README.md
In Ghoshlab/cytoKernel: Differential expression using kernel-based score test
cytoKernel
cytoKernel: An R/Bioconductor package for differential expression using kernel-based score test for high-dimensional biological data.
cytoKernel computes the
feature-wise p values and their corresponding
adjusted p values in high-dimensional biological experiments.
Method
Liu D, Lin X, Ghosh D."Semiparametric regression of
multi-dimensional genetic pathway data: least-squares
kernel machines and linear mixed models". Biometrics. 2007;63(4):1079-1088.
Zhan X, Patterson AD, Ghosh D. "Kernel approaches for
differential expression analysis of mass spectrometry-based
metabolomics data". BMC Bioinformatics. 2015;16:77. Published 2015 Mar 11.
Liu D, Ghosh D, Lin X. "Estimation and testing for the effect > of a genetic pathway on a disease outcome using logistic
kernel machine regression via logistic mixed models". BMC
Bioinf. 2008; 9(1):292.
https://doi.org/10.1186/1471-2105-9-292
Installing cytoKernel
The R-package cytoKernel can be installed from GitHub using the R package
devtools:
Use to install the latest version of cytoKernel from GitHub:
if (!require("devtools")) install.packages("devtools")
devtools::install_github("Ghoshlab/cytoKernel")
It can also be installed using Bioconductor:
# install BiocManager from CRAN (if not already installed)
if (!requireNamespace("BiocManager", quietly=TRUE))
install.packages("BiocManager")
# install cytoKernel package
BiocManager::install("cytoKernel")
After installation, the package can be loaded into R.
library(cytoKernel)
Using cytoKernel
The main function in the cytoKernel package is CytoK(). The CytoK()
function needs two required objects and three optional objects: (1)
object: a data frame or a matrix or a Summarized Experiment with one
assay object with observations (e.g., cluster-marker combinations or genes) on the rows.
and samples as the columns (e.g. let’s call it dataSE).
(2) group_factor: a binary categorical response variable
that represents the group condition for each sample. For example if the samples represent two different groups or conditions (e.g., before stimulation and after stimulation), provide CytoK() with a phenotype representing which columns in the object are different groups. (e.g. let’s call it groupSamples).
(3) lowerRho (optional) a positive value that represents the lower bound of the kernel parameter. Default is 2.
(4) upperRho (optional) a positive value that represents the upper bound of the kernel parameter. Default is 12.
(5) gridRho (optional) a positive value that represents the number of grid points in the interval of upper and bound of the kernel parameter. Default is 4.
(6) alpha (optional) level of significance to control the False Discovery
rate (FDR). Default is 0.05.
(7) featureVars (optional) Vector of the columns which identify features. If a SummarizedExperiment is used for data, row variables will be used. Default is NULL.
To run the CytoK() function,
CytoKOutput <- CytoK(object = dataSE,
group_factor =groupSamples, lowerRho=2, upperRho=12, gridRho=4,
alpha = 0.05, featureVars = NULL)
Individual slots can be extracted using accessor methods:
CytoKFeatures(CytoKOutput) # extracts the data.frame with shrunken effect size, shrunken effect size sd, unadjusted p value and adjusted p value for each feature
CytoKFeaturesOrdered(CytoKOutput) # extracts the data.frame with shrunken effect size, shrunken effect size sd, unadjusted p value and adjusted p value for each feature ordered by unadjusted p value from low to high
CytoKDEfeatures(CytoKOutput) # extracts the percent of differentially expressed features
CytoKData(CytoKOutput) # extracts the original data object
CytoKalpha(CytoKOutput) # extracts the specified level of significance
CytoKFeatureVars(CytoKOutput) # extracts the value of featureVars
The heatmap of the expressed matrix of features on rows ordered by the adjusted p values from low to high can be directly
plotted using the plotCytoK() function.
plotCytoK(object = CytoKOutput,
group_factor =groupSamples,topK=K,...)
For more details, see vignettes.
Bug reports
Report bugs as issues on the GitHub repository new
issue
Contributors
Ghoshlab/cytoKernel documentation built on Dec. 17, 2021, 9:32 p.m.
R Package Documentation
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cytoKernel
cytoKernel: An R/Bioconductor package for differential expression using kernel-based score test for high-dimensional biological data.
cytoKernel computes the
feature-wise p values and their corresponding
adjusted p values in high-dimensional biological experiments.
Method
Liu D, Lin X, Ghosh D."Semiparametric regression of multi-dimensional genetic pathway data: least-squares kernel machines and linear mixed models". Biometrics. 2007;63(4):1079-1088.
Zhan X, Patterson AD, Ghosh D. "Kernel approaches for differential expression analysis of mass spectrometry-based metabolomics data". BMC Bioinformatics. 2015;16:77. Published 2015 Mar 11.
Liu D, Ghosh D, Lin X. "Estimation and testing for the effect > of a genetic pathway on a disease outcome using logistic kernel machine regression via logistic mixed models". BMC Bioinf. 2008; 9(1):292. https://doi.org/10.1186/1471-2105-9-292
Installing cytoKernel
The R-package cytoKernel can be installed from GitHub using the R package devtools:
Use to install the latest version of cytoKernel from GitHub:
if (!require("devtools")) install.packages("devtools")
devtools::install_github("Ghoshlab/cytoKernel")
It can also be installed using Bioconductor:
# install BiocManager from CRAN (if not already installed)
if (!requireNamespace("BiocManager", quietly=TRUE))
install.packages("BiocManager")
# install cytoKernel package
BiocManager::install("cytoKernel")
After installation, the package can be loaded into R.
library(cytoKernel)
Using cytoKernel
The main function in the cytoKernel package is CytoK(). The CytoK()
function needs two required objects and three optional objects: (1)
object: a data frame or a matrix or a Summarized Experiment with one
assay object with observations (e.g., cluster-marker combinations or genes) on the rows.
and samples as the columns (e.g. let’s call it dataSE).
(2) group_factor: a binary categorical response variable
that represents the group condition for each sample. For example if the samples represent two different groups or conditions (e.g., before stimulation and after stimulation), provide CytoK() with a phenotype representing which columns in the object are different groups. (e.g. let’s call it groupSamples).
(3) lowerRho (optional) a positive value that represents the lower bound of the kernel parameter. Default is 2.
(4) upperRho (optional) a positive value that represents the upper bound of the kernel parameter. Default is 12.
(5) gridRho (optional) a positive value that represents the number of grid points in the interval of upper and bound of the kernel parameter. Default is 4.
(6) alpha (optional) level of significance to control the False Discovery
rate (FDR). Default is 0.05.
(7) featureVars (optional) Vector of the columns which identify features. If a SummarizedExperiment is used for data, row variables will be used. Default is NULL.
To run the CytoK() function,
CytoKOutput <- CytoK(object = dataSE,
group_factor =groupSamples, lowerRho=2, upperRho=12, gridRho=4,
alpha = 0.05, featureVars = NULL)
Individual slots can be extracted using accessor methods:
CytoKFeatures(CytoKOutput) # extracts the data.frame with shrunken effect size, shrunken effect size sd, unadjusted p value and adjusted p value for each feature
CytoKFeaturesOrdered(CytoKOutput) # extracts the data.frame with shrunken effect size, shrunken effect size sd, unadjusted p value and adjusted p value for each feature ordered by unadjusted p value from low to high
CytoKDEfeatures(CytoKOutput) # extracts the percent of differentially expressed features
CytoKData(CytoKOutput) # extracts the original data object
CytoKalpha(CytoKOutput) # extracts the specified level of significance
CytoKFeatureVars(CytoKOutput) # extracts the value of featureVars
The heatmap of the expressed matrix of features on rows ordered by the adjusted p values from low to high can be directly
plotted using the plotCytoK() function.
plotCytoK(object = CytoKOutput,
group_factor =groupSamples,topK=K,...)
For more details, see vignettes.
Bug reports
Report bugs as issues on the GitHub repository new issue
Contributors
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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