AllCloseByRegions: Extract clusters of RNA editing sites located closely in...
In TransBioInfoLab/rnaEditr: Statistical analysis of RNA editing sites and hyper-editing regions
View source: R/AllCloseByRegions.R
AllCloseByRegions R Documentation
Extract clusters of RNA editing sites located closely in genomic
regions.
Description
A wrapper function to extract clusters of RNA editing sites
that are located closely in genomic regions.
Usage
AllCloseByRegions(
regions_gr,
rnaEditMatrix,
maxGap = 50,
minSites = 3,
progressBar = "time"
)
Arguments
regions_gr
A GRanges object of input genomic regions.
rnaEditMatrix
A matrix (or data frame) of RNA editing level values on
individual sites, with row names as site IDs in the form of
"chrAA:XXXXXXXX", and column names as sample IDs. Please make sure to
follow the format of example dataset (data(rnaedit_df)).
maxGap
An integer, genomic locations within maxGap from each
other are placed into the same cluster. Defaults to 50.
minSites
An integer, minimum number of RNA editing sites within each
resulting cluster. Defaults to 3.
progressBar
Name of the progress bar to use. There are currently five
types of progress bars: "time", "none", "text",
"tk", and "win". Defaults to "time". See
create_progress_bar for more details.
Details
The algorithm of this function is based on the
clusterMaker function in the bumphunter
R package. Each cluster is essentially a group of site locations such that
two consecutive locations in the cluster are separated by less than
maxGap.
Value
A GRanges object containing genomic regions of RNA editing sites
located closely within each input pre-defined genomic region.
See Also
TransformToGR, AllCoeditedRegions,
CreateEditingTable, SummarizeAllRegions,
TestAssociations, AnnotateResults
Examples
data(rnaedit_df)
exm_regions <- TransformToGR(
genes_char = c("PHACTR4", "CCR5", "METTL7A"),
type = "symbol",
genome = "hg19"
)
AllCloseByRegions(
regions_gr = exm_regions,
rnaEditMatrix = rnaedit_df,
maxGap = 50,
minSites = 3,
progressBar = "time"
)
TransBioInfoLab/rnaEditr documentation built on Nov. 29, 2022, 3:31 p.m.
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View source: R/AllCloseByRegions.R
| AllCloseByRegions | R Documentation |
Extract clusters of RNA editing sites located closely in genomic regions.
Description
A wrapper function to extract clusters of RNA editing sites that are located closely in genomic regions.
Usage
AllCloseByRegions( regions_gr, rnaEditMatrix, maxGap = 50, minSites = 3, progressBar = "time" )
Arguments
regions_gr |
A GRanges object of input genomic regions. |
rnaEditMatrix |
A matrix (or data frame) of RNA editing level values on
individual sites, with row names as site IDs in the form of
"chrAA:XXXXXXXX", and column names as sample IDs. Please make sure to
follow the format of example dataset ( |
maxGap |
An integer, genomic locations within |
minSites |
An integer, minimum number of RNA editing sites within each resulting cluster. Defaults to 3. |
progressBar |
Name of the progress bar to use. There are currently five
types of progress bars: |
Details
The algorithm of this function is based on the
clusterMaker function in the bumphunter
R package. Each cluster is essentially a group of site locations such that
two consecutive locations in the cluster are separated by less than
maxGap.
Value
A GRanges object containing genomic regions of RNA editing sites located closely within each input pre-defined genomic region.
See Also
TransformToGR, AllCoeditedRegions,
CreateEditingTable, SummarizeAllRegions,
TestAssociations, AnnotateResults
Examples
data(rnaedit_df)
exm_regions <- TransformToGR(
genes_char = c("PHACTR4", "CCR5", "METTL7A"),
type = "symbol",
genome = "hg19"
)
AllCloseByRegions(
regions_gr = exm_regions,
rnaEditMatrix = rnaedit_df,
maxGap = 50,
minSites = 3,
progressBar = "time"
)
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.
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