Nothing
R/epiNetwork.R
In epihet: Determining Epigenetic Heterogeneity from Bisulfite Sequencing Data
Defines functions
epiNetwork
Documented in
epiNetwork
#' @title Construct co-epihet network based on DEH loci.
#' @description Construct co-epihet network for DEH loci or for genes with
#' genome region containing DEH loci using WGCNA
#' and identify modules that are significantly associated with the measured
#' clinical traits for co-epihet DEH loci network,we identify genes with genome
#' region containing DEH loci in each module.
#' @param node.type a character suggest node type in network. Possible values
#' are 'locus','gene' (default:locus)
#' @param DEH the dataframe containing the chromosome number, loci and strand
#' information of DEH loci generated from diffHet() function
#' @param compare.matrix The comparison matrix generated from
#' the compMatrix() function.
#' @param value A character, which is used to identify DEH loci.
#' Possible values are 'pdr', 'epipoly',and 'shannon'(default:pdr)
#' @param group The subtype group to be used to construct network
#' @param subtype A dataframe containing the subtype information
#' for the samples in the comparison matrix. The row names should
#' be the names of the samples and there should be one column
#' containing the subtype information for each sample
#' @param datTraits a dataframe containing the clinical traits for all patients
#' from the subtype group
#' @param annotation.obj a GRanges object containing gene annotation
#' information
#' @param networktype network type in WGCNA (default:signed)
#' @param method character string specifying the correlation to be
#' used in WGCNA (default:pearson)
#' @param prefix character string containing the file name base for files
#' containing the consensus
#' topological overlaps in WGCNA
#' @param mergeCutHeight a numeric, dendrogram cut height for module merging
#' (default: 0.25)
#' @param minModuleSize a numeric, minimum module size for module detection
#' in WGCNA (default: 30)
#' @return a list, if node type is CpG site, it contains the epigenetic
#' heterogeneity matrix for patients
#' module information, gene.list which is a data frame containing genes with
#' genome region containing DEH loci from one module
#' if node type is gene,it contains the epigenetic heterogeneity matrix for
#' patients and module information.
#' @export
epiNetwork <- function(node.type = "locus", DEH, compare.matrix,
value = "pdr", group, subtype, datTraits = NULL,
annotation.obj, networktype = "signed", method = "pearson",
prefix = NULL, mergeCutHeight = 0.25, minModuleSize = 30) {
# obtain the epigenetic heterogeneity marix on each
# DEH loci for patients from the group subtype
stopifnot(is(annotation.obj,"GRanges"))
group.samples <- subtype[which(subtype[, 2] == group), 1]
compare.matrix <- compare.matrix[which(compare.matrix$type == value), ]
rownames(compare.matrix) <- compare.matrix$location
group.matrix <- compare.matrix[, group.samples]
DEH.loci <- paste(DEH[, 1], DEH[, 2], sep = "-")
value.matrix <- group.matrix[DEH.loci, ]
value.matrix <- t(value.matrix)
DEH.loci <- data.frame(loci = DEH.loci, stringsAsFactors = FALSE)
userset <- userobj(DEH)
o <- GenomicRanges::findOverlaps(userset, annotation.obj)
hit.matrix <- as.matrix(o)
if (node.type == "locus") {
input.matrix = value.matrix
nSamples = nrow(value.matrix)
} else {
geneid <- unique(subjectHits(o))
if (length(geneid) == 0) {
print("no gene annotated by DEH loci")
} else {
i<-NULL
mean.matrix <- foreach(i = geneid, .combine = cbind) %do%
{
gene.name <- mcols(annotation.obj[i])[, 2]
queryhit.id <- hit.matrix[which(hit.matrix[, 2] == i), 1]
queryhit.loci <- mcols(userset[queryhit.id])
epivalue <- value.matrix[, queryhit.loci$loci]
if (nrow(queryhit.loci) == 1) {
data.na <- data.frame(epivalue)
} else {
data.na <- as.data.frame(apply(epivalue, 1, mean))
}
colnames(data.na) <- gene.name
data.na
}
mean.matrix <- mean.matrix[, colSums(mean.matrix) != 0]
nSamples <- dim(mean.matrix)[1]
input.matrix <- mean.matrix
}
}
# Choose a set of soft-thresholding powers
powers <- c(seq_len(10), seq(from = 12, to = 30, by = 2))
# Call the network topology analysis function
sft <- WGCNA::pickSoftThreshold(input.matrix, powerVector = powers,
verbose = 5)
# select beta:
beta <- data.frame(power = sft$fitIndices[, 1],
R2 = -sign(sft$fitIndices[, 3]) * sft$fitIndices[, 2],
stringsAsFactors = FALSE)
if (max(beta$R2) < 0.8) {
if (nSamples < 20) {
if (networktype == "signed") {
softpowers = 20
} else {
softpowers <- 10
}
} else if (nSamples >= 20 & nSamples < 30) {
if (networktype == "signed") {
softpowers <- 18
} else {
softpowers <- 9
}
} else if (nSamples >= 30 & nSamples < 40) {
if (networktype == "signed") {
softpowers <- 16
} else {
softpowers <- 8
}
} else if (nSamples >= 40 & nSamples < 60) {
if (networktype == "signed") {
softpowers <- 14
} else {
softpowers <- 7
}
} else if (nSamples >= 60) {
if (networktype == "signed") {
softpowers <- 12
} else {
softpowers <- 6
}
}
} else {
softpowers <- min(beta$power[beta$R2 > 0.8])
}
net <- WGCNA::blockwiseModules(input.matrix, power = softpowers,
corType = method, networkType = networktype,
TOMType = "unsigned", minModuleSize = minModuleSize,
reassignThreshold = 1e-06, mergeCutHeight = mergeCutHeight,
numericLabels = TRUE, pamRespectsDendro = FALSE,
saveTOMs = TRUE, nThreads = 1, saveTOMFileBase = prefix,
verbose = 3, maxBlockSize = nrow(DEH))
# To see how many modules were identified and what
# the module sizes are
print("the number of modules and the size of each module:")
print(table(net$colors))
moduleLabels <- net$colors
# Convert labels to colors for plotting
moduleColors <- WGCNA::labels2colors(net$colors)
print("save a hierarchical clustering dendrogram for modules in PDF")
pdf(paste("./", prefix, "dengram_module.pdf", sep = ""))
f <- WGCNA::plotDendroAndColors(net$dendrograms[[1]],
moduleColors[net$blockGenes[[1]]], "Module colors",
dendroLabels = FALSE, hang = 0.03, addGuide = TRUE,
guideHang = 0.05)
dev.off()
if (node.type == "locus") {
module <- data.frame(DEHloci = DEH.loci$loci,
label = moduleLabels, color = moduleColors,
stringsAsFactors = FALSE)
} else {
module <- data.frame(gene = colnames(input.matrix),
label = moduleLabels, color = moduleColors,
stringsAsFactors = FALSE)
}
MEs0 <- WGCNA::moduleEigengenes(input.matrix, moduleColors)$eigengenes
print(paste(prefix, "save network, module and module eigengenes",
sep = ":"))
save(net, module, MEs0,
file = paste("./", prefix,"networkConstruction_auto.rda", sep = ""))
# cilinical traits
if (length(datTraits)) {
print("Relating modules to external clinical traits:")
MEs <- WGCNA::orderMEs(MEs0)
moduleTraitCor <- WGCNA::cor(MEs, datTraits,use = "p")
moduleTraitPvalue <- WGCNA::corPvalueStudent(moduleTraitCor,nSamples)
# Will display correlations and their p-values
textMatrix <- paste(signif(moduleTraitCor, 2),
"\n(", signif(moduleTraitPvalue, 1), ")",sep = "")
dim(textMatrix) <- dim(moduleTraitCor)
pdf(paste(prefix, "clinicaltrait_heatmap.pdf",sep = ""))
par(mar = c(6, 8.5, 3, 3))
# Display the correlation values within a heatmap
# plot
h <- WGCNA::labeledHeatmap(Matrix = moduleTraitCor,
xLabels = names(datTraits), yLabels = names(MEs),
ySymbols = names(MEs), colorLabels = FALSE,
colors = WGCNA::blueWhiteRed(50), textMatrix = textMatrix,
setStdMargins = FALSE, cex.text = 0.5,
zlim = c(-1, 1), main = paste("Module-trait relationships"))
print(h)
dev.off()
} else {
print("No clinical traits")
}
# annotate gene with DEH loci
if (node.type == "locus") {
print(" identifying genes involved in modules")
geneset <- data.frame(DEHloci = mcols(userset[hit.matrix[,1]])$loci,
gene = mcols(annotation.obj[hit.matrix[,2]])$name,
stringsAsFactors = FALSE)
gene.module <- merge(geneset, module)
gene.list <- unique(gene.module[, -1])
# plot barplot showing the number of genes in each
# module
gene.num <- as.data.frame(table(gene.list$color))
gene.num$Var2 = paste("ME", gene.num$Var1,sep = "")
Var2<-NULL
Freq<-NULL
g <- ggplot(data = gene.num, aes(x = Var2, y = Freq,fill = Var2)) +
geom_bar(stat = "identity",
colour = "black",
position = position_dodge(width = 0.8),width = 0.7) +
geom_text(aes(label = Freq),position = position_dodge(width = 0.8),
vjust = -0.5)
g <- g + labs(x = "Module", y = "Number of Gene") +
theme(legend.title = element_blank()) +
theme(axis.text.x = element_text(angle = 45,hjust = 1, vjust = 1))+
theme(legend.position = "none") +
scale_fill_manual(values = as.character(gene.num$Var1))
g <- g +
theme(axis.text.x = element_text(size = 10,colour = "black"),
axis.text.y = element_text(size = 10,colour = "black"),
axis.title = element_text(size = 10,colour = "black")) +
theme(axis.line = element_line(size = 0.5,colour = "black"),
panel.background = element_rect(fill = "white",
colour = "darkgrey"),
plot.background = element_rect(fill = "white",
colour = "white"),
strip.text = element_text(size = 12,colour = "black"),
strip.background = element_rect(fill = "white",
colour = "black"))
ggsave(paste(prefix, "num_gene_module.pdf",sep = "_"),
dpi = 300, width = 6, height = 6)
save(gene.list, file = paste("./", prefix,"gene.module.rda", sep = ""))
} else {
gene.num <- as.data.frame(table(module$color))
gene.num$Var2 = paste("ME", gene.num$Var1,sep = "")
Var2<-NULL
Freq<-NULL
g <- ggplot(data = gene.num, aes(x = Var2, y = Freq,fill = Var2)) +
geom_bar(stat = "identity",colour = "black",
position = position_dodge(width = 0.8),width = 0.7) +
geom_text(aes(label = Freq),
position = position_dodge(width = 0.8),vjust = -0.5)
g <- g + labs(x = "Module", y = "Number of Gene") +
theme(legend.title = element_blank()) +
theme(axis.text.x = element_text(angle = 45,
hjust = 1, vjust = 1)) + theme(legend.position = "none") +
scale_fill_manual(values = as.character(gene.num$Var1))
g <- g +
theme(axis.text.x = element_text(size = 10, colour = "black"),
axis.text.y = element_text(size = 10,colour = "black"),
axis.title = element_text(size = 10, colour = "black")) +
theme(axis.line = element_line(size = 0.5, colour = "black"),
panel.background = element_rect(fill = "white",
colour = "darkgrey"),
plot.background = element_rect(fill = "white",
colour = "white"),
strip.text = element_text(size = 12,colour = "black"),
strip.background = element_rect(fill = "white",
colour = "black"))
ggsave(paste(prefix, "num_gene_module.pdf",sep = "_"),
dpi = 300, width = 6, height = 6)
}
if (node.type == "locus") {
result <- list(epimatrix = input.matrix, module = module,
geneofmodule = gene.list)
} else {
result <- list(epimatrix = input.matrix, module = module)
}
return(result)
}
Try the epihet package in your browser
Any scripts or data that you put into this service are public.
epihet documentation built on Dec. 31, 2020, 2:01 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 epiNetwork
Documented in epiNetwork
#' @title Construct co-epihet network based on DEH loci.
#' @description Construct co-epihet network for DEH loci or for genes with
#' genome region containing DEH loci using WGCNA
#' and identify modules that are significantly associated with the measured
#' clinical traits for co-epihet DEH loci network,we identify genes with genome
#' region containing DEH loci in each module.
#' @param node.type a character suggest node type in network. Possible values
#' are 'locus','gene' (default:locus)
#' @param DEH the dataframe containing the chromosome number, loci and strand
#' information of DEH loci generated from diffHet() function
#' @param compare.matrix The comparison matrix generated from
#' the compMatrix() function.
#' @param value A character, which is used to identify DEH loci.
#' Possible values are 'pdr', 'epipoly',and 'shannon'(default:pdr)
#' @param group The subtype group to be used to construct network
#' @param subtype A dataframe containing the subtype information
#' for the samples in the comparison matrix. The row names should
#' be the names of the samples and there should be one column
#' containing the subtype information for each sample
#' @param datTraits a dataframe containing the clinical traits for all patients
#' from the subtype group
#' @param annotation.obj a GRanges object containing gene annotation
#' information
#' @param networktype network type in WGCNA (default:signed)
#' @param method character string specifying the correlation to be
#' used in WGCNA (default:pearson)
#' @param prefix character string containing the file name base for files
#' containing the consensus
#' topological overlaps in WGCNA
#' @param mergeCutHeight a numeric, dendrogram cut height for module merging
#' (default: 0.25)
#' @param minModuleSize a numeric, minimum module size for module detection
#' in WGCNA (default: 30)
#' @return a list, if node type is CpG site, it contains the epigenetic
#' heterogeneity matrix for patients
#' module information, gene.list which is a data frame containing genes with
#' genome region containing DEH loci from one module
#' if node type is gene,it contains the epigenetic heterogeneity matrix for
#' patients and module information.
#' @export
epiNetwork <- function(node.type = "locus", DEH, compare.matrix,
value = "pdr", group, subtype, datTraits = NULL,
annotation.obj, networktype = "signed", method = "pearson",
prefix = NULL, mergeCutHeight = 0.25, minModuleSize = 30) {
# obtain the epigenetic heterogeneity marix on each
# DEH loci for patients from the group subtype
stopifnot(is(annotation.obj,"GRanges"))
group.samples <- subtype[which(subtype[, 2] == group), 1]
compare.matrix <- compare.matrix[which(compare.matrix$type == value), ]
rownames(compare.matrix) <- compare.matrix$location
group.matrix <- compare.matrix[, group.samples]
DEH.loci <- paste(DEH[, 1], DEH[, 2], sep = "-")
value.matrix <- group.matrix[DEH.loci, ]
value.matrix <- t(value.matrix)
DEH.loci <- data.frame(loci = DEH.loci, stringsAsFactors = FALSE)
userset <- userobj(DEH)
o <- GenomicRanges::findOverlaps(userset, annotation.obj)
hit.matrix <- as.matrix(o)
if (node.type == "locus") {
input.matrix = value.matrix
nSamples = nrow(value.matrix)
} else {
geneid <- unique(subjectHits(o))
if (length(geneid) == 0) {
print("no gene annotated by DEH loci")
} else {
i<-NULL
mean.matrix <- foreach(i = geneid, .combine = cbind) %do%
{
gene.name <- mcols(annotation.obj[i])[, 2]
queryhit.id <- hit.matrix[which(hit.matrix[, 2] == i), 1]
queryhit.loci <- mcols(userset[queryhit.id])
epivalue <- value.matrix[, queryhit.loci$loci]
if (nrow(queryhit.loci) == 1) {
data.na <- data.frame(epivalue)
} else {
data.na <- as.data.frame(apply(epivalue, 1, mean))
}
colnames(data.na) <- gene.name
data.na
}
mean.matrix <- mean.matrix[, colSums(mean.matrix) != 0]
nSamples <- dim(mean.matrix)[1]
input.matrix <- mean.matrix
}
}
# Choose a set of soft-thresholding powers
powers <- c(seq_len(10), seq(from = 12, to = 30, by = 2))
# Call the network topology analysis function
sft <- WGCNA::pickSoftThreshold(input.matrix, powerVector = powers,
verbose = 5)
# select beta:
beta <- data.frame(power = sft$fitIndices[, 1],
R2 = -sign(sft$fitIndices[, 3]) * sft$fitIndices[, 2],
stringsAsFactors = FALSE)
if (max(beta$R2) < 0.8) {
if (nSamples < 20) {
if (networktype == "signed") {
softpowers = 20
} else {
softpowers <- 10
}
} else if (nSamples >= 20 & nSamples < 30) {
if (networktype == "signed") {
softpowers <- 18
} else {
softpowers <- 9
}
} else if (nSamples >= 30 & nSamples < 40) {
if (networktype == "signed") {
softpowers <- 16
} else {
softpowers <- 8
}
} else if (nSamples >= 40 & nSamples < 60) {
if (networktype == "signed") {
softpowers <- 14
} else {
softpowers <- 7
}
} else if (nSamples >= 60) {
if (networktype == "signed") {
softpowers <- 12
} else {
softpowers <- 6
}
}
} else {
softpowers <- min(beta$power[beta$R2 > 0.8])
}
net <- WGCNA::blockwiseModules(input.matrix, power = softpowers,
corType = method, networkType = networktype,
TOMType = "unsigned", minModuleSize = minModuleSize,
reassignThreshold = 1e-06, mergeCutHeight = mergeCutHeight,
numericLabels = TRUE, pamRespectsDendro = FALSE,
saveTOMs = TRUE, nThreads = 1, saveTOMFileBase = prefix,
verbose = 3, maxBlockSize = nrow(DEH))
# To see how many modules were identified and what
# the module sizes are
print("the number of modules and the size of each module:")
print(table(net$colors))
moduleLabels <- net$colors
# Convert labels to colors for plotting
moduleColors <- WGCNA::labels2colors(net$colors)
print("save a hierarchical clustering dendrogram for modules in PDF")
pdf(paste("./", prefix, "dengram_module.pdf", sep = ""))
f <- WGCNA::plotDendroAndColors(net$dendrograms[[1]],
moduleColors[net$blockGenes[[1]]], "Module colors",
dendroLabels = FALSE, hang = 0.03, addGuide = TRUE,
guideHang = 0.05)
dev.off()
if (node.type == "locus") {
module <- data.frame(DEHloci = DEH.loci$loci,
label = moduleLabels, color = moduleColors,
stringsAsFactors = FALSE)
} else {
module <- data.frame(gene = colnames(input.matrix),
label = moduleLabels, color = moduleColors,
stringsAsFactors = FALSE)
}
MEs0 <- WGCNA::moduleEigengenes(input.matrix, moduleColors)$eigengenes
print(paste(prefix, "save network, module and module eigengenes",
sep = ":"))
save(net, module, MEs0,
file = paste("./", prefix,"networkConstruction_auto.rda", sep = ""))
# cilinical traits
if (length(datTraits)) {
print("Relating modules to external clinical traits:")
MEs <- WGCNA::orderMEs(MEs0)
moduleTraitCor <- WGCNA::cor(MEs, datTraits,use = "p")
moduleTraitPvalue <- WGCNA::corPvalueStudent(moduleTraitCor,nSamples)
# Will display correlations and their p-values
textMatrix <- paste(signif(moduleTraitCor, 2),
"\n(", signif(moduleTraitPvalue, 1), ")",sep = "")
dim(textMatrix) <- dim(moduleTraitCor)
pdf(paste(prefix, "clinicaltrait_heatmap.pdf",sep = ""))
par(mar = c(6, 8.5, 3, 3))
# Display the correlation values within a heatmap
# plot
h <- WGCNA::labeledHeatmap(Matrix = moduleTraitCor,
xLabels = names(datTraits), yLabels = names(MEs),
ySymbols = names(MEs), colorLabels = FALSE,
colors = WGCNA::blueWhiteRed(50), textMatrix = textMatrix,
setStdMargins = FALSE, cex.text = 0.5,
zlim = c(-1, 1), main = paste("Module-trait relationships"))
print(h)
dev.off()
} else {
print("No clinical traits")
}
# annotate gene with DEH loci
if (node.type == "locus") {
print(" identifying genes involved in modules")
geneset <- data.frame(DEHloci = mcols(userset[hit.matrix[,1]])$loci,
gene = mcols(annotation.obj[hit.matrix[,2]])$name,
stringsAsFactors = FALSE)
gene.module <- merge(geneset, module)
gene.list <- unique(gene.module[, -1])
# plot barplot showing the number of genes in each
# module
gene.num <- as.data.frame(table(gene.list$color))
gene.num$Var2 = paste("ME", gene.num$Var1,sep = "")
Var2<-NULL
Freq<-NULL
g <- ggplot(data = gene.num, aes(x = Var2, y = Freq,fill = Var2)) +
geom_bar(stat = "identity",
colour = "black",
position = position_dodge(width = 0.8),width = 0.7) +
geom_text(aes(label = Freq),position = position_dodge(width = 0.8),
vjust = -0.5)
g <- g + labs(x = "Module", y = "Number of Gene") +
theme(legend.title = element_blank()) +
theme(axis.text.x = element_text(angle = 45,hjust = 1, vjust = 1))+
theme(legend.position = "none") +
scale_fill_manual(values = as.character(gene.num$Var1))
g <- g +
theme(axis.text.x = element_text(size = 10,colour = "black"),
axis.text.y = element_text(size = 10,colour = "black"),
axis.title = element_text(size = 10,colour = "black")) +
theme(axis.line = element_line(size = 0.5,colour = "black"),
panel.background = element_rect(fill = "white",
colour = "darkgrey"),
plot.background = element_rect(fill = "white",
colour = "white"),
strip.text = element_text(size = 12,colour = "black"),
strip.background = element_rect(fill = "white",
colour = "black"))
ggsave(paste(prefix, "num_gene_module.pdf",sep = "_"),
dpi = 300, width = 6, height = 6)
save(gene.list, file = paste("./", prefix,"gene.module.rda", sep = ""))
} else {
gene.num <- as.data.frame(table(module$color))
gene.num$Var2 = paste("ME", gene.num$Var1,sep = "")
Var2<-NULL
Freq<-NULL
g <- ggplot(data = gene.num, aes(x = Var2, y = Freq,fill = Var2)) +
geom_bar(stat = "identity",colour = "black",
position = position_dodge(width = 0.8),width = 0.7) +
geom_text(aes(label = Freq),
position = position_dodge(width = 0.8),vjust = -0.5)
g <- g + labs(x = "Module", y = "Number of Gene") +
theme(legend.title = element_blank()) +
theme(axis.text.x = element_text(angle = 45,
hjust = 1, vjust = 1)) + theme(legend.position = "none") +
scale_fill_manual(values = as.character(gene.num$Var1))
g <- g +
theme(axis.text.x = element_text(size = 10, colour = "black"),
axis.text.y = element_text(size = 10,colour = "black"),
axis.title = element_text(size = 10, colour = "black")) +
theme(axis.line = element_line(size = 0.5, colour = "black"),
panel.background = element_rect(fill = "white",
colour = "darkgrey"),
plot.background = element_rect(fill = "white",
colour = "white"),
strip.text = element_text(size = 12,colour = "black"),
strip.background = element_rect(fill = "white",
colour = "black"))
ggsave(paste(prefix, "num_gene_module.pdf",sep = "_"),
dpi = 300, width = 6, height = 6)
}
if (node.type == "locus") {
result <- list(epimatrix = input.matrix, module = module,
geneofmodule = gene.list)
} else {
result <- list(epimatrix = input.matrix, module = module)
}
return(result)
}
Try the epihet 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.
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.