Nothing
inst/Scripts/ReadAndSaveSimulation.R
In chipseq: chipseq: A package for analyzing chipseq data
library(ShortRead)
library(chipseq)
simulatedReads <-
readAligned("/home/dsarkar/chipseq-simulation/",
pattern = "allChr.map",
type = "MAQMapShort",
filter = alignQualityFilter(15))
simulatedReads <- as.list(simulatedReads)
save(simulatedReads, file = "simulatedReads.rda")
sessionInfo()
## for across chromosome comparison, we should have started with
## number of reads proportional to chromosome lengths. Instead, we
## had the same number from all chromosomes.
## sampling the results proportional to chromosome lengths will not
## work because the effective lengths of chromosomes are not the same
## as official lengths (due to gaps, repeats, etc.). However, we can
## estimate this "thinning" effect by the proportion of original reads
## for which alignments were found.
library(BSgenome.Mmusculus.UCSC.mm9)
ref.chromlens <- seqlengths(Mmusculus)[names(simulatedReads)]
aligned.reads <- sapply(simulatedReads, function(x) length(x[["+"]]))
## aligned.props <- aligned.reads / 1e6
keep.props <- (aligned.reads/1e6) * (ref.chromlens/1e6)
keep.props <- keep.props / max(keep.props)
## for each chromosome, choose a suitable subset
for (chr in names(simulatedReads))
{
cat(chr, fill = TRUE)
n <- aligned.reads[chr]
x <- rbinom(1, size = n, prob = keep.props[chr])
simulatedReads[[chr]][["+"]] <-
sample(simulatedReads[[chr]][["+"]], x)
}
save(simulatedReads, file = "simulatedReadsSampled.rda")
Try the chipseq package in your browser
Any scripts or data that you put into this service are public.
chipseq documentation built on Nov. 8, 2020, 5:19 p.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.
library(ShortRead)
library(chipseq)
simulatedReads <-
readAligned("/home/dsarkar/chipseq-simulation/",
pattern = "allChr.map",
type = "MAQMapShort",
filter = alignQualityFilter(15))
simulatedReads <- as.list(simulatedReads)
save(simulatedReads, file = "simulatedReads.rda")
sessionInfo()
## for across chromosome comparison, we should have started with
## number of reads proportional to chromosome lengths. Instead, we
## had the same number from all chromosomes.
## sampling the results proportional to chromosome lengths will not
## work because the effective lengths of chromosomes are not the same
## as official lengths (due to gaps, repeats, etc.). However, we can
## estimate this "thinning" effect by the proportion of original reads
## for which alignments were found.
library(BSgenome.Mmusculus.UCSC.mm9)
ref.chromlens <- seqlengths(Mmusculus)[names(simulatedReads)]
aligned.reads <- sapply(simulatedReads, function(x) length(x[["+"]]))
## aligned.props <- aligned.reads / 1e6
keep.props <- (aligned.reads/1e6) * (ref.chromlens/1e6)
keep.props <- keep.props / max(keep.props)
## for each chromosome, choose a suitable subset
for (chr in names(simulatedReads))
{
cat(chr, fill = TRUE)
n <- aligned.reads[chr]
x <- rbinom(1, size = n, prob = keep.props[chr])
simulatedReads[[chr]][["+"]] <-
sample(simulatedReads[[chr]][["+"]], x)
}
save(simulatedReads, file = "simulatedReadsSampled.rda")
Try the chipseq 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.