R/gs_alluvial.R
In federicomarini/GeneTonic: Enjoy Analyzing And Integrating The Results From Differential Expression Analysis And Functional Enrichment Analysis
Defines functions
gs_alluvial
Documented in
gs_alluvial
#' Alluvial (sankey) plot for a set of genesets and the associated genes
#'
#' Generate an interactive alluvial plot linking genesets to their associated
#' genes
#'
#' @param res_enrich A `data.frame` object, storing the result of the functional
#' enrichment analysis. See more in the main function, [GeneTonic()], to check the
#' formatting requirements (a minimal set of columns should be present).
#' @param res_de A `DESeqResults` object.
#' @param annotation_obj A `data.frame` object with the feature annotation
#' information, with at least two columns, `gene_id` and `gene_name`.
#' @param gtl A `GeneTonic`-list object, containing in its slots the arguments
#' specified above: `dds`, `res_de`, `res_enrich`, and `annotation_obj` - the names
#' of the list _must_ be specified following the content they are expecting
#' @param n_gs Integer value, corresponding to the maximal number of gene sets to
#' be displayed
#' @param gs_ids Character vector, containing a subset of `gs_id` as they are
#' available in `res_enrich`. Lists the gene sets to be displayed.
#'
#' @return A `plotly` object
#' @export
#'
#' @examples
#'
#' library("macrophage")
#' library("DESeq2")
#' library("org.Hs.eg.db")
#' library("AnnotationDbi")
#'
#' # dds object
#' data("gse", package = "macrophage")
#' dds_macrophage <- DESeqDataSet(gse, design = ~ line + condition)
#' rownames(dds_macrophage) <- substr(rownames(dds_macrophage), 1, 15)
#' dds_macrophage <- estimateSizeFactors(dds_macrophage)
#'
#' # annotation object
#' anno_df <- data.frame(
#' gene_id = rownames(dds_macrophage),
#' gene_name = mapIds(org.Hs.eg.db,
#' keys = rownames(dds_macrophage),
#' column = "SYMBOL",
#' keytype = "ENSEMBL"
#' ),
#' stringsAsFactors = FALSE,
#' row.names = rownames(dds_macrophage)
#' )
#'
#' # res object
#' data(res_de_macrophage, package = "GeneTonic")
#' res_de <- res_macrophage_IFNg_vs_naive
#'
#' # res_enrich object
#' data(res_enrich_macrophage, package = "GeneTonic")
#' res_enrich <- shake_topGOtableResult(topgoDE_macrophage_IFNg_vs_naive)
#' res_enrich <- get_aggrscores(res_enrich, res_de, anno_df)
#'
#' gs_alluvial(
#' res_enrich = res_enrich,
#' res_de = res_de,
#' annotation_obj = anno_df,
#' n_gs = 4
#' )
#' # or using the alias...
#' gs_sankey(
#' res_enrich = res_enrich,
#' res_de = res_de,
#' annotation_obj = anno_df,
#' n_gs = 4
#' )
gs_alluvial <- function(res_enrich,
res_de,
annotation_obj,
gtl = NULL,
n_gs = 5,
gs_ids = NULL) {
if (!is.null(gtl)) {
checkup_gtl(gtl)
dds <- gtl$dds
res_de <- gtl$res_de
res_enrich <- gtl$res_enrich
annotation_obj <- gtl$annotation_obj
}
# res_enhanced <- get_aggrscores(res_enrich, res_de, annotation_obj = annotation_obj)
n_gs <- min(n_gs, nrow(res_enrich))
gs_to_use <- unique(
c(
res_enrich$gs_id[seq_len(n_gs)], # the ones from the top
gs_ids[gs_ids %in% res_enrich$gs_id] # the ones specified from the custom list
)
)
enrich2list <- lapply(gs_to_use, function(gs) {
go_genes <- res_enrich[gs, "gs_genes"]
go_genes <- unlist(strsplit(go_genes, ","))
return(go_genes)
})
names(enrich2list) <- res_enrich[gs_to_use, "gs_description"]
list2df <- lapply(seq_along(enrich2list), function(gs) {
data.frame(
gsid = rep(names(enrich2list[gs]), length(enrich2list[[gs]])),
gene = enrich2list[[gs]]
)
})
list2df <- do.call("rbind", list2df)
list2df$value <- 1
colnames(list2df) <- c("source", "target", "value")
list2df$source <- as.character(list2df$source)
list2df$target <- as.character(list2df$target)
list2df$target <- paste(list2df$target, " ", sep = "") # genes might need a space for better rendering...
# From these flows we need to create a node data frame: it lists every entities involved in the flow
nodes <- data.frame(
name = c(as.character(list2df$source), as.character(list2df$target)) %>% unique()
)
# connections must be provided using id, not using real name like in the links data.frame...
list2df$id_source <- match(list2df$source, nodes$name) - 1
list2df$id_target <- match(list2df$target, nodes$name) - 1
# list2df %>% head
allnodes <- c(unique(list2df$source), unique(list2df$target))
allcols <- c(
viridis(length(unique(list2df$source))), # for genesets
rep("steelblue", length(unique(list2df$target))) # for genes
)
p <- plot_ly(
type = "sankey",
domain = list(
x = c(0, 1),
y = c(0, 1)
),
orientation = "h",
valueformat = ".0f",
# valuesuffix = " genes in the set",
node = list(
label = allnodes,
color = allcols,
pad = 15,
thickness = 20,
line = list(color = "black", width = 0.5)
),
link = list(
source = list2df$id_source,
target = list2df$id_target,
value = list2df$value
)
) %>%
plotly::layout(
title = "Geneset-Gene Sankey Diagram", font = list(size = 10)
)
return(p)
}
#' @rdname gs_alluvial
#' @export
gs_sankey <- gs_alluvial
federicomarini/GeneTonic documentation built on March 27, 2024, 4:19 p.m.
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Defines functions gs_alluvial
Documented in gs_alluvial
#' Alluvial (sankey) plot for a set of genesets and the associated genes
#'
#' Generate an interactive alluvial plot linking genesets to their associated
#' genes
#'
#' @param res_enrich A `data.frame` object, storing the result of the functional
#' enrichment analysis. See more in the main function, [GeneTonic()], to check the
#' formatting requirements (a minimal set of columns should be present).
#' @param res_de A `DESeqResults` object.
#' @param annotation_obj A `data.frame` object with the feature annotation
#' information, with at least two columns, `gene_id` and `gene_name`.
#' @param gtl A `GeneTonic`-list object, containing in its slots the arguments
#' specified above: `dds`, `res_de`, `res_enrich`, and `annotation_obj` - the names
#' of the list _must_ be specified following the content they are expecting
#' @param n_gs Integer value, corresponding to the maximal number of gene sets to
#' be displayed
#' @param gs_ids Character vector, containing a subset of `gs_id` as they are
#' available in `res_enrich`. Lists the gene sets to be displayed.
#'
#' @return A `plotly` object
#' @export
#'
#' @examples
#'
#' library("macrophage")
#' library("DESeq2")
#' library("org.Hs.eg.db")
#' library("AnnotationDbi")
#'
#' # dds object
#' data("gse", package = "macrophage")
#' dds_macrophage <- DESeqDataSet(gse, design = ~ line + condition)
#' rownames(dds_macrophage) <- substr(rownames(dds_macrophage), 1, 15)
#' dds_macrophage <- estimateSizeFactors(dds_macrophage)
#'
#' # annotation object
#' anno_df <- data.frame(
#' gene_id = rownames(dds_macrophage),
#' gene_name = mapIds(org.Hs.eg.db,
#' keys = rownames(dds_macrophage),
#' column = "SYMBOL",
#' keytype = "ENSEMBL"
#' ),
#' stringsAsFactors = FALSE,
#' row.names = rownames(dds_macrophage)
#' )
#'
#' # res object
#' data(res_de_macrophage, package = "GeneTonic")
#' res_de <- res_macrophage_IFNg_vs_naive
#'
#' # res_enrich object
#' data(res_enrich_macrophage, package = "GeneTonic")
#' res_enrich <- shake_topGOtableResult(topgoDE_macrophage_IFNg_vs_naive)
#' res_enrich <- get_aggrscores(res_enrich, res_de, anno_df)
#'
#' gs_alluvial(
#' res_enrich = res_enrich,
#' res_de = res_de,
#' annotation_obj = anno_df,
#' n_gs = 4
#' )
#' # or using the alias...
#' gs_sankey(
#' res_enrich = res_enrich,
#' res_de = res_de,
#' annotation_obj = anno_df,
#' n_gs = 4
#' )
gs_alluvial <- function(res_enrich,
res_de,
annotation_obj,
gtl = NULL,
n_gs = 5,
gs_ids = NULL) {
if (!is.null(gtl)) {
checkup_gtl(gtl)
dds <- gtl$dds
res_de <- gtl$res_de
res_enrich <- gtl$res_enrich
annotation_obj <- gtl$annotation_obj
}
# res_enhanced <- get_aggrscores(res_enrich, res_de, annotation_obj = annotation_obj)
n_gs <- min(n_gs, nrow(res_enrich))
gs_to_use <- unique(
c(
res_enrich$gs_id[seq_len(n_gs)], # the ones from the top
gs_ids[gs_ids %in% res_enrich$gs_id] # the ones specified from the custom list
)
)
enrich2list <- lapply(gs_to_use, function(gs) {
go_genes <- res_enrich[gs, "gs_genes"]
go_genes <- unlist(strsplit(go_genes, ","))
return(go_genes)
})
names(enrich2list) <- res_enrich[gs_to_use, "gs_description"]
list2df <- lapply(seq_along(enrich2list), function(gs) {
data.frame(
gsid = rep(names(enrich2list[gs]), length(enrich2list[[gs]])),
gene = enrich2list[[gs]]
)
})
list2df <- do.call("rbind", list2df)
list2df$value <- 1
colnames(list2df) <- c("source", "target", "value")
list2df$source <- as.character(list2df$source)
list2df$target <- as.character(list2df$target)
list2df$target <- paste(list2df$target, " ", sep = "") # genes might need a space for better rendering...
# From these flows we need to create a node data frame: it lists every entities involved in the flow
nodes <- data.frame(
name = c(as.character(list2df$source), as.character(list2df$target)) %>% unique()
)
# connections must be provided using id, not using real name like in the links data.frame...
list2df$id_source <- match(list2df$source, nodes$name) - 1
list2df$id_target <- match(list2df$target, nodes$name) - 1
# list2df %>% head
allnodes <- c(unique(list2df$source), unique(list2df$target))
allcols <- c(
viridis(length(unique(list2df$source))), # for genesets
rep("steelblue", length(unique(list2df$target))) # for genes
)
p <- plot_ly(
type = "sankey",
domain = list(
x = c(0, 1),
y = c(0, 1)
),
orientation = "h",
valueformat = ".0f",
# valuesuffix = " genes in the set",
node = list(
label = allnodes,
color = allcols,
pad = 15,
thickness = 20,
line = list(color = "black", width = 0.5)
),
link = list(
source = list2df$id_source,
target = list2df$id_target,
value = list2df$value
)
) %>%
plotly::layout(
title = "Geneset-Gene Sankey Diagram", font = list(size = 10)
)
return(p)
}
#' @rdname gs_alluvial
#' @export
gs_sankey <- gs_alluvial
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