| Platforms | OS | R CMD check | |:----------------:|:----------------:|:----------------:| | Travis CI | Linux | | | Bioc (devel) | Multiple | | | Bioc (release) | Multiple | |
pcaExplorer
is a Bioconductor package containing a Shiny application for
analyzing expression data in different conditions and experimental factors.
It is a general-purpose interactive companion tool for RNA-seq analysis, which guides the user in exploring the Principal Components of the data under inspection.
pcaExplorer
provides tools and functionality to detect outlier samples, genes
that show particular patterns, and additionally provides a functional interpretation of
the principal components for further quality assessment and hypothesis generation
on the input data.
Moreover, a novel visualization approach is presented to simultaneously assess the effect of more than one experimental factor on the expression levels.
Thanks to its interactive/reactive design, it is designed to become a practical companion to any RNA-seq dataset analysis, making exploratory data analysis accessible also to the bench biologist, while providing additional insight also for the experienced data analyst.
pcaExplorer
can be easily installed using BiocManager::install()
:
if (!requireNamespace("BiocManager", quietly=TRUE))
install.packages("BiocManager")
BiocManager::install("pcaExplorer")
or, optionally,
BiocManager::install("federicomarini/pcaExplorer")
# or alternatively...
devtools::install_github("federicomarini/pcaExplorer")
This command loads the pcaExplorer
package
library("pcaExplorer")
The pcaExplorer
app can be launched in different modes:
pcaExplorer(dds = dds, dst = dst)
, where dds
is a DESeqDataSet
object and dst
is a DESeqTransform
object, which were created during an existing session for the analysis of an RNA-seq
dataset with the DESeq2
package
pcaExplorer(dds = dds)
, where dds
is a DESeqDataSet
object. The dst
object is automatically
computed upon launch.
pcaExplorer(countmatrix = countmatrix, coldata = coldata)
, where countmatrix
is a count matrix, generated
after assigning reads to features such as genes via tools such as HTSeq-count
or featureCounts
, and coldata
is a data frame containing the experimental covariates of the experiments, such as condition, tissue, cell line,
run batch and so on.
pcaExplorer()
, and then subsequently uploading the count matrix and the covariates data frame through the
user interface. These files need to be formatted as tab separated files, which is a common format for storing
such count values.
Additional parameters and objects that can be provided to the main pcaExplorer
function are:
pca2go
, which is an object created by the pca2go
function, which scans the genes with high loadings in
each principal component and each direction, and looks for functions (such as GO Biological Processes) that
are enriched above the background. The offline pca2go
function is based on the routines and algorithms of
the topGO
package, but as an alternative, this object can be computed live during the execution of the app
exploiting the goana
function, provided by the limma
package. Although this likely provides more general
(and probably less informative) functions, it is a good compromise for obtaining a further data interpretation.
annotation
, a data frame object, with row.names
as gene identifiers (e.g. ENSEMBL ids) identical to the
row names of the count matrix or dds
object, and an extra column gene_name
, containing e.g. HGNC-based
gene symbols. This can be used for making information extraction easier, as ENSEMBL ids (a usual choice when
assigning reads to features) do not provide an immediate readout for which gene they refer to. This can be
either passed as a parameter when launching the app, or also uploaded as a tab separated text file.
For additional details regarding the functions of pcaExplorer, please consult the documentation or write an email to marinif@uni-mainz.de.
Please use https://github.com/federicomarini/pcaExplorer/issues for reporting bugs, issues or for suggesting new features to be implemented.
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