getPeakReads: Get reads from indexed bam files for defined regions
In dhelekal/mmdiff3: Statistical Testing for ChIP-Seq data sets
Description
Usage
Arguments
Value
See Also
Examples
Description
This function collects all short reads from bam files that map
to pre-defined regions of interest. Note, that it fetches the exact start and
end positions of mapped fragments, not the coverage. In the case of
single-end reads, the left most postions of fragments mapping to the positive
strands and the right most positions of fragments
mapping to the negative strands are stored. To find centers of fragments use
estimateFragmentCenters(). Positions are given relative to the start
of the peak. Also computed are TotalCounts, i.e. number of fragments mapping
to a peak region, as well as number of fragments mapping to forward and
reverse strand.
Usage
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getPeakReads(MD, PeakBoundary = 200, strand.specific = FALSE,
filter.duplicates = FALSE, run.parallel = FALSE, BPPARAM = bpparam())
Arguments
MD
DBAmmd Object. This Object can be created using DBAmmd().
PeakBoundary
Defines flanking regions of peaks.
The estimated fragment length is a good guess
(DEFAULT: 200).
strand.specific
if strand specific reads should be kept apart.
(DEFAULT:FALSE)
filter.duplicates
wether duplicate fragments should be removed.
(DEFAULT: FALSE)
run.parallel
whether to run in parallel
(currently no parallelization implemented)
(DEFAULT: FALSE)
BPPARAM
an optional parameter object passed internally
to bplapply when parallel=TRUE.
If not specified, the parameters last registered with
register will be used.
Value
DBAmmd object with updated slots
See Also
DBAmmd, estimateFragmentCenters
Examples
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## Example using a small data set provided in the MMDiffBamSubset package
# setting the Experiment meta data:
ExpData <- list(dataDir=system.file("extdata", package="MMDiffBamSubset"),
sampleSheet="Cfp1.csv")
MetaData <- list('ExpData' = ExpData)
# Creating a DBAmmd data set:
MMD <- DBAmmd(MetaData)
# defining a small Region for which to get reads:
Regions <- GRanges(seqnames=c('chr1'),
IRanges(start = c(4560912,4677889), end = c(4562680,4679681)))
MMD <- setRegions(MMD,Regions)
MMD <- getPeakReads(MMD)
# To access Left ends of fragments mapping to positive strand:
Reads.L <- Reads(MMD,'Left.p')
# To access Right ends of fragments mapping to negative strand:
Reads.R <- Reads(MMD,'Right.n')
# To access Matrix of TotalCounts:
C.t <- Counts(MMD,whichCounts='T')
# Counts on positive strand:
C.p <- Counts(MMD,whichCounts='p')
# Counts on negative strand:
C.n <- Counts(MMD,whichCounts='n')
dhelekal/mmdiff3 documentation built on July 25, 2019, 8:18 p.m.
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Description Usage Arguments Value See Also Examples
Description
This function collects all short reads from bam files that map
to pre-defined regions of interest. Note, that it fetches the exact start and
end positions of mapped fragments, not the coverage. In the case of
single-end reads, the left most postions of fragments mapping to the positive
strands and the right most positions of fragments
mapping to the negative strands are stored. To find centers of fragments use
estimateFragmentCenters(). Positions are given relative to the start
of the peak. Also computed are TotalCounts, i.e. number of fragments mapping
to a peak region, as well as number of fragments mapping to forward and
reverse strand.
Usage
1 2 | getPeakReads(MD, PeakBoundary = 200, strand.specific = FALSE,
filter.duplicates = FALSE, run.parallel = FALSE, BPPARAM = bpparam())
|
Arguments
MD |
DBAmmd Object. This Object can be created using |
PeakBoundary |
Defines flanking regions of peaks. The estimated fragment length is a good guess (DEFAULT: 200). |
strand.specific |
if strand specific reads should be kept apart. (DEFAULT:FALSE) |
filter.duplicates |
wether duplicate fragments should be removed. (DEFAULT: FALSE) |
run.parallel |
whether to run in parallel (currently no parallelization implemented) (DEFAULT: FALSE) |
BPPARAM |
an optional parameter object passed internally
to |
Value
DBAmmd object with updated slots
See Also
DBAmmd, estimateFragmentCenters
Examples
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 | ## Example using a small data set provided in the MMDiffBamSubset package
# setting the Experiment meta data:
ExpData <- list(dataDir=system.file("extdata", package="MMDiffBamSubset"),
sampleSheet="Cfp1.csv")
MetaData <- list('ExpData' = ExpData)
# Creating a DBAmmd data set:
MMD <- DBAmmd(MetaData)
# defining a small Region for which to get reads:
Regions <- GRanges(seqnames=c('chr1'),
IRanges(start = c(4560912,4677889), end = c(4562680,4679681)))
MMD <- setRegions(MMD,Regions)
MMD <- getPeakReads(MMD)
# To access Left ends of fragments mapping to positive strand:
Reads.L <- Reads(MMD,'Left.p')
# To access Right ends of fragments mapping to negative strand:
Reads.R <- Reads(MMD,'Right.n')
# To access Matrix of TotalCounts:
C.t <- Counts(MMD,whichCounts='T')
# Counts on positive strand:
C.p <- Counts(MMD,whichCounts='p')
# Counts on negative strand:
C.n <- Counts(MMD,whichCounts='n')
|
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