R/quickMap.R
In Krutik6/TimiRGeN: Time sensitive microRNA-mRNA integration, analysis and network generation tool
Defines functions
quickMap
Documented in
quickMap
#' @title quickMap
#' @description Generates a heatmap of all miRNA:mRNA binding pairs that
#' have been filtered. Pairs are ranked by decreasing correlation.
#' @param filt_df Dataframe from the matrixFilter function.
#' @param numpairs Number of pairs to plot. Must be an integer more than 1.
#' @return Heatmap of miRNA-mRNA pairs.
#' @export
#' @usage quickMap(filt_df, numpairs)
#' @importFrom gplots heatmap.2
#' @examples
#' Filt_df <- data.frame(row.names = c("mmu-miR-145a-3p:Adamts15",
#' "mmu-miR-146a-5p:Acy1"),
#' corr = c(-0.9191653, -0.7826041),
#' miR = c("mmu-miR-145a-3p", "mmu-miR-146a-5p"),
#' mRNA = c("Adamts15", "Acy1"),
#' miR_Entrez = c(387163, NA),
#' mRNA_Entrez = c(235130, 109652),
#' TargetScan = c(1, 0),
#' miRDB = c(0, 0),
#' Predicted_Interactions = c(1, 0),
#' miRTarBase = c(0, 1),
#' Pred_Fun = c(1, 1))
#'
#' MAE <- MultiAssayExperiment()
#'
#' MAE <- matrixFilter(MAE, miningMatrix = Filt_df, negativeOnly = FALSE,
#' threshold = 1, predictedOnly = FALSE)
#'
#' quickMap(filt_df = MAE[[1]], numpairs = 2)
quickMap <- function(filt_df, numpairs){
if (missing(filt_df)) stop('filt_df is missing. Add the assay/ dataframe which is the output from matrixFiler.')
if (missing(numpairs)) stop('numpairs is missing. Add an integer greater than 1.')
tracecol <- NULL
Ranks <- filt_df[,c(1,2,3)][order(filt_df$corr, decreasing = FALSE),]
Ranks$miR <- Ranks$mRNA <- NULL
Ranks <- as.matrix(Ranks)
Ranks <- cbind(Ranks[,1], Ranks[,1])
par(oma = c(0, 2, 0, 12))
par(cex.main=1.5)
Ranks[order(Ranks)]
my_palette <- grDevices::colorRampPalette(c("red", "yellow", "white", "cyan",
"blue"))(n = 200)
x <- seq(1:numpairs)
heatmap.2(Ranks[1:numpairs,],
trace = "n",
labCol = "",
ylab = "",
Colv = FALSE,
dendrogram = "none",
labRow = paste0(x, " : ", rownames(Ranks[1:numpairs,])),
main = "miR-mRNA pairs",
cexRow = 1.2,
key.title = "",
Rowv=FALSE,
rowsep=c(1:numpairs),
sepcolor="white",
key.xlab = "Corr",
key.ylab = "",
col = my_palette,
density.info=c("none"),
denscol=tracecol)
}
Krutik6/TimiRGeN documentation built on Jan. 27, 2024, 7:46 p.m.
R Package Documentation
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Defines functions quickMap
Documented in quickMap
#' @title quickMap
#' @description Generates a heatmap of all miRNA:mRNA binding pairs that
#' have been filtered. Pairs are ranked by decreasing correlation.
#' @param filt_df Dataframe from the matrixFilter function.
#' @param numpairs Number of pairs to plot. Must be an integer more than 1.
#' @return Heatmap of miRNA-mRNA pairs.
#' @export
#' @usage quickMap(filt_df, numpairs)
#' @importFrom gplots heatmap.2
#' @examples
#' Filt_df <- data.frame(row.names = c("mmu-miR-145a-3p:Adamts15",
#' "mmu-miR-146a-5p:Acy1"),
#' corr = c(-0.9191653, -0.7826041),
#' miR = c("mmu-miR-145a-3p", "mmu-miR-146a-5p"),
#' mRNA = c("Adamts15", "Acy1"),
#' miR_Entrez = c(387163, NA),
#' mRNA_Entrez = c(235130, 109652),
#' TargetScan = c(1, 0),
#' miRDB = c(0, 0),
#' Predicted_Interactions = c(1, 0),
#' miRTarBase = c(0, 1),
#' Pred_Fun = c(1, 1))
#'
#' MAE <- MultiAssayExperiment()
#'
#' MAE <- matrixFilter(MAE, miningMatrix = Filt_df, negativeOnly = FALSE,
#' threshold = 1, predictedOnly = FALSE)
#'
#' quickMap(filt_df = MAE[[1]], numpairs = 2)
quickMap <- function(filt_df, numpairs){
if (missing(filt_df)) stop('filt_df is missing. Add the assay/ dataframe which is the output from matrixFiler.')
if (missing(numpairs)) stop('numpairs is missing. Add an integer greater than 1.')
tracecol <- NULL
Ranks <- filt_df[,c(1,2,3)][order(filt_df$corr, decreasing = FALSE),]
Ranks$miR <- Ranks$mRNA <- NULL
Ranks <- as.matrix(Ranks)
Ranks <- cbind(Ranks[,1], Ranks[,1])
par(oma = c(0, 2, 0, 12))
par(cex.main=1.5)
Ranks[order(Ranks)]
my_palette <- grDevices::colorRampPalette(c("red", "yellow", "white", "cyan",
"blue"))(n = 200)
x <- seq(1:numpairs)
heatmap.2(Ranks[1:numpairs,],
trace = "n",
labCol = "",
ylab = "",
Colv = FALSE,
dendrogram = "none",
labRow = paste0(x, " : ", rownames(Ranks[1:numpairs,])),
main = "miR-mRNA pairs",
cexRow = 1.2,
key.title = "",
Rowv=FALSE,
rowsep=c(1:numpairs),
sepcolor="white",
key.xlab = "Corr",
key.ylab = "",
col = my_palette,
density.info=c("none"),
denscol=tracecol)
}
R Package Documentation
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We want your feedback!
Note that we can't provide technical support on individual packages. You should contact the package authors for that.
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