosscorr$cross.correlation$y >= whs.thresh]) cat("Window half size",crosscorr$whs,"\n",file=stdout()) # Compute phantom peak coefficient ph.peakidx <- which( ( crosscorr$cross.correlation$x >= ( chip.data$read.length - round(2*iparams$sep.range[2]) ) ) & ( crosscorr$cross.correlation$x <= ( chip.data$read.length + round(1.5*iparams$sep.range[2]) ) ) ) ph.peakidx <- ph.peakidx[ which.max(crosscorr$cross.correlation$y[ph.peakidx]) ] crosscorr$phantom.cc <- crosscorr$cross.correlation[ph.peakidx,] cat("Phantom peak location",crosscorr$phantom.cc$x,"\n",file=stdout()) cat("Phantom peak Correlation",crosscorr$phantom.cc$y,"\n",file=stdout()) crosscorr$phantom.coeff <- crosscorr$peak$y / crosscorr$phantom.cc$y crosscorr$phantom.coeff <- crosscorr$peak$y / crosscorr$min.cc$y cat("Normalized cross-correlation coefficient (NCCC)",crosscorr$phantom.coeff,"\n",file=stdout()) crosscorr$rel.phantom.coeff <- (crosscorr$peak$y - crosscorr$min.cc$y) / (crosscorr$phantom.cc$y - crosscorr$min.cc$y) cat("Relative Cross correlation Coefficient (RCCC)",crosscorr$rel.phantom.coeff,"\n",file=stdout()) crosscorr$phantom.quality.tag <- NA if ( (crosscorr$rel.phantom.coeff >= 0) & (crosscorr$rel.phantom.coeff < 0.25) ) { crosscorr$phantom.quality.tag <- -2 } else if ( (crosscorr$rel.phantom.coeff >= 0.25) & (crosscorr$rel.phantom.coeff < 0.5) ) { crosscorr$phantom.quality.tag <- -1 } else if ( (crosscorr$rel.phantom.coeff >= 0.5) & (crosscorr$rel.phantom.coeff < 1) ) { crosscorr$phantom.quality.tag <- 0 } else if ( (crosscorr$rel.phantom.coeff >= 1) & (crosscorr$rel.phantom.coeff < 1.5) ) { crosscorr$phantom.quality.tag <- 1 } else if ( (crosscorr$rel.phantom.coeff >= 1.5) ) { crosscorr$phantom.quality.tag <- 2 } cat("Phantom Peak Quality Tag",crosscorr$phantom.quality.tag,"\n",file=stdout()) # Output result to result file if required #Filename\tnumReads\tPeak_shift\tPeak_Correlation\tRead_length\tPhantomPeak_Correlation\tMin_Correlation_Shift\tMin_Correlation\tNormalized_CrossCorrelation_Coefficient\tRelative_CrossCorrelation_Coefficient\tQualityTag) if (! is.na(iparams$output.result.file)) { cat(get.file.parts(iparams$chip.file)$fullname, chip.data$num.tags, paste(cc.peak$x,collapse=","), paste(cc.peak$y,collapse=","), crosscorr$phantom.cc$x, crosscorr$phantom.cc$y, crosscorr$min.cc$x, crosscorr$min.cc$y, crosscorr$phantom.coeff, crosscorr$rel.phantom.coeff, crosscorr$phantom.quality.tag, sep="\t", file=iparams$output.result.file, append=TRUE) cat("\n", file=iparams$output.result.file, append=TRUE) } # Save figure if required if (! is.na(iparams$output.plot.file)) { pdf(file=iparams$output.plot.file,width=5,height=5) par(mar = c(4,3.5,2,0.5), mgp = c(1.5,0.5,0), cex = 0.8); plot(crosscorr$cross.correlation, type='l', xlab=sprintf("strand-shift (%s)",paste(cc.peak$x,collapse=",")), ylab="cross-correlation") abline(v=cc.peak$x,lty=2,col=2) abline(v=crosscorr$phantom.cc$x,lty=2,col=4) title(main=get.file.parts(iparams$chip.file)$fullname, sub=sprintf("NSC=%g,RSC=%g,Qtag=%d",crosscorr$phantom.coeff,crosscorr$rel.phantom.coeff,crosscorr$phantom.quality.tag)) dev.off(); } # Save RData file if required if (! is.na(iparams$output.rdata.file)) { save(iparams, crosscorr, cc.peak, file=iparams$output.rdata.file); } # ################################# # Call peaks # ################################# if ( !is.na(iparams$output.npeak.file) || !is.na(iparams$output.rpeak.file) ) { # Remove local tag anomalies cat('Removing read stacks\n',file=stdout()) chip.data <- remove.local.tag.anomalies(chip.data$tags) control.data <- remove.local.tag.anomalies(control.data$tags) # Open multiple processes if required if (is.na(iparams$n.nodes)) { cluster.nodes <- NULL } else { cluster.nodes <- makeCluster(iparams$n.nodes) } # Find peaks cat('Finding peaks\n',file=stdout()) if (!is.na(iparams$npeak)) { iparams$fdr <- 0.96 } narrow.peaks <- find.binding.positions(signal.data=chip.data,control.data=control.data,fdr=iparams$fdr,method=tag.lwcc,whs=crosscorr$whs,cluster=cluster.nodes) if (!is.na(iparams$n.nodes)) { stopCluster(cluster.nodes) } cat(paste("Detected",sum(unlist(lapply(narrow.peaks$npl,function(d) length(d$x)))),"peaks"),"\n",file=stdout()) # Write to narrowPeak file if (!is.na(iparams$output.npeak.file)) { write.narrowpeak.binding(narrow.peaks,iparams$output.npeak.file,margin=round(crosscorr$whs/2),npeaks=iparams$npeak) #system(paste('gzip -f ',iparams$output.npeak.file)) } # Compute and write regionPeak file if (!is.na(iparams$output.rpeak.file)) { region.peaks <- add.broad.peak.regions(chip.data,control.data,narrow.peaks,window.size=max(50,round(crosscorr$whs/4)),z.thr=10) write.narrowpeak.binding(region.peaks,iparams$output.rpeak.file,margin=round(crosscorr$whs/2),npeaks=iparams$npeak) #system(paste('gzip -f ',iparams$output.rpeak.file)) } # Save Rdata file if (! is.na(iparams$output.rdata.file)) { save(iparams, crosscorr, cc.peak, narrow.peaks, region.peaks, file=iparams$output.rdata.file); } }