plotStrandedCoverage: Plot strand-specific read coverage for a GRanges object
In yueli-compbio/RIPSeeker: RIPSeeker: a statistical package for identifying protein-associated transcripts from RIP-seq experiments
Description
Usage
Arguments
Details
Author(s)
References
See Also
Examples
Description
Plot read counts within fixed bin across the entire chromosome.
Usage
1
plotStrandedCoverage(gr, binSize = 1000, plotLegend = FALSE, ylim, ...)
Arguments
gr
GRanges object containing the alignments.
binSize
Integer indicate the size of the bin used to compute and plot the read counts.
plotLegend
Binary indcator. If TRUE, legend will be plotted on the top left the plot. Legend is expected to be the chromsome name and length, which must be available in the GRange object argument.
ylim
A two element scale on the y-axis, indicating the maximum read counts on the + and - strand to be plotted (e.g., ylim=c(-200, 200)).
...
Extra arguments passed to plotCoverage.
Details
Read count on + and - strand are displayed as red and blue bars on the positive and negative y-axis, respectively. The x-axis indicates the positions across the chromosmoe. The plot can be used to examine for each chromosome the overall alignment properties such as strand specificity (expected in non-strand-specific sequencing) and aggregation of reads.
Author(s)
Yue Li
References
P. Aboyoun, H. Pages and M. Lawrence (). GenomicRanges: Representation and manipulation of genomic intervals. R package version 1.8.9.
See Also
Examples
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# Retrieve system files
extdata.dir <- system.file("extdata", package="RIPSeeker")
bamFiles <- list.files(extdata.dir, ".bam$", recursive=TRUE, full.names=TRUE)
bamFiles <- grep("PRC2", bamFiles, value=TRUE)
alignGal <- getAlignGal(bamFiles[1], reverseComplement=TRUE, genomeBuild="mm9")
alignGR <- as(alignGal, "GRanges")
alignGRList <- GRangesList(as.list(split(alignGR, seqnames(alignGR))))
binSize <- 1000
plotStrandedCoverage(gr=alignGRList$chrX, binSize=binSize,
xlab="", ylab="", plotLegend=TRUE, box.lty=0, legend.cex=2 )
yueli-compbio/RIPSeeker documentation built on May 8, 2019, 2:34 a.m.
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Description Usage Arguments Details Author(s) References See Also Examples
Description
Plot read counts within fixed bin across the entire chromosome.
Usage
1 | plotStrandedCoverage(gr, binSize = 1000, plotLegend = FALSE, ylim, ...)
|
Arguments
gr |
|
binSize |
Integer indicate the size of the bin used to compute and plot the read counts. |
plotLegend |
Binary indcator. If TRUE, legend will be plotted on the top left the plot. Legend is expected to be the chromsome name and length, which must be available in the GRange object argument. |
ylim |
A two element scale on the y-axis, indicating the maximum read counts on the + and - strand to be plotted (e.g., ylim=c(-200, 200)). |
... |
Extra arguments passed to |
Details
Read count on + and - strand are displayed as red and blue bars on the positive and negative y-axis, respectively. The x-axis indicates the positions across the chromosmoe. The plot can be used to examine for each chromosome the overall alignment properties such as strand specificity (expected in non-strand-specific sequencing) and aggregation of reads.
Author(s)
Yue Li
References
P. Aboyoun, H. Pages and M. Lawrence (). GenomicRanges: Representation and manipulation of genomic intervals. R package version 1.8.9.
See Also
Examples
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 | # Retrieve system files
extdata.dir <- system.file("extdata", package="RIPSeeker")
bamFiles <- list.files(extdata.dir, ".bam$", recursive=TRUE, full.names=TRUE)
bamFiles <- grep("PRC2", bamFiles, value=TRUE)
alignGal <- getAlignGal(bamFiles[1], reverseComplement=TRUE, genomeBuild="mm9")
alignGR <- as(alignGal, "GRanges")
alignGRList <- GRangesList(as.list(split(alignGR, seqnames(alignGR))))
binSize <- 1000
plotStrandedCoverage(gr=alignGRList$chrX, binSize=binSize,
xlab="", ylab="", plotLegend=TRUE, box.lty=0, legend.cex=2 )
|
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