normalize.edaseq: Normalization based on the EDASeq package
In metaseqR: An R package for the analysis and result reporting of RNA-Seq data by combining multiple statistical algorithms.
Description
Usage
Arguments
Value
Author(s)
Examples
View source: R/metaseqr.norm.R
Description
This function is a wrapper over EDASeq normalization. It
accepts a matrix of gene counts (e.g. produced by
importing an externally generated table of counts to the
main metaseqr pipeline).
Usage
1
2
3
normalize.edaseq(gene.counts, sample.list,
norm.args = NULL, gene.data = NULL,
output = c("matrix", "native"))
Arguments
gene.counts
a table where each row represents a
gene and each column a sample. Each cell contains the
read counts for each gene and sample. Such a table can be
produced outside metaseqr and is imported during the
basic metaseqr workflow.
sample.list
the list containing condition names
and the samples under each condition.
norm.args
a list of EDASeq normalization
parameters. See the result of
get.defaults("normalization", "edaseq") for
an example and how you can modify it.
gene.data
an optional annotation data frame (such
the ones produced by get.annotation) which
contains the GC content for each gene and from which the
gene lengths can be inferred by chromosome coordinates.
output
the class of the output object. It can be
"matrix" (default) for versatility with other
tools or "native" for the EDASeq native S4 object
(SeqExpressionSet). In the latter case it should be
handled with suitable EDASeq methods.
Value
A matrix or a SeqExpressionSet with normalized counts.
Author(s)
Panagiotis Moulos
Examples
1
2
3
4
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17
require(DESeq)
data.matrix <- counts(makeExampleCountDataSet())
sample.list <- list(A=c("A1","A2"),B=c("B1","B2","B3"))
diagplot.boxplot(data.matrix,sample.list)
lengths <- round(1000*runif(nrow(data.matrix)))
starts <- round(1000*runif(nrow(data.matrix)))
ends <- starts + lengths
gc=runif(nrow(data.matrix))
gene.data <- data.frame(
chromosome=c(rep("chr1",nrow(data.matrix)/2),
rep("chr2",nrow(data.matrix)/2)),
start=starts,end=ends,gene_id=rownames(data.matrix),gc_content=gc
)
norm.data.matrix <- normalize.edaseq(data.matrix,sample.list,
gene.data=gene.data)
diagplot.boxplot(norm.data.matrix,sample.list)
metaseqR documentation built on Nov. 8, 2020, 5:57 p.m.
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Description Usage Arguments Value Author(s) Examples
View source: R/metaseqr.norm.R
Description
This function is a wrapper over EDASeq normalization. It accepts a matrix of gene counts (e.g. produced by importing an externally generated table of counts to the main metaseqr pipeline).
Usage
1 2 3 | normalize.edaseq(gene.counts, sample.list,
norm.args = NULL, gene.data = NULL,
output = c("matrix", "native"))
|
Arguments
gene.counts |
a table where each row represents a gene and each column a sample. Each cell contains the read counts for each gene and sample. Such a table can be produced outside metaseqr and is imported during the basic metaseqr workflow. |
sample.list |
the list containing condition names and the samples under each condition. |
norm.args |
a list of EDASeq normalization
parameters. See the result of
|
gene.data |
an optional annotation data frame (such
the ones produced by |
output |
the class of the output object. It can be
|
Value
A matrix or a SeqExpressionSet with normalized counts.
Author(s)
Panagiotis Moulos
Examples
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 | require(DESeq)
data.matrix <- counts(makeExampleCountDataSet())
sample.list <- list(A=c("A1","A2"),B=c("B1","B2","B3"))
diagplot.boxplot(data.matrix,sample.list)
lengths <- round(1000*runif(nrow(data.matrix)))
starts <- round(1000*runif(nrow(data.matrix)))
ends <- starts + lengths
gc=runif(nrow(data.matrix))
gene.data <- data.frame(
chromosome=c(rep("chr1",nrow(data.matrix)/2),
rep("chr2",nrow(data.matrix)/2)),
start=starts,end=ends,gene_id=rownames(data.matrix),gc_content=gc
)
norm.data.matrix <- normalize.edaseq(data.matrix,sample.list,
gene.data=gene.data)
diagplot.boxplot(norm.data.matrix,sample.list)
|
R Package Documentation
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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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