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R/mergePlusMinusPeaks.R
In ChIPpeakAnno: Batch annotation of the peaks identified from either ChIP-seq, ChIP-chip experiments or any experiments resulted in large number of chromosome ranges
Defines functions
mergePlusMinusPeaks
Documented in
mergePlusMinusPeaks
#' Merge peaks from plus strand and minus strand
#'
#' Merge peaks from plus strand and minus strand within certain distance apart,
#' and output merged peaks as bed format.
#'
#'
#' @param peaks.file Specify the peak file. The peak file should contain peaks
#' from both plus and minus strand
#' @param columns Specify the column names in the peak file
#' @param sep Specify column delimiter, default tab-delimited
#' @param header Specify whether the file has a header row, default TRUE
#' @param distance.threshold Specify the maximum gap allowed between the plus
#' stranded and the nagative stranded peak
#' @param plus.strand.start.gt.minus.strand.end Specify whether plus strand
#' peak start greater than the paired negative strand peak end. Default to TRUE
#' @param output.bedfile Specify the bed output file name
#' @return output the merged peaks in bed file and a data frame of the bed
#' format
#' @author Lihua Julie Zhu
#' @seealso annotatePeakInBatch, findOverlappingPeaks, makeVennDiagram
#' @references Zhu L.J. et al. (2010) ChIPpeakAnno: a Bioconductor package to
#' annotate ChIP-seq and ChIP-chip data. BMC Bioinformatics 2010,
#' 11:237doi:10.1186/1471-2105-11-237
#' @keywords misc
#' @export
#' @importFrom matrixStats rowMins rowMaxs
#' @importFrom utils read.table write.table
#' @examples
#'
#'
#' if (interactive())
#' {
#' data(myPeakList)
#' data(TSS.human.NCBI36)
#' library(matrixStats)
#' peaks <- system.file("extdata", "guide-seq-peaks.txt",
#' package = "ChIPpeakAnno")
#' merged.bed <- mergePlusMinusPeaks(peaks.file = peaks,
#' columns=c("name", "chromosome",
#' "start", "end", "strand",
#' "count", "count"),
#' sep = "\t", header = TRUE,
#' distance.threshold = 100,
#' plus.strand.start.gt.minus.strand.end = TRUE,
#' output.bedfile = "T2test100bp.bed")
#' }
#'
mergePlusMinusPeaks <- function(peaks.file,
columns=c("name", "chromosome", "start",
"end", "strand", "count",
"count", "count", "count"),
sep = "\t", header = TRUE,
distance.threshold = 100,
plus.strand.start.gt.minus.strand.end = TRUE,
output.bedfile)
{
peaks<- read.table (peaks.file, sep = sep, header = header)
if (dim(peaks)[2] != length(columns))
stop("Number of columns specified differs from the number of columns
in the input peak file, please modify the column specification
in parameter columns accordingly!")
if (length(intersect(columns, "strand")) != 1)
stop("Please include one strand column in columns and
corresponding peaks.file")
colnames(peaks) <- columns
pos.peaks <- subset(peaks, peaks[, which(columns == "strand")] == "+")
neg.peaks <- subset(peaks, peaks[, which(columns == "strand")] == "-")
if (dim(pos.peaks)[1] == 0 || dim(neg.peaks)[1] == 0)
stop("Need peaks from both + and - strand to merge")
pos.gr <- makeGRangesFromDataFrame(pos.peaks)
neg.gr <- makeGRangesFromDataFrame(neg.peaks)
names(pos.gr) <- paste(paste(seqnames(pos.gr), strand(pos.gr), sep=""),
start(pos.gr),end(pos.gr), sep=":")
names(neg.gr) <- paste(paste(seqnames(neg.gr), strand(neg.gr), sep=""),
start(neg.gr),end(neg.gr), sep=":")
if (plus.strand.start.gt.minus.strand.end)
gr <- annotatePeakInBatch(pos.gr, featureType = "TSS",
AnnotationData = neg.gr,
output="nearestStart",
PeakLocForDistance = "TSS")
else
gr <- annotatePeakInBatch(neg.gr, featureType = "TSS",
AnnotationData = pos.gr,
output="nearestStart",
PeakLocForDistance = "end")
pos.peaks <-
cbind(peak = paste(paste(pos.peaks[,which(columns == "chromosome")],
"+", sep = ""),
pos.peaks[,which(columns == "start")],
pos.peaks[,which(columns == "end")], sep=":"),
pos.peaks)
neg.peaks <-
cbind(feature = paste(paste(neg.peaks[,which(columns == "chromosome")],
"-", sep = ""),
neg.peaks[,which(columns == "start")],
neg.peaks[,which(columns == "end")], sep=":"),
neg.peaks)
if (!plus.strand.start.gt.minus.strand.end)
{
colnames(pos.peaks)[1] <- "feature"
colnames(neg.peaks)[1] <- "peak"
}
new.count.columns <- which(columns == "count") + 1
colnames(neg.peaks)[new.count.columns] <-
paste("minus", colnames(neg.peaks)[new.count.columns], sep=":")
colnames(pos.peaks)[new.count.columns] <-
paste("plus", colnames(pos.peaks)[new.count.columns], sep=":")
pos.peaks <- pos.peaks[, c(1, new.count.columns)]
neg.peaks <- neg.peaks[, c(1, new.count.columns)]
ann.peaks <- as.data.frame(gr[abs(gr$distancetoFeature) <=
distance.threshold &
gr$distancetoFeature < 0,])
temp <- merge(pos.peaks, ann.peaks)
temp1 <- merge(neg.peaks, temp)
temp1 <- cbind(temp1,
totalCount = rowSums(temp1[,grep("count",
colnames(temp1))]))
temp1$names = paste(temp1$peak, temp1$feature, sep=":")
temp1$minStart <- rowMins(as.matrix(temp1[, c("start_position", "start")]))
temp1$maxEnd <- rowMaxs(as.matrix(temp1[, c("end_position", "end")]))
bed.temp <-
temp1[, c("seqnames", "minStart", "maxEnd", "names", "totalCount")]
bed.temp <- cbind(bed.temp, strand = "+")
write.table(bed.temp, file = output.bedfile, sep = "\t", col.names = FALSE,
row.names=FALSE, quote=FALSE)
bed.temp
}
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ChIPpeakAnno documentation built on April 1, 2021, 6:01 p.m.
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Defines functions mergePlusMinusPeaks
Documented in mergePlusMinusPeaks
#' Merge peaks from plus strand and minus strand
#'
#' Merge peaks from plus strand and minus strand within certain distance apart,
#' and output merged peaks as bed format.
#'
#'
#' @param peaks.file Specify the peak file. The peak file should contain peaks
#' from both plus and minus strand
#' @param columns Specify the column names in the peak file
#' @param sep Specify column delimiter, default tab-delimited
#' @param header Specify whether the file has a header row, default TRUE
#' @param distance.threshold Specify the maximum gap allowed between the plus
#' stranded and the nagative stranded peak
#' @param plus.strand.start.gt.minus.strand.end Specify whether plus strand
#' peak start greater than the paired negative strand peak end. Default to TRUE
#' @param output.bedfile Specify the bed output file name
#' @return output the merged peaks in bed file and a data frame of the bed
#' format
#' @author Lihua Julie Zhu
#' @seealso annotatePeakInBatch, findOverlappingPeaks, makeVennDiagram
#' @references Zhu L.J. et al. (2010) ChIPpeakAnno: a Bioconductor package to
#' annotate ChIP-seq and ChIP-chip data. BMC Bioinformatics 2010,
#' 11:237doi:10.1186/1471-2105-11-237
#' @keywords misc
#' @export
#' @importFrom matrixStats rowMins rowMaxs
#' @importFrom utils read.table write.table
#' @examples
#'
#'
#' if (interactive())
#' {
#' data(myPeakList)
#' data(TSS.human.NCBI36)
#' library(matrixStats)
#' peaks <- system.file("extdata", "guide-seq-peaks.txt",
#' package = "ChIPpeakAnno")
#' merged.bed <- mergePlusMinusPeaks(peaks.file = peaks,
#' columns=c("name", "chromosome",
#' "start", "end", "strand",
#' "count", "count"),
#' sep = "\t", header = TRUE,
#' distance.threshold = 100,
#' plus.strand.start.gt.minus.strand.end = TRUE,
#' output.bedfile = "T2test100bp.bed")
#' }
#'
mergePlusMinusPeaks <- function(peaks.file,
columns=c("name", "chromosome", "start",
"end", "strand", "count",
"count", "count", "count"),
sep = "\t", header = TRUE,
distance.threshold = 100,
plus.strand.start.gt.minus.strand.end = TRUE,
output.bedfile)
{
peaks<- read.table (peaks.file, sep = sep, header = header)
if (dim(peaks)[2] != length(columns))
stop("Number of columns specified differs from the number of columns
in the input peak file, please modify the column specification
in parameter columns accordingly!")
if (length(intersect(columns, "strand")) != 1)
stop("Please include one strand column in columns and
corresponding peaks.file")
colnames(peaks) <- columns
pos.peaks <- subset(peaks, peaks[, which(columns == "strand")] == "+")
neg.peaks <- subset(peaks, peaks[, which(columns == "strand")] == "-")
if (dim(pos.peaks)[1] == 0 || dim(neg.peaks)[1] == 0)
stop("Need peaks from both + and - strand to merge")
pos.gr <- makeGRangesFromDataFrame(pos.peaks)
neg.gr <- makeGRangesFromDataFrame(neg.peaks)
names(pos.gr) <- paste(paste(seqnames(pos.gr), strand(pos.gr), sep=""),
start(pos.gr),end(pos.gr), sep=":")
names(neg.gr) <- paste(paste(seqnames(neg.gr), strand(neg.gr), sep=""),
start(neg.gr),end(neg.gr), sep=":")
if (plus.strand.start.gt.minus.strand.end)
gr <- annotatePeakInBatch(pos.gr, featureType = "TSS",
AnnotationData = neg.gr,
output="nearestStart",
PeakLocForDistance = "TSS")
else
gr <- annotatePeakInBatch(neg.gr, featureType = "TSS",
AnnotationData = pos.gr,
output="nearestStart",
PeakLocForDistance = "end")
pos.peaks <-
cbind(peak = paste(paste(pos.peaks[,which(columns == "chromosome")],
"+", sep = ""),
pos.peaks[,which(columns == "start")],
pos.peaks[,which(columns == "end")], sep=":"),
pos.peaks)
neg.peaks <-
cbind(feature = paste(paste(neg.peaks[,which(columns == "chromosome")],
"-", sep = ""),
neg.peaks[,which(columns == "start")],
neg.peaks[,which(columns == "end")], sep=":"),
neg.peaks)
if (!plus.strand.start.gt.minus.strand.end)
{
colnames(pos.peaks)[1] <- "feature"
colnames(neg.peaks)[1] <- "peak"
}
new.count.columns <- which(columns == "count") + 1
colnames(neg.peaks)[new.count.columns] <-
paste("minus", colnames(neg.peaks)[new.count.columns], sep=":")
colnames(pos.peaks)[new.count.columns] <-
paste("plus", colnames(pos.peaks)[new.count.columns], sep=":")
pos.peaks <- pos.peaks[, c(1, new.count.columns)]
neg.peaks <- neg.peaks[, c(1, new.count.columns)]
ann.peaks <- as.data.frame(gr[abs(gr$distancetoFeature) <=
distance.threshold &
gr$distancetoFeature < 0,])
temp <- merge(pos.peaks, ann.peaks)
temp1 <- merge(neg.peaks, temp)
temp1 <- cbind(temp1,
totalCount = rowSums(temp1[,grep("count",
colnames(temp1))]))
temp1$names = paste(temp1$peak, temp1$feature, sep=":")
temp1$minStart <- rowMins(as.matrix(temp1[, c("start_position", "start")]))
temp1$maxEnd <- rowMaxs(as.matrix(temp1[, c("end_position", "end")]))
bed.temp <-
temp1[, c("seqnames", "minStart", "maxEnd", "names", "totalCount")]
bed.temp <- cbind(bed.temp, strand = "+")
write.table(bed.temp, file = output.bedfile, sep = "\t", col.names = FALSE,
row.names=FALSE, quote=FALSE)
bed.temp
}
Try the ChIPpeakAnno package in your browser
Any scripts or data that you put into this service are public.
R Package Documentation
Browse R Packages
We want your feedback!
Note that we can't provide technical support on individual packages. You should contact the package authors for that.
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