Mercurial > repos > davidvanzessen > shm_csr
view baseline/Baseline_Main.r @ 66:43a1aa648537 draft
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author | davidvanzessen |
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date | Thu, 07 Dec 2017 03:44:38 -0500 |
parents | c33d93683a09 |
children | ba33b94637ca |
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######################################################################################### # License Agreement # # THIS WORK IS PROVIDED UNDER THE TERMS OF THIS CREATIVE COMMONS PUBLIC LICENSE # ("CCPL" OR "LICENSE"). THE WORK IS PROTECTED BY COPYRIGHT AND/OR OTHER # APPLICABLE LAW. ANY USE OF THE WORK OTHER THAN AS AUTHORIZED UNDER THIS LICENSE # OR COPYRIGHT LAW IS PROHIBITED. # # BY EXERCISING ANY RIGHTS TO THE WORK PROVIDED HERE, YOU ACCEPT AND AGREE TO BE # BOUND BY THE TERMS OF THIS LICENSE. TO THE EXTENT THIS LICENSE MAY BE CONSIDERED # TO BE A CONTRACT, THE LICENSOR GRANTS YOU THE RIGHTS CONTAINED HERE IN # CONSIDERATION OF YOUR ACCEPTANCE OF SUCH TERMS AND CONDITIONS. # # BASELIne: Bayesian Estimation of Antigen-Driven Selection in Immunoglobulin Sequences # Coded by: Mohamed Uduman & Gur Yaari # Copyright 2012 Kleinstein Lab # Version: 1.3 (01/23/2014) ######################################################################################### op <- options(); options(showWarnCalls=FALSE, showErrorCalls=FALSE, warn=-1) library('seqinr') if( F & Sys.info()[1]=="Linux"){ library("multicore") } # Load functions and initialize global variables source("Baseline_Functions.r") # Initialize parameters with user provided arguments arg <- commandArgs(TRUE) #arg = c(2,1,5,5,0,1,"1:26:38:55:65:104:116", "test.fasta","","sample") #arg = c(1,1,5,5,0,1,"1:38:55:65:104:116:200", "test.fasta","","sample") #arg = c(1,1,5,5,1,1,"1:26:38:55:65:104:116", "/home/mu37/Wu/Wu_Cloned_gapped_sequences_D-masked.fasta","/home/mu37/Wu/","Wu") testID <- as.numeric(arg[1]) # 1 = Focused, 2 = Local species <- as.numeric(arg[2]) # 1 = Human. 2 = Mouse substitutionModel <- as.numeric(arg[3]) # 0 = Uniform substitution, 1 = Smith DS et al. 1996, 5 = FiveS mutabilityModel <- as.numeric(arg[4]) # 0 = Uniform mutablity, 1 = Tri-nucleotide (Shapiro GS et al. 2002) , 5 = FiveS clonal <- as.numeric(arg[5]) # 0 = Independent sequences, 1 = Clonally related, 2 = Clonally related & only non-terminal mutations fixIndels <- as.numeric(arg[6]) # 0 = Do nothing, 1 = Try and fix Indels region <- as.numeric(strsplit(arg[7],":")[[1]]) # StartPos:LastNucleotideF1:C1:F2:C2:F3:C3 inputFilePath <- arg[8] # Full path to input file outputPath <- arg[9] # Full path to location of output files outputID <- arg[10] # ID for session output if(testID==5){ traitChangeModel <- 1 if( !is.na(any(arg[11])) ) traitChangeModel <- as.numeric(arg[11]) # 1 <- Chothia 1998 initializeTraitChange(traitChangeModel) } # Initialize other parameters/variables # Initialzie the codon table ( definitions of R/S ) computeCodonTable(testID) # Initialize # Test Name testName<-"Focused" if(testID==2) testName<-"Local" if(testID==3) testName<-"Imbalanced" if(testID==4) testName<-"ImbalancedSilent" # Indel placeholders initialization indelPos <- NULL delPos <- NULL insPos <- NULL # Initialize in Tranistion & Mutability matrixes substitution <- initializeSubstitutionMatrix(substitutionModel,species) mutability <- initializeMutabilityMatrix(mutabilityModel,species) # FWR/CDR boundaries flagTrim <- F if( is.na(region[7])){ flagTrim <- T region[7]<-region[6] } readStart = min(region,na.rm=T) readEnd = max(region,na.rm=T) if(readStart>1){ region = region - (readStart - 1) } region_Nuc = c( (region[1]*3-2) , (region[2:7]*3) ) region_Cod = region readStart = (readStart*3)-2 readEnd = (readEnd*3) FWR_Nuc <- c( rep(TRUE,(region_Nuc[2])), rep(FALSE,(region_Nuc[3]-region_Nuc[2])), rep(TRUE,(region_Nuc[4]-region_Nuc[3])), rep(FALSE,(region_Nuc[5]-region_Nuc[4])), rep(TRUE,(region_Nuc[6]-region_Nuc[5])), rep(FALSE,(region_Nuc[7]-region_Nuc[6])) ) CDR_Nuc <- (1-FWR_Nuc) CDR_Nuc <- as.logical(CDR_Nuc) FWR_Nuc_Mat <- matrix( rep(FWR_Nuc,4), ncol=length(FWR_Nuc), nrow=4, byrow=T) CDR_Nuc_Mat <- matrix( rep(CDR_Nuc,4), ncol=length(CDR_Nuc), nrow=4, byrow=T) FWR_Codon <- c( rep(TRUE,(region[2])), rep(FALSE,(region[3]-region[2])), rep(TRUE,(region[4]-region[3])), rep(FALSE,(region[5]-region[4])), rep(TRUE,(region[6]-region[5])), rep(FALSE,(region[7]-region[6])) ) CDR_Codon <- (1-FWR_Codon) CDR_Codon <- as.logical(CDR_Codon) # Read input FASTA file tryCatch( inputFASTA <- baseline.read.fasta(inputFilePath, seqtype="DNA",as.string=T,set.attributes=F,forceDNAtolower=F) , error = function(ex){ cat("Error|Error reading input. Please enter or upload a valid FASTA file.\n") q() } ) if (length(inputFASTA)==1) { cat("Error|Error reading input. Please enter or upload a valid FASTA file.\n") q() } # Process sequence IDs/names names(inputFASTA) <- sapply(names(inputFASTA),function(x){trim(x)}) # Convert non nucleotide characters to N inputFASTA[length(inputFASTA)] = gsub("\t","",inputFASTA[length(inputFASTA)]) inputFASTA <- lapply(inputFASTA,replaceNonFASTAChars) # Process the FASTA file and conver to Matrix[inputSequence, germlineSequence] processedInput <- processInputAdvanced(inputFASTA) matInput <- processedInput[[1]] germlines <- processedInput[[2]] lenGermlines = length(unique(germlines)) groups <- processedInput[[3]] lenGroups = length(unique(groups)) rm(processedInput) rm(inputFASTA) # # remove clones with less than 2 seqeunces # tableGL <- table(germlines) # singletons <- which(tableGL<8) # rowsToRemove <- match(singletons,germlines) # if(any(rowsToRemove)){ # matInput <- matInput[-rowsToRemove,] # germlines <- germlines[-rowsToRemove] # groups <- groups[-rowsToRemove] # } # # # remove unproductive seqs # nonFuctionalSeqs <- sapply(rownames(matInput),function(x){any(grep("unproductive",x))}) # if(any(nonFuctionalSeqs)){ # if(sum(nonFuctionalSeqs)==length(germlines)){ # write.table("Unproductive",file=paste(outputPath,outputID,".txt",sep=""),quote=F,sep="\t",row.names=F,col.names=T) # q() # } # matInput <- matInput[-which(nonFuctionalSeqs),] # germlines <- germlines[-which(nonFuctionalSeqs)] # germlines[1:length(germlines)] <- 1:length(germlines) # groups <- groups[-which(nonFuctionalSeqs)] # } # # if(class(matInput)=="character"){ # write.table("All unproductive seqs",file=paste(outputPath,outputID,".txt",sep=""),quote=F,sep="\t",row.names=F,col.names=T) # q() # } # # if(nrow(matInput)<10 | is.null(nrow(matInput))){ # write.table(paste(nrow(matInput), "seqs only",sep=""),file=paste(outputPath,outputID,".txt",sep=""),quote=F,sep="\t",row.names=F,col.names=T) # q() # } # replace leading & trailing "-" with "N: matInput <- t(apply(matInput,1,replaceLeadingTrailingDashes,readEnd)) # Trim (nucleotide) input sequences to the last codon #matInput[,1] <- apply(matrix(matInput[,1]),1,trimToLastCodon) # # Check for Indels # if(fixIndels){ # delPos <- fixDeletions(matInput) # insPos <- fixInsertions(matInput) # }else{ # # Check for indels # indelPos <- checkForInDels(matInput) # indelPos <- apply(cbind(indelPos[[1]],indelPos[[2]]),1,function(x){(x[1]==T & x[2]==T)}) # } # If indels are present, remove mutations in the seqeunce & throw warning at end #matInput[indelPos,] <- apply(matrix(matInput[indelPos,],nrow=sum(indelPos),ncol=2),1,function(x){x[1]=x[2]; return(x) }) colnames(matInput)=c("Input","Germline") # If seqeunces are clonal, create effective sequence for each clone & modify germline/group definitions germlinesOriginal = NULL if(clonal){ germlinesOriginal <- germlines collapseCloneResults <- tapply(1:nrow(matInput),germlines,function(i){ collapseClone(matInput[i,1],matInput[i[1],2],readEnd,nonTerminalOnly=(clonal-1)) }) matInput = t(sapply(collapseCloneResults,function(x){return(x[[1]])})) names_groups = tapply(groups,germlines,function(x){names(x[1])}) groups = tapply(groups,germlines,function(x){array(x[1],dimnames=names(x[1]))}) names(groups) = names_groups names_germlines = tapply(germlines,germlines,function(x){names(x[1])}) germlines = tapply( germlines,germlines,function(x){array(x[1],dimnames=names(x[1]))} ) names(germlines) = names_germlines matInputErrors = sapply(collapseCloneResults,function(x){return(x[[2]])}) } # Selection Analysis # if (length(germlines)>sequenceLimit) { # # Code to parallelize processing goes here # stop( paste("Error: Cannot process more than ", Upper_limit," sequences",sep="") ) # } # if (length(germlines)<sequenceLimit) {} # Compute expected mutation frequencies matExpected <- getExpectedIndividual(matInput) # Count observed number of mutations in the different regions mutations <- lapply( 1:nrow(matInput), function(i){ #cat(i,"\n") seqI = s2c(matInput[i,1]) seqG = s2c(matInput[i,2]) matIGL = matrix(c(seqI,seqG),ncol=length(seqI),nrow=2,byrow=T) retVal <- NA tryCatch( retVal <- analyzeMutations2NucUri(matIGL) , error = function(ex){ retVal <- NA } ) return( retVal ) }) matObserved <- t(sapply( mutations, processNucMutations2 )) numberOfSeqsWithMutations <- numberOfSeqsWithMutations(matObserved, testID) #if(sum(numberOfSeqsWithMutations)==0){ # write.table("No mutated sequences",file=paste(outputPath,outputID,".txt",sep=""),quote=F,sep="\t",row.names=F,col.names=T) # q() #} matMutationInfo <- cbind(matObserved,matExpected) rm(matObserved,matExpected) #Bayesian PDFs bayes_pdf = computeBayesianScore(matMutationInfo, test=testName, max_sigma=20,length_sigma=4001) bayesPDF_cdr = bayes_pdf[[1]] bayesPDF_fwr = bayes_pdf[[2]] rm(bayes_pdf) bayesPDF_germlines_cdr = tapply(bayesPDF_cdr,germlines,function(x) groupPosteriors(x,length_sigma=4001)) bayesPDF_germlines_fwr = tapply(bayesPDF_fwr,germlines,function(x) groupPosteriors(x,length_sigma=4001)) bayesPDF_groups_cdr = tapply(bayesPDF_cdr,groups,function(x) groupPosteriors(x,length_sigma=4001)) bayesPDF_groups_fwr = tapply(bayesPDF_fwr,groups,function(x) groupPosteriors(x,length_sigma=4001)) if(lenGroups>1){ groups <- c(groups,lenGroups+1) names(groups)[length(groups)] = "All sequences combined" bayesPDF_groups_cdr[[lenGroups+1]] = groupPosteriors(bayesPDF_groups_cdr,length_sigma=4001) bayesPDF_groups_fwr[[lenGroups+1]] = groupPosteriors(bayesPDF_groups_fwr,length_sigma=4001) } #Bayesian Outputs bayes_cdr = t(sapply(bayesPDF_cdr,calcBayesOutputInfo)) bayes_fwr = t(sapply(bayesPDF_fwr,calcBayesOutputInfo)) bayes_germlines_cdr = t(sapply(bayesPDF_germlines_cdr,calcBayesOutputInfo)) bayes_germlines_fwr = t(sapply(bayesPDF_germlines_fwr,calcBayesOutputInfo)) bayes_groups_cdr = t(sapply(bayesPDF_groups_cdr,calcBayesOutputInfo)) bayes_groups_fwr = t(sapply(bayesPDF_groups_fwr,calcBayesOutputInfo)) #P-values simgaP_cdr = sapply(bayesPDF_cdr,computeSigmaP) simgaP_fwr = sapply(bayesPDF_fwr,computeSigmaP) simgaP_germlines_cdr = sapply(bayesPDF_germlines_cdr,computeSigmaP) simgaP_germlines_fwr = sapply(bayesPDF_germlines_fwr,computeSigmaP) simgaP_groups_cdr = sapply(bayesPDF_groups_cdr,computeSigmaP) simgaP_groups_fwr = sapply(bayesPDF_groups_fwr,computeSigmaP) #Format output # Round expected mutation frequencies to 3 decimal places matMutationInfo[germlinesOriginal[indelPos],] = NA if(nrow(matMutationInfo)==1){ matMutationInfo[5:8] = round(matMutationInfo[,5:8]/sum(matMutationInfo[,5:8],na.rm=T),3) }else{ matMutationInfo[,5:8] = t(round(apply(matMutationInfo[,5:8],1,function(x){ return(x/sum(x,na.rm=T)) }),3)) } listPDFs = list() nRows = length(unique(groups)) + length(unique(germlines)) + length(groups) matOutput = matrix(NA,ncol=18,nrow=nRows) rowNumb = 1 for(G in unique(groups)){ #print(G) matOutput[rowNumb,c(1,2,11:18)] = c("Group",names(groups)[groups==G][1],bayes_groups_cdr[G,],bayes_groups_fwr[G,],simgaP_groups_cdr[G],simgaP_groups_fwr[G]) listPDFs[[rowNumb]] = list("CDR"=bayesPDF_groups_cdr[[G]],"FWR"=bayesPDF_groups_fwr[[G]]) names(listPDFs)[rowNumb] = names(groups[groups==paste(G)])[1] #if(names(groups)[which(groups==G)[1]]!="All sequences combined"){ gs = unique(germlines[groups==G]) rowNumb = rowNumb+1 if( !is.na(gs) ){ for( g in gs ){ matOutput[rowNumb,c(1,2,11:18)] = c("Germline",names(germlines)[germlines==g][1],bayes_germlines_cdr[g,],bayes_germlines_fwr[g,],simgaP_germlines_cdr[g],simgaP_germlines_fwr[g]) listPDFs[[rowNumb]] = list("CDR"=bayesPDF_germlines_cdr[[g]],"FWR"=bayesPDF_germlines_fwr[[g]]) names(listPDFs)[rowNumb] = names(germlines[germlines==paste(g)])[1] rowNumb = rowNumb+1 indexesOfInterest = which(germlines==g) numbSeqsOfInterest = length(indexesOfInterest) rowNumb = seq(rowNumb,rowNumb+(numbSeqsOfInterest-1)) matOutput[rowNumb,] = matrix( c( rep("Sequence",numbSeqsOfInterest), rownames(matInput)[indexesOfInterest], c(matMutationInfo[indexesOfInterest,1:4]), c(matMutationInfo[indexesOfInterest,5:8]), c(bayes_cdr[indexesOfInterest,]), c(bayes_fwr[indexesOfInterest,]), c(simgaP_cdr[indexesOfInterest]), c(simgaP_fwr[indexesOfInterest]) ), ncol=18, nrow=numbSeqsOfInterest,byrow=F) increment=0 for( ioi in indexesOfInterest){ listPDFs[[min(rowNumb)+increment]] = list("CDR"=bayesPDF_cdr[[ioi]] , "FWR"=bayesPDF_fwr[[ioi]]) names(listPDFs)[min(rowNumb)+increment] = rownames(matInput)[ioi] increment = increment + 1 } rowNumb=max(rowNumb)+1 } } } colsToFormat = 11:18 matOutput[,colsToFormat] = formatC( matrix(as.numeric(matOutput[,colsToFormat]), nrow=nrow(matOutput), ncol=length(colsToFormat)) , digits=3) matOutput[matOutput== " NaN"] = NA colnames(matOutput) = c("Type", "ID", "Observed_CDR_R", "Observed_CDR_S", "Observed_FWR_R", "Observed_FWR_S", "Expected_CDR_R", "Expected_CDR_S", "Expected_FWR_R", "Expected_FWR_S", paste( rep(testName,6), rep(c("Sigma","CIlower","CIupper"),2),rep(c("CDR","FWR"),each=3), sep="_"), paste( rep(testName,2), rep("P",2),c("CDR","FWR"), sep="_") ) fileName = paste(outputPath,outputID,".txt",sep="") write.table(matOutput,file=fileName,quote=F,sep="\t",row.names=T,col.names=NA) fileName = paste(outputPath,outputID,".RData",sep="") save(listPDFs,file=fileName) indelWarning = FALSE if(sum(indelPos)>0){ indelWarning = "<P>Warning: The following sequences have either gaps and/or deletions, and have been ommited from the analysis."; indelWarning = paste( indelWarning , "<UL>", sep="" ) for(indels in names(indelPos)[indelPos]){ indelWarning = paste( indelWarning , "<LI>", indels, "</LI>", sep="" ) } indelWarning = paste( indelWarning , "</UL></P>", sep="" ) } cloneWarning = FALSE if(clonal==1){ if(sum(matInputErrors)>0){ cloneWarning = "<P>Warning: The following clones have sequences of unequal length."; cloneWarning = paste( cloneWarning , "<UL>", sep="" ) for(clone in names(matInputErrors)[matInputErrors]){ cloneWarning = paste( cloneWarning , "<LI>", names(germlines)[as.numeric(clone)], "</LI>", sep="" ) } cloneWarning = paste( cloneWarning , "</UL></P>", sep="" ) } } cat(paste("Success",outputID,indelWarning,cloneWarning,sep="|"))