In this vignette, we demonstrate the unsegmented block bootstrap functionality implemented in nullranges. “Unsegmented” refers to the fact that this implementation does not consider segmentation of the genome for sampling of blocks, see the segmented block bootstrap vignette for the alternative implementation.
First we use the DNase hypersensitivity peaks in A549 downloaded from AnnotationHub, and pre-processed as described in the nullrangesOldData package.
The following chunk of code evaluates various types of bootstrap/permutation schemes, first within chromosome, and then across chromosome (the default). The default type
is bootstrap, and the default for withinChrom
is FALSE
(bootstrapping with blocks moving across chromosomes).
set.seed(5) # reproducibility
library(microbenchmark)
blockLength <- 5e5
microbenchmark(
list=alist(
p_within=bootRanges(dhs, blockLength=blockLength,
type="permute", withinChrom=TRUE),
b_within=bootRanges(dhs, blockLength=blockLength,
type="bootstrap", withinChrom=TRUE),
p_across=bootRanges(dhs, blockLength=blockLength,
type="permute", withinChrom=FALSE),
b_across=bootRanges(dhs, blockLength=blockLength,
type="bootstrap", withinChrom=FALSE)
), times=10)
## Unit: milliseconds
## expr min lq mean median uq max neval cld
## p_within 897.2097 927.1124 1313.7631 1096.8132 1541.1075 2417.8384 10 b
## b_within 759.5548 818.6938 1268.0355 1083.1196 1654.2082 2363.9962 10 b
## p_across 194.0010 251.6306 354.7816 352.2426 474.0413 503.4351 10 a
## b_across 253.1948 339.3142 454.4203 497.9549 514.1838 668.9512 10 a
We create some synthetic ranges in order to visualize the different options of the unsegmented bootstrap implemented in nullranges.
library(GenomicRanges)
seq_nms <- rep(c("chr1","chr2","chr3"),c(4,5,2))
gr <- GRanges(seqnames=seq_nms,
IRanges(start=c(1,101,121,201,
101,201,216,231,401,
1,101),
width=c(20, 5, 5, 30,
20, 5, 5, 5, 30,
80, 40)),
seqlengths=c(chr1=300,chr2=450,chr3=200),
chr=factor(seq_nms))
The following function uses functionality from plotgardener to plot the ranges. Note in the plotting helper function that chr
will be used to color ranges by chromosome of origin.
suppressPackageStartupMessages(library(plotgardener))
plotGRanges <- function(gr) {
pageCreate(width = 5, height = 2, xgrid = 0,
ygrid = 0, showGuides = FALSE)
for (i in seq_along(seqlevels(gr))) {
chrom <- seqlevels(gr)[i]
chromend <- seqlengths(gr)[[chrom]]
suppressMessages({
p <- pgParams(chromstart = 0, chromend = chromend,
x = 0.5, width = 4*chromend/500, height = 0.5,
at = seq(0, chromend, 50),
fill = colorby("chr", palette=palette.colors))
prngs <- plotRanges(data = gr, params = p,
chrom = chrom,
y = 0.25 + (i-1)*.7,
just = c("left", "bottom"))
annoGenomeLabel(plot = prngs, params = p, y = 0.30 + (i-1)*.7)
})
}
}
Visualizing two permutations of blocks within chromosome:
for (i in 1:2) {
gr_prime <- bootRanges(gr, blockLength=100, type="permute", withinChrom=TRUE)
plotGRanges(gr_prime)
}
Visualizing two bootstraps within chromosome:
Visualizing two permutations of blocks across chromosome. Here we use larger blocks than previously.
for (i in 1:2) {
gr_prime <- bootRanges(gr, blockLength=200, type="permute", withinChrom=FALSE)
plotGRanges(gr_prime)
}
Visualizing two bootstraps across chromosome:
## R version 4.2.0 RC (2022-04-19 r82224)
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## attached base packages:
## [1] grid stats4 stats graphics grDevices utils datasets
## [8] methods base
##
## other attached packages:
## [1] microbenchmark_1.4.9 tidyr_1.2.0
## [3] EnsDb.Hsapiens.v86_2.99.0 ensembldb_2.20.0
## [5] AnnotationFilter_1.20.0 GenomicFeatures_1.48.0
## [7] AnnotationDbi_1.58.0 patchwork_1.1.1
## [9] plyranges_1.16.0 nullrangesData_1.1.1
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## [23] GenomicRanges_1.48.0 GenomeInfoDb_1.32.0
## [25] IRanges_2.30.0 S4Vectors_0.34.0
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