R/utils-general.R
In jmacdon/oligo: Preprocessing tools for oligonucleotide arrays
Defines functions
pair2xys
cloneFS
msgOK
txtMsg
readCEL
basicMvAplot
plotM
getBaseProfile
getAffinitySplineCoefficients
divColors
seqColors2
seqColors
darkColors
basicAnnotatedDataFrame
basicPhData2
basicPhData1
basicPData2
basicPData
AffyDate2Posix
NgsDate2Posix
GetAffyTimeDateAsString
stArrayPmInfo
getFidMetaProbesetExtended
getFidMetaProbesetFull
getFidMetaProbesetCore
getFidProbeset
getNgsColorsInfo
getFilenames
basecontent
sequenceDesignMatrix
checkChipTypes
getCelChipType
checkValidFilenames
trigammaInverse
HuberAllRowsByGroup
cleanPlatformName
Documented in
basecontent
cleanPlatformName
darkColors
divColors
getAffinitySplineCoefficients
getBaseProfile
getNgsColorsInfo
plotM
seqColors
seqColors2
sequenceDesignMatrix
cleanPlatformName <- function(x)
gsub("[_-]", ".", paste("pd.", tolower(x), sep=""))
HuberAllRowsByGroup <- function(X, Y, k=1.5){
.Call("R_HuberMatrixRows2",X, Y, k, PACKAGE="oligo")
}
trigammaInverse <- function(x) {
# Solve trigamma(y) = x for y
# Gordon Smyth
# 8 Sept 2002. Last revised 12 March 2004.
# Non-numeric or zero length input
if(!is.numeric(x)) stop("Non-numeric argument to mathematical function")
if(length(x)==0) return(numeric(0))
# Treat out-of-range values as special cases
omit <- is.na(x)
if(any(omit)) {
y <- x
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
omit <- (x < 0)
if(any(omit)) {
y <- x
y[omit] <- NaN
warning("NaNs produced")
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
omit <- (x > 1e7)
if(any(omit)) {
y <- x
y[omit] <- 1/sqrt(x[omit])
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
omit <- (x < 1e-6)
if(any(omit)) {
y <- x
y[omit] <- 1/x[omit]
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
# Newton's method
# 1/trigamma(y) is convex, nearly linear and strictly > y-0.5,
# so iteration to solve 1/x = 1/trigamma is monotonically convergent
y <- 0.5+1/x
iter <- 0
repeat {
iter <- iter+1
tri <- trigamma(y)
dif <- tri*(1-tri/x)/psigamma(y,deriv=2)
y <- y+dif
if(max(-dif/y) < 1e-8) break
if(iter > 50) {
warning("Iteration limit exceeded")
break
}
}
y
}
checkValidFilenames <- function(filenames) {
## must be character
stopifnot(is.character(filenames))
## must exist
dirs <- file.info(filenames)[["isdir"]]
if (any(is.na(dirs))){
msg <- paste("These do not exist:",
paste("\t", filenames[is.na(dirs)], collapse="\n"), sep="\n")
stop(msg, call.=FALSE)
}
## must be files, not dir
if (any(dirs)){
msg <- paste("These are directories:",
paste("\t", filenames[dirs], collapse="\n"), sep="\n")
stop(msg, call.=FALSE)
}
## must be readable
readable <- file.access(filenames, 4) == 0
if (any(!readable)){
msg <- paste("These are not readable:",
paste("\t", filenames[!readable], collapse="\n"), sep="\n")
stop(msg, call.=FALSE)
}
TRUE
}
## checkValidPhenodataForFiles <- function(filenames, pd){
## if (missing(pd)) return(FALSE)
## if (class(pd) != "AnnotatedDataFrame") return(FALSE)
## return(length(filenames) == nrow(pd))
## }
## createDefaultMiame <- function(filenames, notes){
## experimentData <- new("MIAME")
## preproc(experimentData)$filenames <- filenames
## preproc(experimentData)$oligoversion <- packageDescription("oligo", field="Version")
## if (!missing(notes))
## notes(experimentData) <- notes
## experimentData
## }
getCelChipType <- function(x, useAffyio){
ifelse(useAffyio,
read.celfile.header(x)[["cdfName"]],
readCelHeader(x)[["chiptype"]])
}
checkChipTypes <- function(filenames, verbose=TRUE, manufacturer, useAffyio){
if (missing(manufacturer)) stop("'checkChipTypes' needs 'manufacturer'")
if (manufacturer == "affymetrix"){
chips <- sapply(filenames, getCelChipType, useAffyio)
ok <- length(unique(chips)) == 1
if(!ok & verbose) message("All the CEL files must be of the same type.")
}else if(manufacturer == "nimblegen"){
designnamelist <- NULL
for (xysfile in filenames){
firstline <- readxysHeader(xysfile)
designname <- unlist(strsplit(firstline[grep("designname",firstline,fixed=TRUE,useBytes=TRUE)],"="))[2]
designnamelist <- rbind(designnamelist,designname)
}
ok <- length(unique(designnamelist)) == 1
if(!ok & verbose) message("All the XYS files must be of the same type.")
}else{
stop("'manufacturer' ", manufacturer, " unknown")
}
ok
}
sequenceDesignMatrix <- function(seqs){
if(length(unique(sapply(seqs,nchar)))!=1) stop("Sequences must be of same length.")
oligolength <- nchar(seqs[1])
mat <- .Call("gcrma_getSeq2",paste(seqs,collapse=""),length(seqs),oligolength,PACKAGE="oligo")
colnames(mat) <- paste(rep(c("A","C","G"),rep(oligolength,3)),position=rep(1:oligolength,3),sep="_")
return(mat)
}
basecontent <- function(seq) {
good = !is.na(seq)
havena = !all(good)
if(havena)
seq = seq[good]
rv = .Call("basecontent", seq, PACKAGE="oligo")
if(havena) {
z = rv
rv = matrix(NA, nrow=length(good), ncol=ncol(z))
colnames(rv) = colnames(z)
rv[good, ] = z
}
return(rv)
}
## Helper to parse the dots and combine with filenames
getFilenames <- function(filenames, ...){
if (!missing(filenames)){
filenames <- c(filenames, unlist(list(...)))
}else{
filenames <- unlist(list(...))
}
filenames
}
getNgsColorsInfo <- function(path=".", pattern1="_532", pattern2="_635", ...){
files1 <- list.xysfiles(path, pattern=pattern1, ...)
files2 <- list.xysfiles(path, pattern=pattern2, ...)
prefix1 <- sapply(strsplit(basename(files1), pattern1), "[[", 1)
prefix2 <- sapply(strsplit(basename(files2), pattern2), "[[", 1)
sugg <- identical(prefix1, prefix2)
stopifnot(length(files1) == length(files2))
out <- data.frame(color1=files1, color2=files2, stringsAsFactors=FALSE)
if (sugg)
out[["sampleNames"]] <- prefix1
return(out)
}
## Selectors for probes - useful for exon/gene arrays
getFidProbeset <- function(object, sortBy='fsetid'){
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
conn <- db(object)
on.exit(dbDisconnect(conn))
if (!is(object, 'HTAFeatureSet')){
sql <- "SELECT fid, fsetid FROM pmfeature"
}else{
sql <- "SELECT fid, man_fsetid as fsetid FROM pmfeature INNER JOIN featureSet USING(fsetid)"
}
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
getFidMetaProbesetCore <- function(object, sortBy='fsetid'){
conn <- db(object)
on.exit(dbDisconnect(conn))
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
if (!is(object, 'HTAFeatureSet')){
sql <- "SELECT fid, meta_fsetid as fsetid FROM pmfeature INNER JOIN core_mps USING(fsetid)"
}else{
sql <- "SELECT fid, core_mps.transcript_cluster_id as fsetid FROM pmfeature INNER JOIN core_mps USING(fsetid)"
}
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
getFidMetaProbesetFull <- function(object, sortBy='fsetid'){
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
conn <- db(object)
on.exit(dbDisconnect(conn))
sql <- "SELECT fid, meta_fsetid as fsetid FROM pmfeature INNER JOIN full_mps USING(fsetid)"
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
getFidMetaProbesetExtended <- function(object, sortBy='fsetid'){
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
conn <- db(object)
on.exit(dbDisconnect(conn))
sql <- "SELECT fid, meta_fsetid as fsetid FROM pmfeature INNER JOIN extended_mps USING(fsetid)"
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
stArrayPmInfo <- function(object, target='core', sortBy='fsetid'){
## *PmInfo returns a data.frame with 'fid' and 'fsetid'
target <- match.arg(target, c('probeset', 'core', 'full', 'extended'))
theFun <- switch(target,
probeset=getFidProbeset,
core=getFidMetaProbesetCore,
full=getFidMetaProbesetFull,
extended=getFidMetaProbesetExtended)
theFun(object, sortBy=sortBy)
}
## Date/time extractors
GetAffyTimeDateAsString <- function(filenames){
f <- function(x) read.celfile.header(x, "full")[["ScanDate"]]
res <- sapply(filenames, f)
sapply(res, function(x) ifelse(length(x) == 0, NA_character_, x))
}
NgsDate2Posix <- function(txt){
if (!missing(txt)){
original <- txt
tmp <- gsub("(.* )(.{1,3}) ([0-9]{4})", "\\1\\3", txt)
out <- as.POSIXct(tmp, format="%A %B %d %H:%M:%S %Y")
if (any(is.na(out))){
warning("Returning dates/times as strings due to incompatibility.")
out <- original
}
}else{
out <- NULL
}
out
}
AffyDate2Posix <- function(txt){
if (!missing(txt)){
original <- txt
out <- as.POSIXct(txt, format="%m/%d/%y %H:%M:%S")
if (any(is.na(out))){
warning("Returning dates/times as strings - format not recognized.")
out <- original
}
}else{
out <- NULL
}
out
}
basicPData <- function(mat, filenames, dates){
if (missing(dates))
dates <- rep(NA, length(filenames))
stopifnot(length(filenames) == length(dates))
pdd <- data.frame(exprs=filenames, dates=dates)
vmd <- data.frame(labelDescription=c(
"Names of files used in 'exprs'",
"Run dates for files used in 'exprs'"),
channel=factor("_ALL_", levels=c("exprs", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat)
return(phenoData)
}
basicPData2 <- function(mat1, mat2, filenames1, filenames2,
dates1, dates2){
if (missing(dates1)) dates1 <- rep(NA, length(filenames1))
if (missing(dates2)) dates2 <- rep(NA, length(filenames2))
stopifnot(identical(colnames(mat1), colnames(mat2)),
length(filenames1) == length(filenames2),
length(dates1) == length(dates2))
pdd <- data.frame(filenamesChannel1=filenames1,
filenamesChannel2=filenames2,
dates1=dates1, dates2=dates2)
vmd <- data.frame(labelDescription=c(
"Names of files used in 'channel1'",
"Names of files used in 'channel2'",
"Run dates for files used in 'channel1'",
"Run dates for files used in 'channel2'"),
channel=factor(rep(c("channel1", "channel2"), 2),
levels=c("channel1", "channel2", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat1)
return(phenoData)
}
basicPhData1 <- function(mat){
pdd <- data.frame(index=1:ncol(mat))
vmd <- data.frame(labelDescription=c("Index"),
channel=factor("_ALL_", levels=c("exprs", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat)
return(phenoData)
}
basicPhData2 <- function(mat1, mat2){
stopifnot(identical(colnames(mat1), colnames(mat2)))
pdd <- data.frame(index=1:ncol(mat1))
vmd <- data.frame(labelDescription=c("Index"),
channel=factor("_ALL_",
levels=c("channel1", "channel2", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat1)
return(phenoData)
}
basicAnnotatedDataFrame <- function(mat, byrow=FALSE){
Biobase:::annotatedDataFrameFromMatrix(mat, byrow=byrow)
}
## colors I like in oligo
darkColors <- function(n){
cols <- c("#1B9E77", "#D95F02", "#7570B3", "#E7298A", "#66A61E",
"#E6AB02", "#A6761D", "#666666")
fff <- colorRampPalette(cols)
fff(n)
}
seqColors <- function(n){
cols <- c("#F7FBFF", "#DEEBF7", "#C6DBEF", "#9ECAE1", "#6BAED6",
"#4292C6", "#2171B5", "#08519C", "#08306B")
fff <- colorRampPalette(cols)
fff(n)
}
seqColors2 <- function(n){
cols <- c("#FFF7EC", "#FEE8C8", "#FDD49E", "#FDBB84", "#FC8D59",
"#EF6548", "#D7301F", "#B30000", "#7F0000")
fff <- colorRampPalette(cols)
fff(n)
}
divColors <- function(n){
cols <- c("#053061", "#2166AC", "#4393C3", "#92C5DE", "#D1E5F0",
"#FDDBC7", "#F4A582", "#D6604D", "#B2182B", "#67001F")
fff <- colorRampPalette(cols)
fff(n)
}
## gcrma-like stuff
## from jean
getAffinitySplineCoefficients <- function(intensities, sequences){
if (is(sequences, "DNAStringSet"))
sequences <- as.character(sequences)
stopifnot(is.character(sequences))
stopifnot(is.matrix(intensities))
design <- sequenceDesignMatrix(sequences)
rm(sequences)
B <- ns(1:25, df=5)
design <- cbind(design[, 1:25] %*% B,
design[, 26:50] %*% B,
design[, 51:75] %*% B)
fits <- lm(intensities~design)
coefs <- coef(fits)[-1,]
rownames(coefs) <- rep(c("A", "C", "G"), each=5)
coefs
}
getBaseProfile <- function(coefs, probeLength=25, plot=FALSE, ...){
stopifnot(is.vector(coefs))
P <- as.integer(length(coefs)/3)
B <- ns(1:probeLength, df=5)
effects <- matrix(0, nrow=probeLength, ncol=4)
colnames(effects) <- c("A", "C", "G", "T")
for (i in 1:3)
effects[, i] <- B %*% coefs[(i-1)*P + (1:P)]
effects <- sweep(effects, 1, rowMeans(effects))
if(plot) matplot(1:probeLength, effects, ...)
invisible(effects)
}
## SnpSuperSet method?
plotM <- function(x, snp, ...){
crlmmInfo <- file.path(system.file("extdata", package=annotation(x)),
paste(annotation(x), "CrlmmInfo.rda", sep=""))
infoObj <- load(crlmmInfo)
f0 <- get(infoObj)$params$f0
rm(list=infoObj)
obj <- x[snp,]
theM <- getM(obj)[,,]
theF <- cbind(antisense=assayDataElement(obj, "antisenseF")[,],
sense=assayDataElement(obj, "senseF")[,])
theCalls <- calls(obj)[,]
correctedM <- theM + (theCalls - 2) * (f0-theF)
plot(correctedM, ...)
invisible(correctedM)
}
## MA plot functions
maplot <- function (x, transfo=log2, groups, refSamples,
which, pch=".", summaryFun=rowMedians,
plotFun=smoothScatter,
main="vs pseudo-median reference chip",
pairs=FALSE, ...){
transfo <- match.fun(transfo)
stopifnot(is.function(transfo))
summaryFun <- match.fun(summaryFun)
stopifnot(is.function(summaryFun))
## Checking for errors
if (!missing(refSamples)){
if (pairs)
stop("Cannot combine pairs=TRUE with 'refSamples'")
if (!is.numeric(refSamples))
stop("'refSamples' must be integer(s)")
refSamples <- as.integer(refSamples)
rg <- range(refSamples)
if (min(refSamples) < 1 | max(refSamples) > ncol(x))
stop("Ensure 'refSamples' are integers between 1 and ", ncol(x), ".")
}
if (!missing(which)){
if (!is.numeric(which))
stop("'which' must be integer(s)")
which <- as.integer(which)
rg <- range(which)
if (min(which) < 1 | max(which) > ncol(x))
stop("Ensure 'which' contains integers between 1 and ", ncol(x), ".")
}
if (!missing(groups)){
stopifnot(is.factor(groups))
stopifnot(length(groups) == ncol(x))
## if groups is given, 'which' refers to group
if (!missing(which))
if (max(which) > length(levels(groups)))
stop("'which' must be smaller than ", length(levels(groups)))
## if groups is given, 'refSamples' refers to group(s) of
## reference
if (!missing(refSamples))
if (max(refSamples) > length(levels(groups)))
stop("'refSamples' must be smaller than ", length(levels(groups)))
}
## END OF ERROR CHECK
## x <- transfo(exprs(object))
x <- transfo(x)
if (missing(groups)){
if (missing(which))
which <- 1:ncol(x)
if (!pairs) {
if (missing(refSamples)) {
medianchip <- summaryFun(x)
} else if (length(refSamples) > 1) {
medianchip <- summaryFun(x[, refSamples])
} else {
medianchip <- x[, refSamples]
}
M <- sweep(x, 1, medianchip, FUN = "-")
A <- 1/2 * sweep(x, 1, medianchip, FUN = "+")
for (i in which) {
if (missing(refSamples)){
themain <- paste(colnames(x)[i], main)
}else{
if (length(refSamples) == 1) {
if (i != refSamples)
themain <- paste(colnames(x)[i], "vs", colnames(x)[refSamples])
} else {
themain <- paste(colnames(x)[i], main)
}
}
basicMvAplot(A[, i], M[, i], main=themain, xlab="A",
ylab="M", plotFun=plotFun, pch=pch, ...)
}
} else {
basicMvApairsPlot(x[, which], transfo=transfo, plotFun=plotFun, ...)
} ## end if (!pairs)
} else { ## if groups
groups.list <- split(1:ncol(x), groups)
grouped.data <- matrix(0, nrow(x), length(groups.list))
colnames(grouped.data) <- names(groups.list)
for (i in 1:length(groups.list))
grouped.data[, i] <- rowMeans(x[, groups.list[[i]], drop = FALSE])
if (missing(which))
which <- 1:length(groups.list)
if (!pairs) {
if (missing(refSamples)) {
medianchip <- summaryFun(grouped.data)
} else if (length(refSamples) == 1) {
medianchip <- grouped.data[, refSamples]
} else {
medianchip <- summaryFun(grouped.data[, refSamples])
}
M <- sweep(grouped.data, 1, medianchip, FUN = "-")
A <- 1/2 * sweep(grouped.data, 1, medianchip, FUN = "+")
for (i in which) {
if (missing(refSamples)){
main <- paste(levels(groups)[i], main)
}else{
if (length(refSamples) == 1) {
if (i != refSamples)
main <- paste(levels(groups)[i], "vs", levels(groups)[refSamples])
} else {
main <- paste(levels(groups)[i], main)
}
}
basicMvAplot(A[, i], M[, i], main=main, xlab="A",
ylab="M", pch=pch, plotFun=plotFun, ...)
}
} else {
basicMvApairsPlot(grouped.data[, which], transfo=transfo, plotFun=plotFun, ...)
} ## end if(!pairs)
}
}
basicMvAplot <- function(A, M, subset=sample(length(M), min(c(1e4, length(M)))),
show.statistics=TRUE, span=2/3,
family.loess="gaussian", cex=2,
plotFun=smoothScatter, addLoess=TRUE, lwd=1, lty=1,
loess.col="red", ...){
fn.call <- list(...)
nmdots <- names(fn.call)
sigma <- IQR(M)
mean <- median(M)
yloc <- ifelse(is.element("ylim", nmdots), max(fn.call[['ylim']]), max(M))
xloc <- ifelse(is.element("xlim", nmdots), max(fn.call[['xlim']]), max(A))
plotFun(A, M, cex=cex, ...)
if (addLoess) {
aux <- loess(M[subset]~A[subset], degree=1, span=span,
family=family.loess)[['fitted']]
o <- order(A[subset])
A <- A[subset][o]
M <- aux[o]
o <- which(!duplicated(A))
lines(approx(A[o], M[o]), col=loess.col, lwd=lwd, lty=lty)
}
abline(0, 0, col="blue")
if (show.statistics){
txt <- paste("IQR:", format(sigma, digits = 3))
txt2 <- paste("Median:", format(mean, digits = 3))
text(xloc, yloc, paste(txt2, txt, sep="\n"), cex=cex, adj=c(1, 1))
}
}
basicMvApairsPlot <- function (x, labels=colnames(x), transfo=log2, span=2/3,
family.loess="gaussian", digits=3,
main="MVA plot", xlab="A", ylab="M",
cex=2, plotFun=smoothScatter, addLoess=TRUE,
parParams=list(mgp=c(0, .2, 0), mar=rep(1, 4), oma=c(1, 2, 2, 1)), ...){
x <- transfo(x)
J <- ncol(x)
frame()
old.par <- par(no.readonly=TRUE)
on.exit(par(old.par))
par(mfrow=c(J, J))
do.call(par, parParams)
for (j in 1:(J - 1)) {
par(mfg=c(j, j))
plot(1, 1, type="n", xaxt="n", yaxt="n", xlab="", ylab="")
text(1, 1, labels[j], cex=cex)
for (k in (j + 1):J) {
par(mfg=c(j, k))
yy <- x[, j] - x[, k]
xx <- (x[, j] + x[, k])/2
sigma <- IQR(yy)
mean <- median(yy)
basicMvAplot(xx, yy, tck=0, plotFun=plotFun, addLoess=addLoess,
show.statistics=FALSE, pch=".", xlab="", ylab="", tck=0, span=span, ...)
par(mfg=c(k, j))
qs <- unique(quantile(xx, seq(0, 1, .1)))
grps <- cut(xx, qs, include.lowest=TRUE)
ng <- length(qs)
boxplot(yy~grps, range=0, xaxt='n', yaxt='n', xlab='', ylab='', xlim=c(0, ng), ...)
## txt <- paste("IQR:", format(sigma, digits=digits))
## txt2 <- paste("Median:", format(mean, digits=digits))
## plot(c(0, 1), c(0, 1), type="n", ylab="", xlab="", xaxt="n", yaxt="n")
## text(0.5, 0.5, paste(txt2, txt, sep="\n"), cex=cex)
}
}
par(mfg=c(J, J))
plot(1, 1, type="n", xaxt="n", yaxt="n", xlab="", ylab="")
text(1, 1, labels[J], cex=cex)
mtext(xlab, 1, outer=TRUE, cex=1.5)
mtext(ylab, 2, outer=TRUE, cex=1.5)
mtext(main, 3, outer=TRUE, cex=1.5)
invisible()
}
setMethod("MAplot", "matrix",
function(object, what=identity, transfo=identity, groups, refSamples, which,
pch=".", summaryFun=rowMedians, plotFun=smoothScatter,
main="vs pseudo-median reference chip", pairs=FALSE, ...){
stopifnot(is.function(what))
maplot(x=what(object), transfo=transfo, groups=groups,
refSamples=refSamples, which=which, pch=pch,
summaryFun=summaryFun, main=main, pairs=pairs, ...)
})
readCEL <- function(cels, fid){
g <- function(x) read.celfile(x, TRUE)[['INTENSITY']][['MEAN']]
if (missing(fid)){
sapply(cels, g)
}else{
sapply(cels, function(x) g(x)[fid])
}
}
txtMsg <- function(..., domain=NULL, appendLF=FALSE)
message(..., domain=domain, appendLF=appendLF)
msgOK <- function()
message("OK")
cloneFS <- function(fs){
nms <- sort(assayDataElementNames(fs))
if (is(assayDataElement(fs, nms[1]), "ff_matrix")){
if (nms[1] == "exprs" & length(nms) == 1){
c1 <- clone(assayDataElement(fs, nms),
pattern=file.path(ldPath(), 'oligo-exprs-'))
ad <- assayDataNew(exprs=c1)
slot(fs, "assayData") <- ad
}else if (all (nms == c("channel1", "channel2"))){
c1 <- clone(assayDataElement(fs, 'channel1'),
pattern=file.path(ldPath(), 'oligo-channel1-'))
c2 <- clone(assayDataElement(fs, 'channel2'),
pattern=file.path(ldPath(), 'oligo-channel2-'))
ad <- assayDataNew(channel1=c1, channel2=c2)
slot(fs, "assayData") <- ad
}else{
stop("Don't know how to clone elements: ", nms)
}
}
return(fs)
}
#### Pair -> XYS
pair2xys <- function(pairFile){
hdr <- readLines(pairFile, n=1)
pair <- read.table(pairFile, header=TRUE, comment.char='#', sep='\t', stringsAsFactors=FALSE)
## For the moment, this gets only the PM probes
out <- merge(expand.grid(X=1:1050, Y=1:4200), pair[, c('X', 'Y', 'PM')], all.x=TRUE)
out$COUNT <- with(out, ifelse(is.na(PM), NA, 1L))
out <- out[order(out$Y, out$X),]
rownames(out) <- NULL
names(out) <- c('X', 'Y', 'SIGNAL', 'COUNT')
fout <- gsub("\\.pair$", "\\.xys", pairFile)
writeLines(hdr, fout)
suppressWarnings(write.table(out, file=fout, sep='\t', quote=FALSE, append=TRUE, row.names=FALSE))
fout
}
### parallel stuff
### iExprsProbesets <- function(x, ...){
### rns <- rownames(x)
### grps <- split(1:length(rns), rns)
### it <- idiv(length(grps), ...)
### i <- 1
### nextEl <- function(){
### n <- nextElem(it)
### set <- seq(i, length=n)
### i <<- i+n
### x[unlist(grps[set]),, drop=FALSE]
### }
### obj <- list(nextElem=nextEl)
### class(obj) <- c('iExprsProbesets', 'abstractiter', 'iter')
### obj
### }
jmacdon/oligo documentation built on Aug. 11, 2020, 12:32 a.m.
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.
Defines functions pair2xys cloneFS msgOK txtMsg readCEL basicMvAplot plotM getBaseProfile getAffinitySplineCoefficients divColors seqColors2 seqColors darkColors basicAnnotatedDataFrame basicPhData2 basicPhData1 basicPData2 basicPData AffyDate2Posix NgsDate2Posix GetAffyTimeDateAsString stArrayPmInfo getFidMetaProbesetExtended getFidMetaProbesetFull getFidMetaProbesetCore getFidProbeset getNgsColorsInfo getFilenames basecontent sequenceDesignMatrix checkChipTypes getCelChipType checkValidFilenames trigammaInverse HuberAllRowsByGroup cleanPlatformName
Documented in basecontent cleanPlatformName darkColors divColors getAffinitySplineCoefficients getBaseProfile getNgsColorsInfo plotM seqColors seqColors2 sequenceDesignMatrix
cleanPlatformName <- function(x)
gsub("[_-]", ".", paste("pd.", tolower(x), sep=""))
HuberAllRowsByGroup <- function(X, Y, k=1.5){
.Call("R_HuberMatrixRows2",X, Y, k, PACKAGE="oligo")
}
trigammaInverse <- function(x) {
# Solve trigamma(y) = x for y
# Gordon Smyth
# 8 Sept 2002. Last revised 12 March 2004.
# Non-numeric or zero length input
if(!is.numeric(x)) stop("Non-numeric argument to mathematical function")
if(length(x)==0) return(numeric(0))
# Treat out-of-range values as special cases
omit <- is.na(x)
if(any(omit)) {
y <- x
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
omit <- (x < 0)
if(any(omit)) {
y <- x
y[omit] <- NaN
warning("NaNs produced")
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
omit <- (x > 1e7)
if(any(omit)) {
y <- x
y[omit] <- 1/sqrt(x[omit])
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
omit <- (x < 1e-6)
if(any(omit)) {
y <- x
y[omit] <- 1/x[omit]
if(any(!omit)) y[!omit] <- Recall(x[!omit])
return(y)
}
# Newton's method
# 1/trigamma(y) is convex, nearly linear and strictly > y-0.5,
# so iteration to solve 1/x = 1/trigamma is monotonically convergent
y <- 0.5+1/x
iter <- 0
repeat {
iter <- iter+1
tri <- trigamma(y)
dif <- tri*(1-tri/x)/psigamma(y,deriv=2)
y <- y+dif
if(max(-dif/y) < 1e-8) break
if(iter > 50) {
warning("Iteration limit exceeded")
break
}
}
y
}
checkValidFilenames <- function(filenames) {
## must be character
stopifnot(is.character(filenames))
## must exist
dirs <- file.info(filenames)[["isdir"]]
if (any(is.na(dirs))){
msg <- paste("These do not exist:",
paste("\t", filenames[is.na(dirs)], collapse="\n"), sep="\n")
stop(msg, call.=FALSE)
}
## must be files, not dir
if (any(dirs)){
msg <- paste("These are directories:",
paste("\t", filenames[dirs], collapse="\n"), sep="\n")
stop(msg, call.=FALSE)
}
## must be readable
readable <- file.access(filenames, 4) == 0
if (any(!readable)){
msg <- paste("These are not readable:",
paste("\t", filenames[!readable], collapse="\n"), sep="\n")
stop(msg, call.=FALSE)
}
TRUE
}
## checkValidPhenodataForFiles <- function(filenames, pd){
## if (missing(pd)) return(FALSE)
## if (class(pd) != "AnnotatedDataFrame") return(FALSE)
## return(length(filenames) == nrow(pd))
## }
## createDefaultMiame <- function(filenames, notes){
## experimentData <- new("MIAME")
## preproc(experimentData)$filenames <- filenames
## preproc(experimentData)$oligoversion <- packageDescription("oligo", field="Version")
## if (!missing(notes))
## notes(experimentData) <- notes
## experimentData
## }
getCelChipType <- function(x, useAffyio){
ifelse(useAffyio,
read.celfile.header(x)[["cdfName"]],
readCelHeader(x)[["chiptype"]])
}
checkChipTypes <- function(filenames, verbose=TRUE, manufacturer, useAffyio){
if (missing(manufacturer)) stop("'checkChipTypes' needs 'manufacturer'")
if (manufacturer == "affymetrix"){
chips <- sapply(filenames, getCelChipType, useAffyio)
ok <- length(unique(chips)) == 1
if(!ok & verbose) message("All the CEL files must be of the same type.")
}else if(manufacturer == "nimblegen"){
designnamelist <- NULL
for (xysfile in filenames){
firstline <- readxysHeader(xysfile)
designname <- unlist(strsplit(firstline[grep("designname",firstline,fixed=TRUE,useBytes=TRUE)],"="))[2]
designnamelist <- rbind(designnamelist,designname)
}
ok <- length(unique(designnamelist)) == 1
if(!ok & verbose) message("All the XYS files must be of the same type.")
}else{
stop("'manufacturer' ", manufacturer, " unknown")
}
ok
}
sequenceDesignMatrix <- function(seqs){
if(length(unique(sapply(seqs,nchar)))!=1) stop("Sequences must be of same length.")
oligolength <- nchar(seqs[1])
mat <- .Call("gcrma_getSeq2",paste(seqs,collapse=""),length(seqs),oligolength,PACKAGE="oligo")
colnames(mat) <- paste(rep(c("A","C","G"),rep(oligolength,3)),position=rep(1:oligolength,3),sep="_")
return(mat)
}
basecontent <- function(seq) {
good = !is.na(seq)
havena = !all(good)
if(havena)
seq = seq[good]
rv = .Call("basecontent", seq, PACKAGE="oligo")
if(havena) {
z = rv
rv = matrix(NA, nrow=length(good), ncol=ncol(z))
colnames(rv) = colnames(z)
rv[good, ] = z
}
return(rv)
}
## Helper to parse the dots and combine with filenames
getFilenames <- function(filenames, ...){
if (!missing(filenames)){
filenames <- c(filenames, unlist(list(...)))
}else{
filenames <- unlist(list(...))
}
filenames
}
getNgsColorsInfo <- function(path=".", pattern1="_532", pattern2="_635", ...){
files1 <- list.xysfiles(path, pattern=pattern1, ...)
files2 <- list.xysfiles(path, pattern=pattern2, ...)
prefix1 <- sapply(strsplit(basename(files1), pattern1), "[[", 1)
prefix2 <- sapply(strsplit(basename(files2), pattern2), "[[", 1)
sugg <- identical(prefix1, prefix2)
stopifnot(length(files1) == length(files2))
out <- data.frame(color1=files1, color2=files2, stringsAsFactors=FALSE)
if (sugg)
out[["sampleNames"]] <- prefix1
return(out)
}
## Selectors for probes - useful for exon/gene arrays
getFidProbeset <- function(object, sortBy='fsetid'){
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
conn <- db(object)
on.exit(dbDisconnect(conn))
if (!is(object, 'HTAFeatureSet')){
sql <- "SELECT fid, fsetid FROM pmfeature"
}else{
sql <- "SELECT fid, man_fsetid as fsetid FROM pmfeature INNER JOIN featureSet USING(fsetid)"
}
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
getFidMetaProbesetCore <- function(object, sortBy='fsetid'){
conn <- db(object)
on.exit(dbDisconnect(conn))
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
if (!is(object, 'HTAFeatureSet')){
sql <- "SELECT fid, meta_fsetid as fsetid FROM pmfeature INNER JOIN core_mps USING(fsetid)"
}else{
sql <- "SELECT fid, core_mps.transcript_cluster_id as fsetid FROM pmfeature INNER JOIN core_mps USING(fsetid)"
}
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
getFidMetaProbesetFull <- function(object, sortBy='fsetid'){
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
conn <- db(object)
on.exit(dbDisconnect(conn))
sql <- "SELECT fid, meta_fsetid as fsetid FROM pmfeature INNER JOIN full_mps USING(fsetid)"
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
getFidMetaProbesetExtended <- function(object, sortBy='fsetid'){
if (!is.null(sortBy))
sortBy <- match.arg(sortBy, c('fid', 'fsetid'))
conn <- db(object)
on.exit(dbDisconnect(conn))
sql <- "SELECT fid, meta_fsetid as fsetid FROM pmfeature INNER JOIN extended_mps USING(fsetid)"
featureInfo <- dbGetQuery(conn, sql)
if (!is.null(sortBy)){
featureInfo <- featureInfo[order(featureInfo[[sortBy]]),]
rownames(featureInfo) <- NULL
}
return(featureInfo)
}
stArrayPmInfo <- function(object, target='core', sortBy='fsetid'){
## *PmInfo returns a data.frame with 'fid' and 'fsetid'
target <- match.arg(target, c('probeset', 'core', 'full', 'extended'))
theFun <- switch(target,
probeset=getFidProbeset,
core=getFidMetaProbesetCore,
full=getFidMetaProbesetFull,
extended=getFidMetaProbesetExtended)
theFun(object, sortBy=sortBy)
}
## Date/time extractors
GetAffyTimeDateAsString <- function(filenames){
f <- function(x) read.celfile.header(x, "full")[["ScanDate"]]
res <- sapply(filenames, f)
sapply(res, function(x) ifelse(length(x) == 0, NA_character_, x))
}
NgsDate2Posix <- function(txt){
if (!missing(txt)){
original <- txt
tmp <- gsub("(.* )(.{1,3}) ([0-9]{4})", "\\1\\3", txt)
out <- as.POSIXct(tmp, format="%A %B %d %H:%M:%S %Y")
if (any(is.na(out))){
warning("Returning dates/times as strings due to incompatibility.")
out <- original
}
}else{
out <- NULL
}
out
}
AffyDate2Posix <- function(txt){
if (!missing(txt)){
original <- txt
out <- as.POSIXct(txt, format="%m/%d/%y %H:%M:%S")
if (any(is.na(out))){
warning("Returning dates/times as strings - format not recognized.")
out <- original
}
}else{
out <- NULL
}
out
}
basicPData <- function(mat, filenames, dates){
if (missing(dates))
dates <- rep(NA, length(filenames))
stopifnot(length(filenames) == length(dates))
pdd <- data.frame(exprs=filenames, dates=dates)
vmd <- data.frame(labelDescription=c(
"Names of files used in 'exprs'",
"Run dates for files used in 'exprs'"),
channel=factor("_ALL_", levels=c("exprs", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat)
return(phenoData)
}
basicPData2 <- function(mat1, mat2, filenames1, filenames2,
dates1, dates2){
if (missing(dates1)) dates1 <- rep(NA, length(filenames1))
if (missing(dates2)) dates2 <- rep(NA, length(filenames2))
stopifnot(identical(colnames(mat1), colnames(mat2)),
length(filenames1) == length(filenames2),
length(dates1) == length(dates2))
pdd <- data.frame(filenamesChannel1=filenames1,
filenamesChannel2=filenames2,
dates1=dates1, dates2=dates2)
vmd <- data.frame(labelDescription=c(
"Names of files used in 'channel1'",
"Names of files used in 'channel2'",
"Run dates for files used in 'channel1'",
"Run dates for files used in 'channel2'"),
channel=factor(rep(c("channel1", "channel2"), 2),
levels=c("channel1", "channel2", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat1)
return(phenoData)
}
basicPhData1 <- function(mat){
pdd <- data.frame(index=1:ncol(mat))
vmd <- data.frame(labelDescription=c("Index"),
channel=factor("_ALL_", levels=c("exprs", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat)
return(phenoData)
}
basicPhData2 <- function(mat1, mat2){
stopifnot(identical(colnames(mat1), colnames(mat2)))
pdd <- data.frame(index=1:ncol(mat1))
vmd <- data.frame(labelDescription=c("Index"),
channel=factor("_ALL_",
levels=c("channel1", "channel2", "_ALL_")))
phenoData <- new("AnnotatedDataFrame", data=pdd, varMetadata=vmd)
sampleNames(phenoData) <- colnames(mat1)
return(phenoData)
}
basicAnnotatedDataFrame <- function(mat, byrow=FALSE){
Biobase:::annotatedDataFrameFromMatrix(mat, byrow=byrow)
}
## colors I like in oligo
darkColors <- function(n){
cols <- c("#1B9E77", "#D95F02", "#7570B3", "#E7298A", "#66A61E",
"#E6AB02", "#A6761D", "#666666")
fff <- colorRampPalette(cols)
fff(n)
}
seqColors <- function(n){
cols <- c("#F7FBFF", "#DEEBF7", "#C6DBEF", "#9ECAE1", "#6BAED6",
"#4292C6", "#2171B5", "#08519C", "#08306B")
fff <- colorRampPalette(cols)
fff(n)
}
seqColors2 <- function(n){
cols <- c("#FFF7EC", "#FEE8C8", "#FDD49E", "#FDBB84", "#FC8D59",
"#EF6548", "#D7301F", "#B30000", "#7F0000")
fff <- colorRampPalette(cols)
fff(n)
}
divColors <- function(n){
cols <- c("#053061", "#2166AC", "#4393C3", "#92C5DE", "#D1E5F0",
"#FDDBC7", "#F4A582", "#D6604D", "#B2182B", "#67001F")
fff <- colorRampPalette(cols)
fff(n)
}
## gcrma-like stuff
## from jean
getAffinitySplineCoefficients <- function(intensities, sequences){
if (is(sequences, "DNAStringSet"))
sequences <- as.character(sequences)
stopifnot(is.character(sequences))
stopifnot(is.matrix(intensities))
design <- sequenceDesignMatrix(sequences)
rm(sequences)
B <- ns(1:25, df=5)
design <- cbind(design[, 1:25] %*% B,
design[, 26:50] %*% B,
design[, 51:75] %*% B)
fits <- lm(intensities~design)
coefs <- coef(fits)[-1,]
rownames(coefs) <- rep(c("A", "C", "G"), each=5)
coefs
}
getBaseProfile <- function(coefs, probeLength=25, plot=FALSE, ...){
stopifnot(is.vector(coefs))
P <- as.integer(length(coefs)/3)
B <- ns(1:probeLength, df=5)
effects <- matrix(0, nrow=probeLength, ncol=4)
colnames(effects) <- c("A", "C", "G", "T")
for (i in 1:3)
effects[, i] <- B %*% coefs[(i-1)*P + (1:P)]
effects <- sweep(effects, 1, rowMeans(effects))
if(plot) matplot(1:probeLength, effects, ...)
invisible(effects)
}
## SnpSuperSet method?
plotM <- function(x, snp, ...){
crlmmInfo <- file.path(system.file("extdata", package=annotation(x)),
paste(annotation(x), "CrlmmInfo.rda", sep=""))
infoObj <- load(crlmmInfo)
f0 <- get(infoObj)$params$f0
rm(list=infoObj)
obj <- x[snp,]
theM <- getM(obj)[,,]
theF <- cbind(antisense=assayDataElement(obj, "antisenseF")[,],
sense=assayDataElement(obj, "senseF")[,])
theCalls <- calls(obj)[,]
correctedM <- theM + (theCalls - 2) * (f0-theF)
plot(correctedM, ...)
invisible(correctedM)
}
## MA plot functions
maplot <- function (x, transfo=log2, groups, refSamples,
which, pch=".", summaryFun=rowMedians,
plotFun=smoothScatter,
main="vs pseudo-median reference chip",
pairs=FALSE, ...){
transfo <- match.fun(transfo)
stopifnot(is.function(transfo))
summaryFun <- match.fun(summaryFun)
stopifnot(is.function(summaryFun))
## Checking for errors
if (!missing(refSamples)){
if (pairs)
stop("Cannot combine pairs=TRUE with 'refSamples'")
if (!is.numeric(refSamples))
stop("'refSamples' must be integer(s)")
refSamples <- as.integer(refSamples)
rg <- range(refSamples)
if (min(refSamples) < 1 | max(refSamples) > ncol(x))
stop("Ensure 'refSamples' are integers between 1 and ", ncol(x), ".")
}
if (!missing(which)){
if (!is.numeric(which))
stop("'which' must be integer(s)")
which <- as.integer(which)
rg <- range(which)
if (min(which) < 1 | max(which) > ncol(x))
stop("Ensure 'which' contains integers between 1 and ", ncol(x), ".")
}
if (!missing(groups)){
stopifnot(is.factor(groups))
stopifnot(length(groups) == ncol(x))
## if groups is given, 'which' refers to group
if (!missing(which))
if (max(which) > length(levels(groups)))
stop("'which' must be smaller than ", length(levels(groups)))
## if groups is given, 'refSamples' refers to group(s) of
## reference
if (!missing(refSamples))
if (max(refSamples) > length(levels(groups)))
stop("'refSamples' must be smaller than ", length(levels(groups)))
}
## END OF ERROR CHECK
## x <- transfo(exprs(object))
x <- transfo(x)
if (missing(groups)){
if (missing(which))
which <- 1:ncol(x)
if (!pairs) {
if (missing(refSamples)) {
medianchip <- summaryFun(x)
} else if (length(refSamples) > 1) {
medianchip <- summaryFun(x[, refSamples])
} else {
medianchip <- x[, refSamples]
}
M <- sweep(x, 1, medianchip, FUN = "-")
A <- 1/2 * sweep(x, 1, medianchip, FUN = "+")
for (i in which) {
if (missing(refSamples)){
themain <- paste(colnames(x)[i], main)
}else{
if (length(refSamples) == 1) {
if (i != refSamples)
themain <- paste(colnames(x)[i], "vs", colnames(x)[refSamples])
} else {
themain <- paste(colnames(x)[i], main)
}
}
basicMvAplot(A[, i], M[, i], main=themain, xlab="A",
ylab="M", plotFun=plotFun, pch=pch, ...)
}
} else {
basicMvApairsPlot(x[, which], transfo=transfo, plotFun=plotFun, ...)
} ## end if (!pairs)
} else { ## if groups
groups.list <- split(1:ncol(x), groups)
grouped.data <- matrix(0, nrow(x), length(groups.list))
colnames(grouped.data) <- names(groups.list)
for (i in 1:length(groups.list))
grouped.data[, i] <- rowMeans(x[, groups.list[[i]], drop = FALSE])
if (missing(which))
which <- 1:length(groups.list)
if (!pairs) {
if (missing(refSamples)) {
medianchip <- summaryFun(grouped.data)
} else if (length(refSamples) == 1) {
medianchip <- grouped.data[, refSamples]
} else {
medianchip <- summaryFun(grouped.data[, refSamples])
}
M <- sweep(grouped.data, 1, medianchip, FUN = "-")
A <- 1/2 * sweep(grouped.data, 1, medianchip, FUN = "+")
for (i in which) {
if (missing(refSamples)){
main <- paste(levels(groups)[i], main)
}else{
if (length(refSamples) == 1) {
if (i != refSamples)
main <- paste(levels(groups)[i], "vs", levels(groups)[refSamples])
} else {
main <- paste(levels(groups)[i], main)
}
}
basicMvAplot(A[, i], M[, i], main=main, xlab="A",
ylab="M", pch=pch, plotFun=plotFun, ...)
}
} else {
basicMvApairsPlot(grouped.data[, which], transfo=transfo, plotFun=plotFun, ...)
} ## end if(!pairs)
}
}
basicMvAplot <- function(A, M, subset=sample(length(M), min(c(1e4, length(M)))),
show.statistics=TRUE, span=2/3,
family.loess="gaussian", cex=2,
plotFun=smoothScatter, addLoess=TRUE, lwd=1, lty=1,
loess.col="red", ...){
fn.call <- list(...)
nmdots <- names(fn.call)
sigma <- IQR(M)
mean <- median(M)
yloc <- ifelse(is.element("ylim", nmdots), max(fn.call[['ylim']]), max(M))
xloc <- ifelse(is.element("xlim", nmdots), max(fn.call[['xlim']]), max(A))
plotFun(A, M, cex=cex, ...)
if (addLoess) {
aux <- loess(M[subset]~A[subset], degree=1, span=span,
family=family.loess)[['fitted']]
o <- order(A[subset])
A <- A[subset][o]
M <- aux[o]
o <- which(!duplicated(A))
lines(approx(A[o], M[o]), col=loess.col, lwd=lwd, lty=lty)
}
abline(0, 0, col="blue")
if (show.statistics){
txt <- paste("IQR:", format(sigma, digits = 3))
txt2 <- paste("Median:", format(mean, digits = 3))
text(xloc, yloc, paste(txt2, txt, sep="\n"), cex=cex, adj=c(1, 1))
}
}
basicMvApairsPlot <- function (x, labels=colnames(x), transfo=log2, span=2/3,
family.loess="gaussian", digits=3,
main="MVA plot", xlab="A", ylab="M",
cex=2, plotFun=smoothScatter, addLoess=TRUE,
parParams=list(mgp=c(0, .2, 0), mar=rep(1, 4), oma=c(1, 2, 2, 1)), ...){
x <- transfo(x)
J <- ncol(x)
frame()
old.par <- par(no.readonly=TRUE)
on.exit(par(old.par))
par(mfrow=c(J, J))
do.call(par, parParams)
for (j in 1:(J - 1)) {
par(mfg=c(j, j))
plot(1, 1, type="n", xaxt="n", yaxt="n", xlab="", ylab="")
text(1, 1, labels[j], cex=cex)
for (k in (j + 1):J) {
par(mfg=c(j, k))
yy <- x[, j] - x[, k]
xx <- (x[, j] + x[, k])/2
sigma <- IQR(yy)
mean <- median(yy)
basicMvAplot(xx, yy, tck=0, plotFun=plotFun, addLoess=addLoess,
show.statistics=FALSE, pch=".", xlab="", ylab="", tck=0, span=span, ...)
par(mfg=c(k, j))
qs <- unique(quantile(xx, seq(0, 1, .1)))
grps <- cut(xx, qs, include.lowest=TRUE)
ng <- length(qs)
boxplot(yy~grps, range=0, xaxt='n', yaxt='n', xlab='', ylab='', xlim=c(0, ng), ...)
## txt <- paste("IQR:", format(sigma, digits=digits))
## txt2 <- paste("Median:", format(mean, digits=digits))
## plot(c(0, 1), c(0, 1), type="n", ylab="", xlab="", xaxt="n", yaxt="n")
## text(0.5, 0.5, paste(txt2, txt, sep="\n"), cex=cex)
}
}
par(mfg=c(J, J))
plot(1, 1, type="n", xaxt="n", yaxt="n", xlab="", ylab="")
text(1, 1, labels[J], cex=cex)
mtext(xlab, 1, outer=TRUE, cex=1.5)
mtext(ylab, 2, outer=TRUE, cex=1.5)
mtext(main, 3, outer=TRUE, cex=1.5)
invisible()
}
setMethod("MAplot", "matrix",
function(object, what=identity, transfo=identity, groups, refSamples, which,
pch=".", summaryFun=rowMedians, plotFun=smoothScatter,
main="vs pseudo-median reference chip", pairs=FALSE, ...){
stopifnot(is.function(what))
maplot(x=what(object), transfo=transfo, groups=groups,
refSamples=refSamples, which=which, pch=pch,
summaryFun=summaryFun, main=main, pairs=pairs, ...)
})
readCEL <- function(cels, fid){
g <- function(x) read.celfile(x, TRUE)[['INTENSITY']][['MEAN']]
if (missing(fid)){
sapply(cels, g)
}else{
sapply(cels, function(x) g(x)[fid])
}
}
txtMsg <- function(..., domain=NULL, appendLF=FALSE)
message(..., domain=domain, appendLF=appendLF)
msgOK <- function()
message("OK")
cloneFS <- function(fs){
nms <- sort(assayDataElementNames(fs))
if (is(assayDataElement(fs, nms[1]), "ff_matrix")){
if (nms[1] == "exprs" & length(nms) == 1){
c1 <- clone(assayDataElement(fs, nms),
pattern=file.path(ldPath(), 'oligo-exprs-'))
ad <- assayDataNew(exprs=c1)
slot(fs, "assayData") <- ad
}else if (all (nms == c("channel1", "channel2"))){
c1 <- clone(assayDataElement(fs, 'channel1'),
pattern=file.path(ldPath(), 'oligo-channel1-'))
c2 <- clone(assayDataElement(fs, 'channel2'),
pattern=file.path(ldPath(), 'oligo-channel2-'))
ad <- assayDataNew(channel1=c1, channel2=c2)
slot(fs, "assayData") <- ad
}else{
stop("Don't know how to clone elements: ", nms)
}
}
return(fs)
}
#### Pair -> XYS
pair2xys <- function(pairFile){
hdr <- readLines(pairFile, n=1)
pair <- read.table(pairFile, header=TRUE, comment.char='#', sep='\t', stringsAsFactors=FALSE)
## For the moment, this gets only the PM probes
out <- merge(expand.grid(X=1:1050, Y=1:4200), pair[, c('X', 'Y', 'PM')], all.x=TRUE)
out$COUNT <- with(out, ifelse(is.na(PM), NA, 1L))
out <- out[order(out$Y, out$X),]
rownames(out) <- NULL
names(out) <- c('X', 'Y', 'SIGNAL', 'COUNT')
fout <- gsub("\\.pair$", "\\.xys", pairFile)
writeLines(hdr, fout)
suppressWarnings(write.table(out, file=fout, sep='\t', quote=FALSE, append=TRUE, row.names=FALSE))
fout
}
### parallel stuff
### iExprsProbesets <- function(x, ...){
### rns <- rownames(x)
### grps <- split(1:length(rns), rns)
### it <- idiv(length(grps), ...)
### i <- 1
### nextEl <- function(){
### n <- nextElem(it)
### set <- seq(i, length=n)
### i <<- i+n
### x[unlist(grps[set]),, drop=FALSE]
### }
### obj <- list(nextElem=nextEl)
### class(obj) <- c('iExprsProbesets', 'abstractiter', 'iter')
### obj
### }
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.
Embedding an R snippet on your website
Add the following code to your website.
For more information on customizing the embed code, read Embedding Snippets.