# HG changeset patch
# User iuc
# Date 1707498385 0
# Node ID 119b069fc845af51288502e8db6a7dc6e3639001
# Parent d6f5fa4ee47366ac4ebf6e3c1d8748c4fdd5d16d
planemo upload for repository https://github.com/galaxyproject/tools-iuc/tree/master/tools/limma_voom commit b4d788c0f159d507159117a063b1f867b243c738
diff -r d6f5fa4ee473 -r 119b069fc845 limma_voom.R
--- a/limma_voom.R Tue Mar 01 08:03:53 2022 +0000
+++ b/limma_voom.R Fri Feb 09 17:06:25 2024 +0000
@@ -46,7 +46,21 @@
# Modified by: Maria Doyle - Jun 2017, Jan 2018, May 2018
# Record starting time
-time_start <- as.character(Sys.time())
+time_start <- Sys.time()
+
+# Setup R error handling to go to stderr
+options(
+ show.error.messages = FALSE,
+ error = function() {
+ cat(geterrmessage(), file = stderr())
+ q("no", 1, FALSE)
+ }
+)
+
+# Unify locale settings
+loc <- Sys.setlocale("LC_MESSAGES", "en_US.UTF-8")
+
+warnings()
# Load all required libraries
library(methods, quietly = TRUE, warn.conflicts = FALSE)
@@ -106,19 +120,19 @@
# Create cata function: default path set, default seperator empty and appending
# true by default (Ripped straight from the cat function with altered argument
# defaults)
-cata <- function(..., file = opt$htmlPath, sep = "", fill = FALSE, labels = NULL,
- append = TRUE) {
- if (is.character(file))
- if (file == "")
+cata <- function(..., file = opt$htmlPath, sep = "", fill = FALSE,
+ labels = NULL, append = TRUE) {
+ if (is.character(file)) {
+ if (file == "") {
file <- stdout()
- else if (substring(file, 1L, 1L) == "|") {
+ } else if (substring(file, 1L, 1L) == "|") {
file <- pipe(substring(file, 2L), "w")
on.exit(close(file))
+ } else {
+ file <- file(file, ifelse(append, "a", "w"))
+ on.exit(close(file))
}
- else {
- file <- file(file, ifelse(append, "a", "w"))
- on.exit(close(file))
- }
+ }
.Internal(cat(list(...), file, sep, fill, labels, append))
}
@@ -162,39 +176,42 @@
# Get options, using the spec as defined by the enclosed list.
# Read the options from the default: commandArgs(TRUE).
-spec <- matrix(c(
- "htmlPath", "R", 1, "character",
- "outPath", "o", 1, "character",
- "filesPath", "j", 2, "character",
- "matrixPath", "m", 2, "character",
- "factFile", "f", 2, "character",
- "factInput", "i", 2, "character",
- "annoPath", "a", 2, "character",
- "contrastFile", "C", 1, "character",
- "contrastInput", "D", 1, "character",
- "cpmReq", "c", 1, "double",
- "totReq", "y", 0, "logical",
- "cntReq", "z", 1, "integer",
- "sampleReq", "s", 1, "integer",
- "filtCounts", "F", 0, "logical",
- "normCounts", "x", 0, "logical",
- "rdaOpt", "r", 0, "logical",
- "lfcReq", "l", 1, "double",
- "pValReq", "p", 1, "double",
- "pAdjOpt", "d", 1, "character",
- "normOpt", "n", 1, "character",
- "robOpt", "b", 0, "logical",
- "trend", "t", 1, "double",
- "weightOpt", "w", 0, "logical",
- "topgenes", "G", 1, "integer",
- "treatOpt", "T", 0, "logical",
- "plots", "P", 1, "character",
- "libinfoOpt", "L", 0, "logical"),
- byrow = TRUE, ncol = 4)
+spec <- matrix(
+ c(
+ "htmlPath", "R", 1, "character",
+ "outPath", "o", 1, "character",
+ "filesPath", "j", 2, "character",
+ "matrixPath", "m", 2, "character",
+ "factFile", "f", 2, "character",
+ "factInput", "i", 2, "character",
+ "annoPath", "a", 2, "character",
+ "contrastFile", "C", 1, "character",
+ "contrastInput", "D", 1, "character",
+ "cpmReq", "c", 1, "double",
+ "totReq", "y", 0, "logical",
+ "cntReq", "z", 1, "integer",
+ "sampleReq", "s", 1, "integer",
+ "filtCounts", "F", 0, "logical",
+ "normCounts", "x", 0, "logical",
+ "rdaOpt", "r", 0, "logical",
+ "lfcReq", "l", 1, "double",
+ "pValReq", "p", 1, "double",
+ "pAdjOpt", "d", 1, "character",
+ "normOpt", "n", 1, "character",
+ "robOpt", "b", 0, "logical",
+ "trend", "t", 1, "double",
+ "weightOpt", "w", 0, "logical",
+ "topgenes", "G", 1, "integer",
+ "treatOpt", "T", 0, "logical",
+ "plots", "P", 1, "character",
+ "libinfoOpt", "L", 0, "logical"
+ ),
+ byrow = TRUE, ncol = 4
+)
opt <- getopt(spec)
-if (is.null(opt$matrixPath) & is.null(opt$filesPath)) {
+if (is.null(opt$matrixPath) && is.null(opt$filesPath)) {
cat("A counts matrix (or a set of counts files) is required.\n")
q(status = 1)
}
@@ -283,10 +300,12 @@
factor_list <- parser$getObject()
factors <- sapply(factor_list, function(x) x[[1]])
filenames_in <- unname(unlist(factor_list[[1]][[2]]))
- sampletable <- data.frame(sample = basename(filenames_in),
- filename = filenames_in,
- row.names = filenames_in,
- stringsAsFactors = FALSE)
+ sampletable <- data.frame(
+ sample = basename(filenames_in),
+ filename = filenames_in,
+ row.names = filenames_in,
+ stringsAsFactors = FALSE
+ )
for (factor in factor_list) {
factorname <- factor[[1]]
sampletable[[factorname]] <- character(nrow(sampletable))
@@ -301,12 +320,11 @@
rem <- c("sample", "filename")
factors <- sampletable[, !(names(sampletable) %in% rem), drop = FALSE]
- #read in count files and create single table
+ # read in count files and create single table
countfiles <- lapply(sampletable$filename, function(x) {
read.delim(x, row.names = 1)
- })
+ })
counts <- do.call("cbind", countfiles)
-
} else {
# Process the single count matrix
counts <- read.table(opt$matrixPath, header = TRUE, sep = "\t", strip.white = TRUE, stringsAsFactors = FALSE, check.names = FALSE)
@@ -317,12 +335,13 @@
# Process factors
if (is.null(opt$factInput)) {
factordata <- read.table(opt$factFile, header = TRUE, sep = "\t", strip.white = TRUE, stringsAsFactors = TRUE)
- if (!setequal(factordata[, 1], colnames(counts)))
+ if (!setequal(factordata[, 1], colnames(counts))) {
stop("Sample IDs in counts and factors files don't match")
+ }
# order samples as in counts matrix
factordata <- factordata[match(colnames(counts), factordata[, 1]), ]
factors <- factordata[, -1, drop = FALSE]
- } else {
+ } else {
factors <- unlist(strsplit(opt$factInput, "|", fixed = TRUE))
factordata <- list()
for (fact in factors) {
@@ -347,19 +366,19 @@
factors <- sapply(factors, make.names)
factors <- data.frame(factors, stringsAsFactors = TRUE)
- # if annotation file provided
+# if annotation file provided
if (have_anno) {
geneanno <- read.table(opt$annoPath, header = TRUE, sep = "\t", quote = "", strip.white = TRUE, stringsAsFactors = FALSE)
}
-#Create output directory
+# Create output directory
dir.create(opt$outPath, showWarnings = FALSE)
# Process contrasts
if (is.null(opt$contrastInput)) {
contrast_data <- read.table(opt$contrastFile, header = TRUE, sep = "\t", quote = "", strip.white = TRUE, stringsAsFactors = FALSE)
contrast_data <- contrast_data[, 1, drop = TRUE]
-} else {
+} else {
# Split up contrasts seperated by comma into a vector then sanitise
contrast_data <- unlist(strsplit(opt$contrastInput, split = ","))
}
@@ -370,15 +389,14 @@
cons <- NULL
cons_d <- NULL
for (i in contrast_data) {
-
# if the contrast is a difference of differences e.g. (A-B)-(X-Y)
if (grepl("\\)-\\(", i)) {
i <- unlist(strsplit(i, split = "\\)-\\("))
i <- gsub("\\(|\\)", "", i)
for (j in i) {
- j <- sanitise_contrast(j)
- j <- paste0("(", j, ")")
- cons_d <- append(cons_d, unlist(j))
+ j <- sanitise_contrast(j)
+ j <- paste0("(", j, ")")
+ cons_d <- append(cons_d, unlist(j))
}
cons_d <- paste(cons_d, collapse = "-")
cons <- append(cons, unlist(cons_d))
@@ -428,10 +446,14 @@
# Initialise data for html links and images, data frame with columns Label and
# Link
-link_data <- data.frame(Label = character(), Link = character(),
- stringsAsFactors = FALSE)
-image_data <- data.frame(Label = character(), Link = character(),
- stringsAsFactors = FALSE)
+link_data <- data.frame(
+ Label = character(), Link = character(),
+ stringsAsFactors = FALSE
+)
+image_data <- data.frame(
+ Label = character(), Link = character(),
+ stringsAsFactors = FALSE
+)
# Initialise vectors for storage of up/down/neutral regulated counts
up_count <- numeric()
@@ -447,11 +469,11 @@
data <- list()
data$counts <- counts
if (have_anno) {
- # order annotation by genes in counts (assumes gene ids are in 1st column of geneanno)
- annoord <- geneanno[match(row.names(counts), geneanno[, 1]), ]
- data$genes <- annoord
+ # order annotation by genes in counts (assumes gene ids are in 1st column of geneanno)
+ annoord <- geneanno[match(row.names(counts), geneanno[, 1]), ]
+ data$genes <- annoord
} else {
- data$genes <- data.frame(GeneID = row.names(counts))
+ data$genes <- data.frame(GeneID = row.names(counts))
}
# Creating naming data
@@ -461,7 +483,7 @@
# Creating colours for the groups
cols <- as.numeric(factors[, 1])
-col.group <- palette()[cols]
+col_group <- palette()[cols]
# If filter crieteria set, filter out genes that do not have a required cpm/counts in a required number of
# samples. Default is no filtering
@@ -469,7 +491,6 @@
nsamples <- ncol(data$counts)
if (filt_cpm || filt_smpcount || filt_totcount) {
-
if (filt_totcount) {
keep <- rowSums(data$counts) >= opt$cntReq
} else if (filt_smpcount) {
@@ -513,22 +534,22 @@
# before filtering
lcpm1 <- cpm(counts, log = TRUE)
- plot(density(lcpm1[, 1]), col = col.group[1], lwd = 2, las = 2, main = "", xlab = "")
+ plot(density(lcpm1[, 1]), col = col_group[1], lwd = 2, las = 2, main = "", xlab = "")
title(main = "Density Plot: Raw counts", xlab = "Log-cpm")
for (i in 2:nsamples) {
den <- density(lcpm1[, i])
- lines(den$x, den$y, col = col.group[i], lwd = 2)
+ lines(den$x, den$y, col = col_group[i], lwd = 2)
}
# after filtering
lcpm2 <- cpm(data$counts, log = TRUE)
- plot(density(lcpm2[, 1]), col = col.group[1], lwd = 2, las = 2, main = "", xlab = "")
+ plot(density(lcpm2[, 1]), col = col_group[1], lwd = 2, las = 2, main = "", xlab = "")
title(main = "Density Plot: Filtered counts", xlab = "Log-cpm")
for (i in 2:nsamples) {
den <- density(lcpm2[, i])
- lines(den$x, den$y, col = col.group[i], lwd = 2)
+ lines(den$x, den$y, col = col_group[i], lwd = 2)
}
- legend("topright", samplenames, text.col = col.group, bty = "n")
+ legend("topright", samplenames, text.col = col_group, bty = "n")
img_name <- "Densityplots.png"
img_addr <- "densityplots.png"
image_data <- rbind(image_data, data.frame(Label = img_name, Link = img_addr, stringsAsFactors = FALSE))
@@ -537,19 +558,19 @@
# PDF
pdf(den_pdf, width = 14)
par(mfrow = c(1, 2), cex.axis = 0.8)
- plot(density(lcpm1[, 1]), col = col.group[1], lwd = 2, las = 2, main = "", xlab = "")
+ plot(density(lcpm1[, 1]), col = col_group[1], lwd = 2, las = 2, main = "", xlab = "")
title(main = "Density Plot: Raw counts", xlab = "Log-cpm")
for (i in 2:nsamples) {
den <- density(lcpm1[, i])
- lines(den$x, den$y, col = col.group[i], lwd = 2)
+ lines(den$x, den$y, col = col_group[i], lwd = 2)
}
- plot(density(lcpm2[, 1]), col = col.group[1], lwd = 2, las = 2, main = "", xlab = "")
+ plot(density(lcpm2[, 1]), col = col_group[1], lwd = 2, las = 2, main = "", xlab = "")
title(main = "Density Plot: Filtered counts", xlab = "Log-cpm")
for (i in 2:nsamples) {
den <- density(lcpm2[, i])
- lines(den$x, den$y, col = col.group[i], lwd = 2)
+ lines(den$x, den$y, col = col_group[i], lwd = 2)
}
- legend("topright", samplenames, text.col = col.group, bty = "n")
+ legend("topright", samplenames, text.col = col_group, bty = "n")
link_name <- "DensityPlots.pdf"
link_addr <- "densityplots.pdf"
link_data <- rbind(link_data, data.frame(Label = link_name, Link = link_addr, stringsAsFactors = FALSE))
@@ -582,7 +603,7 @@
# Calculating normalising factors
print("Calculating Normalisation Factors")
-logcounts <- y #store for plots
+logcounts <- y # store for plots
y <- calcNormFactors(y, method = opt$normOpt)
# Generate contrasts information
@@ -594,20 +615,20 @@
################################################################################
# Plot Box plots (before and after normalisation)
-if (opt$normOpt != "none" & "b" %in% plots) {
+if (opt$normOpt != "none" && "b" %in% plots) {
png(box_png, width = 1000, height = 500)
par(mfrow = c(1, 2), mar = c(6, 4, 2, 2) + 0.1)
labels <- colnames(counts)
lcpm1 <- cpm(y$counts, log = TRUE)
- boxplot(lcpm1, las = 2, col = col.group, xaxt = "n", xlab = "")
+ boxplot(lcpm1, las = 2, col = col_group, xaxt = "n", xlab = "")
axis(1, at = seq_along(labels), labels = FALSE)
abline(h = median(lcpm1), col = 4)
text(x = seq_along(labels), y = par("usr")[3] - 1, srt = 45, adj = 1, labels = labels, xpd = TRUE)
title(main = "Box Plot: Unnormalised counts", ylab = "Log-cpm")
lcpm2 <- cpm(y, log = TRUE)
- boxplot(lcpm2, las = 2, col = col.group, xaxt = "n", xlab = "")
+ boxplot(lcpm2, las = 2, col = col_group, xaxt = "n", xlab = "")
axis(1, at = seq_along(labels), labels = FALSE)
text(x = seq_along(labels), y = par("usr")[3] - 1, srt = 45, adj = 1, labels = labels, xpd = TRUE)
abline(h = median(lcpm2), col = 4)
@@ -620,12 +641,12 @@
pdf(box_pdf, width = 14)
par(mfrow = c(1, 2), mar = c(6, 4, 2, 2) + 0.1)
- boxplot(lcpm1, las = 2, col = col.group, xaxt = "n", xlab = "")
+ boxplot(lcpm1, las = 2, col = col_group, xaxt = "n", xlab = "")
axis(1, at = seq_along(labels), labels = FALSE)
abline(h = median(lcpm1), col = 4)
text(x = seq_along(labels), y = par("usr")[3] - 1, srt = 45, adj = 1, labels = labels, xpd = TRUE)
title(main = "Box Plot: Unnormalised counts", ylab = "Log-cpm")
- boxplot(lcpm2, las = 2, col = col.group, xaxt = "n", xlab = "")
+ boxplot(lcpm2, las = 2, col = col_group, xaxt = "n", xlab = "")
axis(1, at = seq_along(labels), labels = FALSE)
text(x = seq_along(labels), y = par("usr")[3] - 1, srt = 45, adj = 1, labels = labels, xpd = TRUE)
abline(h = median(lcpm2), col = 4)
@@ -644,7 +665,7 @@
# get column of matrix
get_cols <- function(x, inds) {
- x[, inds, drop = FALSE]
+ x[, inds, drop = FALSE]
}
x <- cpm(y, log = TRUE)
@@ -656,19 +677,19 @@
bad <- rowSums(is.finite(x)) < nsamples
if (any(bad)) {
- warning("Rows containing infinite values have been removed")
- x <- x[!bad, , drop = FALSE]
+ warning("Rows containing infinite values have been removed")
+ x <- x[!bad, , drop = FALSE]
}
dd <- matrix(0, nrow = nsamples, ncol = nsamples, dimnames = list(cn, cn))
topindex <- nprobes - top + 1L
for (i in 2L:(nsamples)) {
- for (j in 1L:(i - 1L)) {
- dists <- (get_cols(x, i) - get_cols(x, j))^2
- dists <- sort.int(dists, partial = topindex)
- topdist <- dists[topindex:nprobes]
- dd[i, j] <- sqrt(mean(topdist))
- }
+ for (j in 1L:(i - 1L)) {
+ dists <- (get_cols(x, i) - get_cols(x, j))^2
+ dists <- sort.int(dists, partial = topindex)
+ topdist <- dists[topindex:nprobes]
+ dd[i, j] <- sqrt(mean(topdist))
+ }
}
a1 <- suppressWarnings(cmdscale(as.dist(dd), k = min(ndim, 8), eig = TRUE))
@@ -676,7 +697,7 @@
png(mdsscree_png, width = 1000, height = 500)
par(mfrow = c(1, 2))
plotMDS(y, labels = samplenames, col = as.numeric(factors[, 1]), main = "MDS Plot: Dims 1 and 2")
-barplot(eigen$eigen, names.arg = eigen$name, main = "Scree Plot: Variance Explained", xlab = "Dimension", ylab = "Proportion", las = 1)
+barplot(eigen$eigen, names.arg = eigen$name, main = "Scree Plot: Variance Explained", xlab = "Dimension", ylab = "Proportion", las = 1)
img_name <- paste0("MDSPlot_", names(factors)[1], ".png")
img_addr <- "mdsscree.png"
image_data <- rbind(image_data, data.frame(Label = img_name, Link = img_addr, stringsAsFactors = FALSE))
@@ -685,7 +706,7 @@
pdf(mdsscree_pdf, width = 14)
par(mfrow = c(1, 2))
plotMDS(y, labels = samplenames, col = as.numeric(factors[, 1]), main = "MDS Plot: Dims 1 and 2")
-barplot(eigen$eigen, names.arg = eigen$name, main = "Scree Plot: Variance Explained", xlab = "Dimension", ylab = "Proportion", las = 1)
+barplot(eigen$eigen, names.arg = eigen$name, main = "Scree Plot: Variance Explained", xlab = "Dimension", ylab = "Proportion", las = 1)
link_name <- paste0("MDSPlot_", names(factors)[1], ".pdf")
link_addr <- "mdsscree.pdf"
link_data <- rbind(link_data, data.frame(Label = link_name, Link = link_addr, stringsAsFactors = FALSE))
@@ -693,8 +714,10 @@
# generate Glimma interactive MDS Plot
if ("i" %in% plots) {
- Glimma::glMDSPlot(y, labels = samplenames, groups = factors[, 1],
- folder = "glimma_MDS", launch = FALSE)
+ Glimma::glMDSPlot(y,
+ labels = samplenames, groups = factors[, 1],
+ folder = "glimma_MDS", launch = FALSE
+ )
link_name <- "Glimma_MDSPlot.html"
link_addr <- "glimma_MDS/MDS-Plot.html"
link_data <- rbind(link_data, c(link_name, link_addr))
@@ -789,7 +812,6 @@
# Generating fit data and top table with weights
wts <- vdata$weights
voomfit <- lmFit(vdata, design, weights = wts)
-
} else {
voom_pdf <- make_out("voomplot.pdf")
voom_png <- make_out("voomplot.png")
@@ -812,7 +834,7 @@
voomfit <- lmFit(vdata, design)
}
- # Save normalised counts (log2cpm)
+ # Save normalised counts (log2cpm)
if (want_norm) {
norm_counts <- data.frame(vdata$genes, vdata$E, check.names = FALSE)
write.table(norm_counts, file = norm_out, row.names = FALSE, sep = "\t", quote = FALSE)
@@ -847,7 +869,7 @@
link_data <- rbind(link_data, c(link_name, link_addr))
invisible(dev.off())
- # Save library size info
+# Save library size info
if (want_libinfo) {
efflibsize <- round(y$samples$lib.size * y$samples$norm.factors)
libsizeinfo <- cbind(y$samples, EffectiveLibrarySize = efflibsize)
@@ -869,8 +891,10 @@
}
}
-status <- decideTests(fit, adjust.method = opt$pAdjOpt, p.value = opt$pValReq,
- lfc = opt$lfcReq)
+status <- decideTests(fit,
+ adjust.method = opt$pAdjOpt, p.value = opt$pValReq,
+ lfc = opt$lfcReq
+)
sum_status <- summary(status)
for (i in seq_along(cons)) {
@@ -885,7 +909,7 @@
# Write top expressions table
if (want_treat) {
top <- topTreat(fit, coef = i, adjust.method = opt$pAdjOpt, number = Inf, sort.by = "P")
- } else{
+ } else {
top <- topTable(fit, coef = i, adjust.method = opt$pAdjOpt, number = Inf, sort.by = "P")
}
write.table(top, file = top_out[i], row.names = FALSE, sep = "\t", quote = FALSE)
@@ -895,10 +919,12 @@
# Plot MD (log ratios vs mean average) using limma package on weighted
pdf(md_pdf[i])
- limma::plotMD(fit, status = status[, i], coef = i,
+ limma::plotMD(fit,
+ status = status[, i], coef = i,
main = paste("MD Plot:", unmake_names(con)),
hl.col = alpha(c("firebrick", "blue"), 0.4), values = c(1, -1),
- xlab = "Average Expression", ylab = "logFC")
+ xlab = "Average Expression", ylab = "logFC"
+ )
abline(h = 0, col = "grey", lty = 2)
link_name <- paste0("MDPlot_", con, ".pdf")
link_addr <- paste0("mdplot_", con, ".pdf")
@@ -906,7 +932,7 @@
invisible(dev.off())
# Generate Glimma interactive Volcano, MD plot and tables, requires annotation file (assumes gene labels/symbols in 2nd column)
- if ("i" %in% plots & have_anno) {
+ if ("i" %in% plots && have_anno) {
# make gene labels unique to handle NAs
geneanno <- y$genes
geneanno[, 2] <- make.unique(geneanno[, 2])
@@ -914,25 +940,29 @@
# use the logcpms for the counts
if (want_trend) {
cnts <- logcpm
- } else{
+ } else {
cnts <- vdata$E
}
# MD plot
- Glimma::glMDPlot(fit, coef = i, counts = cnts, anno = geneanno, groups = factors[, 1],
- status = status[, i], sample.cols = col.group,
- main = paste("MD Plot:", unmake_names(con)), side.main = colnames(y$genes)[2],
- folder = paste0("glimma_", unmake_names(con)), launch = FALSE)
+ Glimma::glMDPlot(fit,
+ coef = i, counts = cnts, anno = geneanno, groups = factors[, 1],
+ status = status[, i], sample.cols = col_group,
+ main = paste("MD Plot:", unmake_names(con)), side.main = colnames(y$genes)[2],
+ folder = paste0("glimma_", unmake_names(con)), launch = FALSE
+ )
link_name <- paste0("Glimma_MDPlot_", con, ".html")
link_addr <- paste0("glimma_", con, "/MD-Plot.html")
link_data <- rbind(link_data, c(link_name, link_addr))
# Volcano plot
- Glimma::glXYPlot(x = fit$coefficients[, i], y = -log10(fit$p.value[, i]), counts = cnts, anno = geneanno, groups = factors[, 1],
- status = status[, i], sample.cols = col.group,
+ Glimma::glXYPlot(
+ x = fit$coefficients[, i], y = -log10(fit$p.value[, i]), counts = cnts, anno = geneanno, groups = factors[, 1],
+ status = status[, i], sample.cols = col_group,
main = paste("Volcano Plot:", unmake_names(con)), side.main = colnames(y$genes)[2],
xlab = "logFC", ylab = "-log10(P-value)",
- folder = paste0("glimma_volcano_", unmake_names(con)), launch = FALSE)
+ folder = paste0("glimma_volcano_", unmake_names(con)), launch = FALSE
+ )
link_name <- paste0("Glimma_VolcanoPlot_", con, ".html")
link_addr <- paste0("glimma_volcano_", con, "/XY-Plot.html")
link_data <- rbind(link_data, c(link_name, link_addr))
@@ -946,10 +976,12 @@
} else {
labels <- fit$genes$GeneID
}
- limma::volcanoplot(fit, coef = i,
+ limma::volcanoplot(fit,
+ coef = i,
main = paste("Volcano Plot:", unmake_names(con)),
highlight = opt$topgenes,
- names = labels)
+ names = labels
+ )
link_name <- paste0("VolcanoPlot_", con, ".pdf")
link_addr <- paste0("volplot_", con, ".pdf")
link_data <- rbind(link_data, c(link_name, link_addr))
@@ -960,21 +992,27 @@
par(mfrow = c(1, 2), mar = c(5, 4, 2, 2) + 0.1, oma = c(0, 0, 3, 0))
# MD plot
- limma::plotMD(fit, status = status[, i], coef = i, main = "MD Plot",
+ limma::plotMD(fit,
+ status = status[, i], coef = i, main = "MD Plot",
hl.col = alpha(c("firebrick", "blue"), 0.4), values = c(1, -1),
- xlab = "Average Expression", ylab = "logFC")
+ xlab = "Average Expression", ylab = "logFC"
+ )
abline(h = 0, col = "grey", lty = 2)
# Volcano
if (have_anno) {
# labels must be in second column currently
- limma::volcanoplot(fit, coef = i, main = "Volcano Plot",
+ limma::volcanoplot(fit,
+ coef = i, main = "Volcano Plot",
highlight = opt$topgenes,
- names = fit$genes[, 2])
+ names = fit$genes[, 2]
+ )
} else {
- limma::volcanoplot(fit, coef = i, main = "Volcano Plot",
+ limma::volcanoplot(fit,
+ coef = i, main = "Volcano Plot",
highlight = opt$topgenes,
- names = fit$genes$GeneID)
+ names = fit$genes$GeneID
+ )
}
img_name <- paste0("MDVolPlot_", con)
@@ -999,10 +1037,12 @@
} else {
labels <- rownames(topexp)
}
- heatmap.2(topexp, scale = "row", Colv = FALSE, Rowv = FALSE, dendrogram = "none",
+ heatmap.2(topexp,
+ scale = "row", Colv = FALSE, Rowv = FALSE, dendrogram = "none",
main = paste("Contrast:", unmake_names(con), "\nTop", opt$topgenes, "genes by adj.P.Val"),
trace = "none", density.info = "none", lhei = c(2, 10), margin = c(8, 6), labRow = labels, cexRow = 0.7, srtCol = 45,
- col = mycol, ColSideColors = col.group)
+ col = mycol, ColSideColors = col_group
+ )
link_name <- paste0("Heatmap_", con, ".pdf")
link_addr <- paste0("heatmap_", con, ".pdf")
link_data <- rbind(link_data, c(link_name, link_addr))
@@ -1013,17 +1053,21 @@
# Plot Stripcharts of top genes
pdf(strip_pdf[i], title = paste("Contrast:", unmake_names(con)))
par(mfrow = c(3, 2), cex.main = 0.8, cex.axis = 0.8)
- cols <- unique(col.group)
+ cols <- unique(col_group)
for (j in seq_along(topgenes)) {
lfc <- round(top[topgenes[j], "logFC"], 2)
pval <- round(top[topgenes[j], "adj.P.Val"], 5)
if (want_trend) {
- stripchart(plot_data[topgenes[j], ] ~ factors[, 1], vertical = TRUE, las = 2, pch = 16, cex = 0.8, cex.lab = 0.8, col = cols,
- method = "jitter", ylab = "Normalised log2 expression", main = paste0(labels[j], "\nlogFC=", lfc, ", adj.P.Val=", pval))
+ stripchart(plot_data[topgenes[j], ] ~ factors[, 1],
+ vertical = TRUE, las = 2, pch = 16, cex = 0.8, cex.lab = 0.8, col = cols,
+ method = "jitter", ylab = "Normalised log2 expression", main = paste0(labels[j], "\nlogFC=", lfc, ", adj.P.Val=", pval)
+ )
} else {
- stripchart(plot_data$E[topgenes[j], ] ~ factors[, 1], vertical = TRUE, las = 2, pch = 16, cex = 0.8, cex.lab = 0.8, col = cols,
- method = "jitter", ylab = "Normalised log2 expression", main = paste0(labels[j], "\nlogFC=", lfc, ", adj.P.Val=", pval))
+ stripchart(plot_data$E[topgenes[j], ] ~ factors[, 1],
+ vertical = TRUE, las = 2, pch = 16, cex = 0.8, cex.lab = 0.8, col = cols,
+ method = "jitter", ylab = "Normalised log2 expression", main = paste0(labels[j], "\nlogFC=", lfc, ", adj.P.Val=", pval)
+ )
}
}
link_name <- paste0("Stripcharts_", con, ".pdf")
@@ -1039,11 +1083,13 @@
if (want_rda) {
print("Saving RData")
if (want_weight) {
- save(counts, data, y, status, plot_data, labels, factors, wts, fit, top, contrast_data, contrasts, design,
- file = rda_out, ascii = TRUE)
+ save(counts, data, y, status, plot_data, labels, factors, wts, fit, top, contrast_data, contrasts, design,
+ file = rda_out, ascii = TRUE
+ )
} else {
- save(counts, data, y, status, plot_data, labels, factors, fit, top, contrast_data, contrasts, design,
- file = rda_out, ascii = TRUE)
+ save(counts, data, y, status, plot_data, labels, factors, fit, top, contrast_data, contrasts, design,
+ file = rda_out, ascii = TRUE
+ )
}
link_data <- rbind(link_data, c((paste0(de_method, "_analysis.RData")), (paste0(de_method, "_analysis.RData"))))
}
@@ -1053,9 +1099,11 @@
link_data <- rbind(link_data, c("Session Info", "session_info.txt"))
# Record ending time and calculate total run time
-time_end <- as.character(Sys.time())
-time_taken <- capture.output(round(difftime(time_end, time_start), digits = 3))
+time_end <- Sys.time()
+time_taken <- capture.output(round(difftime(time_end, time_start), digits = 2))
time_taken <- gsub("Time difference of ", "", time_taken, fixed = TRUE)
+time_start <- format(time_start, "%A, %B %d, %Y %H:%M:%S")
+time_end <- format(time_end, "%A, %B %d, %Y %H:%M:%S")
################################################################################
### HTML Generation
################################################################################
@@ -1097,35 +1145,35 @@
cata("")
cata("Plots:
\n")
-#PDFs
+# PDFs
for (i in seq_len(nrow(link_data))) {
- if (grepl(".pdf", link_data$Link[i]) & grepl("density|cpm|boxplot|mds|mdplots|voom|saplot", link_data$Link[i])) {
+ if (grepl(".pdf", link_data$Link[i]) && grepl("density|cpm|boxplot|mds|mdplots|voom|saplot", link_data$Link[i])) {
html_link(link_data$Link[i], link_data$Label[i])
- }
+ }
}
for (i in seq_len(nrow(link_data))) {
if (grepl("mdplot_", link_data$Link[i])) {
html_link(link_data$Link[i], link_data$Label[i])
- }
+ }
}
for (i in seq_len(nrow(link_data))) {
if (grepl("volplot", link_data$Link[i])) {
html_link(link_data$Link[i], link_data$Label[i])
- }
+ }
}
for (i in seq_len(nrow(link_data))) {
if (grepl("heatmap", link_data$Link[i])) {
html_link(link_data$Link[i], link_data$Label[i])
- }
+ }
}
for (i in seq_len(nrow(link_data))) {
if (grepl("stripcharts", link_data$Link[i])) {
html_link(link_data$Link[i], link_data$Label[i])
- }
+ }
}
cata("Tables:
\n")
@@ -1148,11 +1196,11 @@
if ("i" %in% plots) {
cata("Glimma Interactive Results:
\n")
- for (i in seq_len(nrow(link_data))) {
- if (grepl("glimma", link_data$Link[i])) {
- html_link(link_data$Link[i], link_data$Label[i])
- }
+ for (i in seq_len(nrow(link_data))) {
+ if (grepl("glimma", link_data$Link[i])) {
+ html_link(link_data$Link[i], link_data$Label[i])
}
+ }
}
cata("Alt-click links to download file.
\n")
@@ -1165,23 +1213,31 @@
if (filt_cpm || filt_smpcount || filt_totcount) {
if (filt_cpm) {
- temp_str <- paste("Genes without more than", opt$cpmReq,
- "CPM in at least", opt$sampleReq, "samples are insignificant",
- "and filtered out.")
+ temp_str <- paste(
+ "Genes without more than", opt$cpmReq,
+ "CPM in at least", opt$sampleReq, "samples are insignificant",
+ "and filtered out."
+ )
} else if (filt_smpcount) {
- temp_str <- paste("Genes without more than", opt$cntReq,
- "counts in at least", opt$sampleReq, "samples are insignificant",
- "and filtered out.")
+ temp_str <- paste(
+ "Genes without more than", opt$cntReq,
+ "counts in at least", opt$sampleReq, "samples are insignificant",
+ "and filtered out."
+ )
} else if (filt_totcount) {
- temp_str <- paste("Genes without more than", opt$cntReq,
- "counts, after summing counts for all samples, are insignificant",
- "and filtered out.")
+ temp_str <- paste(
+ "Genes without more than", opt$cntReq,
+ "counts, after summing counts for all samples, are insignificant",
+ "and filtered out."
+ )
}
list_item(temp_str)
filter_prop <- round(filtered_count / prefilter_count * 100, digits = 2)
- temp_str <- paste0(filtered_count, " of ", prefilter_count, " (", filter_prop,
- "%) genes were filtered out for low expression.")
+ temp_str <- paste0(
+ filtered_count, " of ", prefilter_count, " (", filter_prop,
+ "%) genes were filtered out for low expression."
+ )
list_item(temp_str)
}
list_item(opt$normOpt, " was the method used to normalise library sizes.")
@@ -1207,22 +1263,28 @@
}
if (opt$pAdjOpt != "none") {
if (opt$pAdjOpt == "BH" || opt$pAdjOpt == "BY") {
- temp_str <- paste0("MD Plot highlighted genes are significant at FDR ",
- "of ", opt$pValReq, " and exhibit log2-fold-change of at ",
- "least ", opt$lfcReq, ".")
+ temp_str <- paste0(
+ "MD Plot highlighted genes are significant at FDR ",
+ "of ", opt$pValReq, " and exhibit log2-fold-change of at ",
+ "least ", opt$lfcReq, "."
+ )
list_item(temp_str)
} else if (opt$pAdjOpt == "holm") {
- temp_str <- paste0("MD Plot highlighted genes are significant at adjusted ",
- "p-value of ", opt$pValReq, " by the Holm(1979) ",
- "method, and exhibit log2-fold-change of at least ",
- opt$lfcReq, ".")
+ temp_str <- paste0(
+ "MD Plot highlighted genes are significant at adjusted ",
+ "p-value of ", opt$pValReq, " by the Holm(1979) ",
+ "method, and exhibit log2-fold-change of at least ",
+ opt$lfcReq, "."
+ )
list_item(temp_str)
}
- } else {
- temp_str <- paste0("MD Plot highlighted genes are significant at p-value ",
- "of ", opt$pValReq, " and exhibit log2-fold-change of at ",
- "least ", opt$lfcReq, ".")
- list_item(temp_str)
+} else {
+ temp_str <- paste0(
+ "MD Plot highlighted genes are significant at p-value ",
+ "of ", opt$pValReq, " and exhibit log2-fold-change of at ",
+ "least ", opt$lfcReq, "."
+ )
+ list_item(temp_str)
}
cata("\n")
@@ -1247,65 +1309,88 @@
table_head_item(row.names(factors)[i])
for (j in seq_len(ncol(factors))) {
table_item(as.character(unmake_names(factors[i, j])))
- }
- cata("\n")
+ }
+ cata("\n")
}
cata("")
cit <- character()
link <- character()
-link[1] <- paste0("", "limma User's Guide", ".")
+link[1] <- paste0(
+ "", "limma User's Guide", "."
+)
-link[2] <- paste0("", "edgeR User's Guide", "")
+link[2] <- paste0(
+ "", "edgeR User's Guide", ""
+)
cit[1] <- paste("Please cite the following paper for this tool:")
-cit[2] <- paste("Liu R, Holik AZ, Su S, Jansz N, Chen K, Leong HS, Blewitt ME,",
- "Asselin-Labat ML, Smyth GK, Ritchie ME (2015). Why weight? ",
- "Modelling sample and observational level variability improves power ",
- "in RNA-seq analyses. Nucleic Acids Research, 43(15), e97.")
-
-cit[3] <- paste("Please cite the paper below for the limma software itself.",
- "Please also try to cite the appropriate methodology articles",
- "that describe the statistical methods implemented in limma,",
- "depending on which limma functions you are using. The",
- "methodology articles are listed in Section 2.1 of the",
- link[1],
- "Cite no. 3 only if sample weights were used.")
-cit[4] <- paste("Smyth GK (2005). Limma: linear models for microarray data.",
- "In: 'Bioinformatics and Computational Biology Solutions using",
- "R and Bioconductor'. R. Gentleman, V. Carey, S. doit,.",
- "Irizarry, W. Huber (eds), Springer, New York, pages 397-420.")
-cit[5] <- paste("Please cite the first paper for the software itself and the",
- "other papers for the various original statistical methods",
- "implemented in edgeR. See Section 1.2 in the", link[2],
- "for more detail.")
-cit[6] <- paste("Robinson MD, McCarthy DJ and Smyth GK (2010). edgeR: a",
- "Bioconductor package for differential expression analysis",
- "of digital gene expression data. Bioinformatics 26, 139-140")
-cit[7] <- paste("Robinson MD and Smyth GK (2007). Moderated statistical tests",
- "for assessing differences in tag abundance. Bioinformatics",
- "23, 2881-2887")
-cit[8] <- paste("Robinson MD and Smyth GK (2008). Small-sample estimation of",
- "negative binomial dispersion, with applications to SAGE data.",
- "Biostatistics, 9, 321-332")
-cit[9] <- paste("McCarthy DJ, Chen Y and Smyth GK (2012). Differential",
- "expression analysis of multifactor RNA-Seq experiments with",
- "respect to biological variation. Nucleic Acids Research 40,",
- "4288-4297")
-cit[10] <- paste("Law CW, Chen Y, Shi W, and Smyth GK (2014). Voom:",
- "precision weights unlock linear model analysis tools for",
- "RNA-seq read counts. Genome Biology 15, R29.")
-cit[11] <- paste("Ritchie ME, Diyagama D, Neilson J, van Laar R,",
- "Dobrovic A, Holloway A and Smyth GK (2006).",
- "Empirical array quality weights for microarray data.",
- "BMC Bioinformatics 7, Article 261.")
+cit[2] <- paste(
+ "Liu R, Holik AZ, Su S, Jansz N, Chen K, Leong HS, Blewitt ME,",
+ "Asselin-Labat ML, Smyth GK, Ritchie ME (2015). Why weight? ",
+ "Modelling sample and observational level variability improves power ",
+ "in RNA-seq analyses. Nucleic Acids Research, 43(15), e97."
+)
+cit[3] <- paste(
+ "Please cite the paper below for the limma software itself.",
+ "Please also try to cite the appropriate methodology articles",
+ "that describe the statistical methods implemented in limma,",
+ "depending on which limma functions you are using. The",
+ "methodology articles are listed in Section 2.1 of the",
+ link[1],
+ "Cite no. 3 only if sample weights were used."
+)
+cit[4] <- paste(
+ "Smyth GK (2005). Limma: linear models for microarray data.",
+ "In: 'Bioinformatics and Computational Biology Solutions using",
+ "R and Bioconductor'. R. Gentleman, V. Carey, S. doit,.",
+ "Irizarry, W. Huber (eds), Springer, New York, pages 397-420."
+)
+cit[5] <- paste(
+ "Please cite the first paper for the software itself and the",
+ "other papers for the various original statistical methods",
+ "implemented in edgeR. See Section 1.2 in the", link[2],
+ "for more detail."
+)
+cit[6] <- paste(
+ "Robinson MD, McCarthy DJ and Smyth GK (2010). edgeR: a",
+ "Bioconductor package for differential expression analysis",
+ "of digital gene expression data. Bioinformatics 26, 139-140"
+)
+cit[7] <- paste(
+ "Robinson MD and Smyth GK (2007). Moderated statistical tests",
+ "for assessing differences in tag abundance. Bioinformatics",
+ "23, 2881-2887"
+)
+cit[8] <- paste(
+ "Robinson MD and Smyth GK (2008). Small-sample estimation of",
+ "negative binomial dispersion, with applications to SAGE data.",
+ "Biostatistics, 9, 321-332"
+)
+cit[9] <- paste(
+ "McCarthy DJ, Chen Y and Smyth GK (2012). Differential",
+ "expression analysis of multifactor RNA-Seq experiments with",
+ "respect to biological variation. Nucleic Acids Research 40,",
+ "4288-4297"
+)
+cit[10] <- paste(
+ "Law CW, Chen Y, Shi W, and Smyth GK (2014). Voom:",
+ "precision weights unlock linear model analysis tools for",
+ "RNA-seq read counts. Genome Biology 15, R29."
+)
+cit[11] <- paste(
+ "Ritchie ME, Diyagama D, Neilson J, van Laar R,",
+ "Dobrovic A, Holloway A and Smyth GK (2006).",
+ "Empirical array quality weights for microarray data.",
+ "BMC Bioinformatics 7, Article 261."
+)
cata("Citations
\n")
cata(cit[1], "\n")
cata("
\n")
@@ -1338,13 +1423,16 @@
cata("\n")
cata("\n")
-table_item("Task started at:"); table_item(time_start)
+table_item("Task started at:")
+table_item(time_start)
cata("
\n")
cata("\n")
-table_item("Task ended at:"); table_item(time_end)
+table_item("Task ended at:")
+table_item(time_end)
cata("
\n")
cata("\n")
-table_item("Task run time:"); table_item(time_taken)
+table_item("Task run time:")
+table_item(time_taken)
cata("
\n")
cata("
\n")
diff -r d6f5fa4ee473 -r 119b069fc845 limma_voom.xml
--- a/limma_voom.xml Tue Mar 01 08:03:53 2022 +0000
+++ b/limma_voom.xml Fri Feb 09 17:06:25 2024 +0000
@@ -1,13 +1,12 @@
-
+
Perform differential expression with limma-voom or limma-trend
- 3.50.1
+ 3.58.1
+ 0
+ 23.0
-
- limma
-
topic_3308
@@ -15,16 +14,20 @@
operation_3563
operation_3223
+
+ limma
+ limma
+
bioconductor-limma
- bioconductor-edger
- r-statmod
- r-scales
+ bioconductor-edger
+ r-statmod
+ r-scales
r-rjson
- r-getopt
- r-gplots
- bioconductor-glimma
+ r-getopt
+ r-gplots
+ bioconductor-glimma
+
+
+
+
+
+
@@ -745,12 +754,6 @@
-
-
-
-
-
-