readTranscriptFeatures-methods: Function for reading exon intron and promoter structure from...
In genomation: Summary, annotation and visualization of genomic data
Description
Usage
Arguments
Value
Note
Examples
Description
Function for reading exon intron and promoter structure from a given bed file
Usage
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readTranscriptFeatures(location,remove.unusual=TRUE,
up.flank=1000,down.flank=1000,unique.prom=TRUE)
## S4 method for signature 'character'
readTranscriptFeatures(location, remove.unusual = TRUE,
up.flank = 1000, down.flank = 1000, unique.prom = TRUE)
Arguments
location
location of the bed file with 12 or more columns.
The file can end in .gz, .bz2, .xz, or .zip
and/or start with http:// or ftp://. If the file is not compressed
it can also start with https:// or ftps://.
remove.unusual
remove the chromomesomes with unsual names, mainly random chromsomes etc
up.flank
up-stream from TSS to detect promoter boundaries
down.flank
down-stream from TSS to detect promoter boundaries
unique.prom
get only the unique promoters, promoter boundaries will not have
a gene name if you set this option to be TRUE
Value
a GRangesList containing locations of exon/intron/promoter/TSS
Note
one bed track per file is only accepted, the bed files with multiple tracks will cause en error
Examples
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my.bed12.file = system.file("extdata/chr21.refseq.hg19.bed", package = "genomation")
my.bed12.file
feats = readTranscriptFeatures(my.bed12.file)
names(feats)
sapply(feats, head)
genomation documentation built on Nov. 8, 2020, 5:21 p.m.
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Description Usage Arguments Value Note Examples
Description
Function for reading exon intron and promoter structure from a given bed file
Usage
1 2 3 4 5 6 | readTranscriptFeatures(location,remove.unusual=TRUE,
up.flank=1000,down.flank=1000,unique.prom=TRUE)
## S4 method for signature 'character'
readTranscriptFeatures(location, remove.unusual = TRUE,
up.flank = 1000, down.flank = 1000, unique.prom = TRUE)
|
Arguments
location |
location of the bed file with 12 or more columns.
The file can end in |
remove.unusual |
remove the chromomesomes with unsual names, mainly random chromsomes etc |
up.flank |
up-stream from TSS to detect promoter boundaries |
down.flank |
down-stream from TSS to detect promoter boundaries |
unique.prom |
get only the unique promoters, promoter boundaries will not have a gene name if you set this option to be TRUE |
Value
a GRangesList containing locations of exon/intron/promoter/TSS
Note
one bed track per file is only accepted, the bed files with multiple tracks will cause en error
Examples
1 2 3 4 5 | my.bed12.file = system.file("extdata/chr21.refseq.hg19.bed", package = "genomation")
my.bed12.file
feats = readTranscriptFeatures(my.bed12.file)
names(feats)
sapply(feats, head)
|
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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