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RCPA is a software package designed for for Consensus Pathway Analysis (RCPA) that im- plements a complete analysis pipeline including: i) download and process data from NCBI Gene Expression Omnibus, ii) perform differential analysis using techniques developed for both microarray and sequencing data, iii) perform pathway analysis using different methods for enrichment analysis and topology-based (TB) analysis, iv) perform meta-analysis and combine methods and datasets to find consensus results, and v) visualize analysis results and ex- plore significantly impacted pathways across multiple analyses. The package supports the analysis of more than 1,000 species, three differential analysis techniques, eight pathway methods, and two pathway databases (GO and KEGG).
This vignette serves as an introductory guide to RCPA’s essential usage and provides users with a solid understanding of its capabilities. Through practical case studies utilizing gene expression data sourced from NCBI GEO, we demonstrate the practical application of RCPA. By the end, users will have a clearer picture of the available functions, their relevance, and a starting point for seeking assistance as needed.
After installation, users can load the package as follows:
unloadNamespace("RCPA")
library(RCPA)
library(SummarizedExperiment)
library(ggplot2)
library(gridExtra)
RCPA provides the downloadGEO
function for downloading, processAffymetrix
and processAgilent
for processing high-throughput gene expression data from NCBI GEO repository supporting both Affymetrix and Agilent technologies. Users then can save the processed data in a SummarizedExperiment
object. The SummarizedExperiment
object is structured in a way that captures the various dimensions and metadata associated with the data, making it an ideal choice for storing and manipulating complex datasets. The assays
attribute of the resulted object contains gene expression values, and colData
attribute stores sample-level metadata, such as clinical information, and experimental conditions.
In this example, we demonstrate the use of function downloadGEO
for downloading an Affymetrix dataset from GEO database (accession ID: GSE5181). Users can run the following code to get the data:
# User-defined directory to save the downloaded data
downloadPath <- file.path(getwd(), "GSE5281")
# Create the directory if it does not exist
if(!dir.exists(downloadPath)) dir.create(downloadPath)
# download the data
downloadedFiles <- RCPA::downloadGEO(GEOID = "GSE5281", platform = "GPL570", protocol = "affymetrix", destDir = downloadPath)
After executing the code, by running head(downloadedFiles)
command to see the output. The function downloadGEO
returns a list of downloaded files, which is assigned to the downloadedFiles variable. The first element of the list is the metadata file, and the remaining elements are the CEL files.
[1] "metadata.csv" "GSM119615.CEL.gz" "GSM119616.CEL.gz" "GSM119617.CEL.gz"
[5] "GSM119618.CEL.gz" "GSM119619.CEL.gz"
We can then process the downloaded files as follow:
# read the metadata file
affySampleInfo <- read.csv(file.path(downloadPath, "metadata.csv"))
# read the CEL files
affyExprs <- RCPA::processAffymetrix(dir = downloadPath, samples = affySampleInfo$geo_accession)
# create the SummarizedExperiment object
affyDataset <- SummarizedExperiment::SummarizedExperiment(assays = affyExprs, colData = affySampleInfo)
By running head(affyDataset)
command, users can expect to get the below output:
class: SummarizedExperiment
dim: 6 161
metadata(0):
assays(1): ''
rownames(6): 1007_s_at 1053_at ... 1255_g_at 1294_at
rowData names(0):
colnames(161): GSM119615 GSM119616 ... GSM238955 GSM238963
colData names(70): title geo_accession ... sex.ch1 Sex.ch1
We can access to the assay data and the sample data stored in the SummarizedExperiment
object using the functions from SummarizedExperiment namely assay
and colData
:
# Access to assay data
affyExprs <- SummarizedExperiment::assay(affyDataset)
# Access to sample information
affySampleInfo <- SummarizedExperiment::colData(affyDataset)
After executing the above code, by running head(affyExprs, c(5,6))
and head(affySampleInfo, c(3, 10))
commands, users can expect to get the below outputs:
> head(affyExprs, c(5,6))
GSM119615 GSM119616 GSM119617 GSM119618 GSM119619 GSM119620
1007_s_at 3.043234 3.055157 3.144277 3.150378 3.084336 2.989966
1053_at 1.698974 1.645050 1.618537 1.589216 1.676278 1.581733
117_at 1.795751 1.770719 1.805597 1.995794 1.688068 1.961556
121_at 2.553174 2.668456 2.801450 2.784216 2.588638 2.692849
1255_g_at 1.626691 1.940055 1.663162 1.483875 2.354096 1.671216
> head(affySampleInfo, c(3, 10))
DataFrame with 3 rows and 10 columns
title geo_accession status submission_date last_update_date
<character> <character> <character> <character> <character>
GSM119615 EC control 1 GSM119615 Public on Jul 10 2006 Jul 10 2006 Jun 26 2019
GSM119616 EC control 2 GSM119616 Public on Jul 10 2006 Jul 10 2006 Jun 26 2019
GSM119617 EC control 3 GSM119617 Public on Jul 10 2006 Jul 10 2006 Jun 26 2019
type channel_count source_name_ch1 organism_ch1 characteristics_ch1
<character> <character> <character> <character> <character>
GSM119615 RNA 1 brain, Entorhinal Co.. Homo sapiens Sample Amount: 10 ug
GSM119616 RNA 1 brain, Entorhinal Co.. Homo sapiens Sample Amount: 10 ug
GSM119617 RNA 1 brain, Entorhinal Co.. Homo sapiens Sample Amount: 10 ug
In this example, we use the function downloadGEO
to download an Agilent dataset from GEO database (accession ID: GSE61196):
# User-defined directory to save the downloaded data
downloadPath <- file.path(getwd(), "GSE61196")
# Create the directory if it does not exist
if(!dir.exists(downloadPath)) dir.create(downloadPath)
# download the data
downloadedFiles <- RCPA::downloadGEO(GEOID = "GSE61196", platform = "GPL4133", protocol = "agilent", destDir = downloadPath)
In the above code, the function downloadGEO
requires users to specify which color channel should be used when downloading an Agilent dataset. When greenOnly = FALSE
, it tells the function that both red and green channels required. Similarly, we run head(downloadedFiles)
command, and get the below output:
> head(downloadedFiles)
[1] "metadata.csv" "GSM1499379.TXT.gz" "GSM1499380.TXT.gz"
[4] "GSM1499381.TXT.gz" "GSM1499382.TXT.gz" "GSM1499383.TXT.gz"
Next, we process the downloaded files as follows:
# read the metadata file
agilSampleInfo <- read.csv(file.path(downloadPath, "metadata.csv"))
# read the TXT files
agilExprs <- processAgilent(dir = downloadPath, samples = agilSampleInfo$geo_accession, greenOnly = FALSE)
# create the SummarizedExperiment object
agilDataset <- SummarizedExperiment::SummarizedExperiment(assays = agilExprs, colData = agilSampleInfo)
We can then run the print(agilDataset)
to display the SummarizedExperiment
object:
class: SummarizedExperiment
dim: 6 21
metadata(0):
assays(1): ''
rownames(6): GE_BrightCorner DarkCorner ... DarkCorner DarkCorner
rowData names(0):
colnames(21): GSM1499379 GSM1499380 ... GSM1499398 GSM1499399
colData names(48): title geo_accession ... tissue.ch1 tissue.ch2
We can access to the assay data and the sample data stored in agilDataset
variable as follows:
# Access to assay data
agilExprs <- SummarizedExperiment::assay(agilDataset)
# Access to sample information
agilSampleInfo <- SummarizedExperiment::colData(agilDataset)
Next, we run print(agilExprs[9:14, 1:6])
and head(agilSampleInfo, c(3,10))
commands, and get the below outputs:
> print(agilExprs[9:14, 1:6])
GSM1499379 GSM1499380 GSM1499381 GSM1499382 GSM1499383 GSM1499384
DarkCorner 4.663415 5.054929 5.113313 5.295257 5.424192 4.885411
DarkCorner 4.964227 5.219474 4.962025 5.199360 5.141188 5.020854
DarkCorner 4.898062 5.091960 4.909536 4.909536 5.424192 5.000929
A_24_P66027 8.090737 8.141476 8.163278 8.089728 8.128815 8.096007
A_32_P77178 5.329005 5.219474 5.551633 5.803849 5.725941 5.369755
A_23_P212522 11.178282 11.469014 11.354861 11.288909 11.435052 11.290439
> head(agilSampleInfo, c(3, 10))
DataFrame with 3 rows and 10 columns
title geo_accession status submission_date
<character> <character> <character> <character>
GSM1499379 human CPE Braak-0 do.. GSM1499379 Public on Dec 31 2014 Sep 08 2014
GSM1499380 human CPE Braak-0 do.. GSM1499380 Public on Dec 31 2014 Sep 08 2014
GSM1499381 human CPE Braak-0 do.. GSM1499381 Public on Dec 31 2014 Sep 08 2014
last_update_date type channel_count source_name_ch1 organism_ch1
<character> <character> <character> <character> <character>
GSM1499379 Dec 31 2014 RNA 2 healthy human choroi.. Homo sapiens
GSM1499380 Dec 31 2014 RNA 2 healthy human choroi.. Homo sapiens
GSM1499381 Dec 31 2014 RNA 2 healthy human choroi.. Homo sapiens
characteristics_ch1
<character>
GSM1499379 tissue: choroid plex..
GSM1499380 tissue: choroid plex..
GSM1499381 tissue: choroid plex..
One can also download read counts data from GEO and create the SummarizedExperiment object to be used in later stages. Here, we download read counts data for GSE153873 from GEO:
# Specify the GEO accession ID
GEOID <- "GSE153873"
# Create a download path
downloadPath <- getwd()
if(!dir.exists(downloadPath)) dir.create(downloadPath)
# Download the data
GEOquery::getGEOSuppFiles(GEOID, fetch_files = TRUE, baseDir = downloadPath)
Users can check the files in the download path using list.files(downloadPath)
command and get the following result:
> list.files(downloadPath)
[1] "GSE153873"
As we can see, when running the GEOquery::getGEOSuppFiles()
function, it will automatically create a folder named GSE153873 in the user-defined download folder and save all the downloaded data in that folder. We can see the files name in this newly-created folder by running list.files(file.path(downloadPath, GEOID))
and get the following output:
> list.files(file.path(downloadPath, GEOID))
[1] "GSE153873_AD.vs.Old_diff.genes.xlsx" "GSE153873_summary_count.ercc.txt.gz"
[3] "GSE153873_summary_count.star.txt.gz"
Accordingly, the read count is saved under the name ``GSE153873_summary_count.star.txt.gz”. We can extract this file and obtain the assay data by running the following code snippet:
# Specify the path to the downloaded read counts file
countsFile <- file.path(downloadPath, GEOID, "GSE153873_summary_count.star.txt.gz")
# Read the downloaded file
countsData <- read.table(countsFile, header = TRUE, sep = "\t", fill = 0, row.names = 1, check.names = FALSE)
By running head(countsData, c(5,6))
, we can see some pieces of the data obtained, which is a dataframe in which rows are genes and columns are samples as follow:
> head(countsData, c(5,6))
20-1T-AD 13-11T-Old 15-13T-Old 16-14T-Old 3-17T-Young 5-18T-Young
SGIP1 1405 1405 1169 2408 859 1164
NECAP2 295 460 334 347 617 585
AZIN2 356 306 385 507 787 751
AGBL4 191 200 173 323 36 89
CLIC4 876 1443 639 792 4806 5968
In addition to assay data, we also need to download the metadata for the samples. The function to download is getGEO
from the GEOquery package. We have to specify the ID of the dataset that we want.
# Download the GEO object to get metadata
GEOObject <- GEOquery::getGEO(GEOID, GSEMatrix = T, getGPL = T, destdir = downloadPath)
# Check the length of GEOObject
print(length(GEOObject))
# Extract the dataset from the GEOObject
samplesData <- GEOObject[[1]]
# Export sample data
metadata <- Biobase::pData(samplesData)
Some datasets on GEO may be derived from different microarray platforms. Therefore, the object GEOObject
can be a list of different datasets. We can find out how many were used by checking the length of the GEOObject
object. Usually there will only be one platform and the dataset we want to analyse will be the first object in the list (GEOObject[[1]]
). Moreover, data submitted to GEO contain sample labels assigned by the experimenters, and some information about the processing protocol. All these data can be extracted by the Biobase::pData()
function. By running head(metadata, c(5,6))
, users can expect to see the following output:
> head(metadata, c(5,6))
title geo_accession status submission_date last_update_date
GSM4656348 13-11T-Old GSM4656348 Public on Jul 07 2020 Jul 06 2020 Oct 13 2020
GSM4656349 15-13T-Old GSM4656349 Public on Jul 07 2020 Jul 06 2020 Oct 13 2020
GSM4656350 20-1T-AD GSM4656350 Public on Jul 07 2020 Jul 06 2020 Oct 13 2020
GSM4656351 16-14T-Old GSM4656351 Public on Jul 07 2020 Jul 06 2020 Oct 13 2020
GSM4656352 3-17T-Young GSM4656352 Public on Jul 07 2020 Jul 06 2020 Oct 13 2020
type
GSM4656348 SRA
GSM4656349 SRA
GSM4656350 SRA
GSM4656351 SRA
GSM4656352 SRA
As we can see, title column of metadata contains the value of the columns labels of countsData. To be consistent with other examples in which the sample IDs are in the standard GEO accession ID form (i.e., GSMxxxx), we will update the columns label of count data as follows:
# Get the sample IDs in the GEO accession ID form
sampleIDs <- rownames(metadata)
# Get the sample titles
sampleTitles <- metadata[, "title"]
# Reorder the columns in the assay data
countsData <- countsData[,sampleTitles]
# Assign sample IDs to columns' labels
colnames(countsData) <- sampleIDs
By running head(countsData, c(5,6))
, the new countsData
is as follows:
> head(countsData, c(5,6))
GSM4656348 GSM4656349 GSM4656350 GSM4656351 GSM4656352 GSM4656353
SGIP1 1405 1169 1405 2408 859 1164
NECAP2 460 334 295 347 617 585
AZIN2 306 385 356 507 787 751
AGBL4 200 173 191 323 36 89
CLIC4 1443 639 876 792 4806 5968
Finally, we can create the SummarizedExperiment
to stored the assay and sample data as follows:
# Create the SummarizedExperiment object
RNASeqDataset <- SummarizedExperiment::SummarizedExperiment(
assays = as.matrix(countsData),
colData = metadata
)
The summary of created RNASeq object after running head(RNASeqDataset)
command can be explored, as:
class: SummarizedExperiment
dim: 6 30
metadata(0):
assays(1): ''
rownames(6): SGIP1 NECAP2 ... CLIC4 SLC45A1
rowData names(0):
colnames(30): GSM4656348 GSM4656349 ... GSM4656376 GSM4656377
colData names(38): title geo_accession ... disease state:ch1 tissue:ch1
Additionally, users can create their own SummarizedExperiment
object from their customized data with the same procedure.
To begin with differential analysis (DE analysis), we can call runDEAnalysis function. This function utilizes one of the limma, DESeq2, and edgeR methods to perform the analysis. It is generally recommended to use limma for differential expression analysis of microarray data, or log-scaled RNA-seq data with TPM, FPKM, or RPKM normalization values. For RNA-seq data with raw counts, DESeq2 or edgeR are recommended.
There are two important arguments in the function: design and contrast. The design matrix defines the statistical model to be fitted in the analysis. The contrast matrix defines the comparisons to be performed in the analysis.
To start, first, we add additional sample information to each of the SummarizedExperiment objects obtained from Stage 1. This completely depends on the experimental design and needs to be specified based on research question. This information is used to define the design matrix for differential expression analysis. For GSE5281 dataset, the samples have two conditions: normal and Alzheimer’s, which are defined in the characteristics_ch1.8 column. Each sample is also associated with a brain region, which is defined in the characteristics_ch1.4 column.
# GSE5281
# Add a column specifying the condition of the sample, which can be either normal or alzheimer
affySampleInfo$condition <- ifelse(grepl("normal", affySampleInfo$characteristics_ch1.8), "normal", "alzheimer")
# Factorize the newly added column
affySampleInfo$condition <- factor(affySampleInfo$condition)
# Add the new column specify the region of the sample tissue
# and use make.names to remove special characters
affySampleInfo$region <- make.names(affySampleInfo$characteristics_ch1.4)
# Factorize the newly added column
affySampleInfo$region <- factor(affySampleInfo$region)
# Update the affyDataset object
SummarizedExperiment::colData(affyDataset) <- affySampleInfo
We can check whether the two new columns are added and saved in the affyDataset
object by running the head(affyDataset)
command line again:
class: SummarizedExperiment
dim: 6 161
metadata(0):
assays(1): ''
rownames(6): 1007_s_at 1053_at ... 1255_g_at 1294_at
rowData names(0):
colnames(161): GSM119615 GSM119616 ... GSM238955 GSM238963
colData names(72): title geo_accession ... condition region
As we can see, these two columns condition and region are added. Next, we will create the design and contrast matrices for DE analysis.
# GSE5281
# Create a design matrix
affyDesign <- model.matrix(~0 + condition + region + condition:region, data = SummarizedExperiment::colData(affyDataset))
# Avoid special characters in column names
colnames(affyDesign) <- make.names(colnames(affyDesign))
# Create a constrast matrix
affyContrast <- limma::makeContrasts(conditionalzheimer-conditionnormal, levels=affyDesign)
Here, the formula ~0 + condition + region + condition:region defines the design matrix to include the main effects of condition and region, as well as the interaction between condition and region. The term ~0 indicates that the intercept should not be included in the design matrix since the intercept is not of interest in the analysis. For more information on how to define the design matrix for different scenarios and interests, please refer to the limma user guide. Next, we make use of the limma::makeContrasts function to define the contrast matrix. The formula conditionalzheimer-conditionnormal defines the contrast matrix to compare the alzheimer condition versus the normal condition.
An example of design matrix and contrast matrix is as follow:
> print(affyDesign[1:5, 1:3])
conditionalzheimer conditionnormal regionorgan.region..hippocampus.
GSM119615 0 1 0
GSM119616 0 1 0
GSM119617 0 1 0
GSM119618 0 1 0
GSM119619 0 1 0
Contrasts
Levels conditionalzheimer - conditionnormal
conditionalzheimer 1
conditionnormal -1
regionorgan.region..hippocampus. 0
regionorgan.region..medial.temporal.gyrus. 0
regionorgan.region..posterior.cingulate. 0
regionorgan.region..posterior.singulate. 0
Given the design matrix and contrast matrix, we can perform the differential analysis using limma for Affymetrix dataset as follow:
# Run differential expression analysis
affyDEExperiment <- RCPA::runDEAnalysis(affyDataset, method = "limma", design = affyDesign, contrast = affyContrast, annotation = "GPL570")
We can check this variable by running affyDEExperiment
in the console:
> affyDEExperiment
class: SummarizedExperiment
dim: 21367 161
metadata(4): DEAnalysis.method DEAnalysis.design DEAnalysis.contrast DEAnalysis.mapping
assays(1): counts
rownames(21367): 55101 92840 ... 9695 83887
rowData names(9): PROBEID ID ... sampleSize pFDR
colnames(161): GSM119615 GSM119616 ... GSM238955 GSM238963
colData names(72): title geo_accession ... condition region
The function runDEAnalysis() outputs a SummarizedExperiment object, and this new object extends the input SummarizedExperiment object to include the results of the differential analysis. In essence, the resulting object not only retains the expression data matrix and sample information but also incorporates the differential expression analysis results, which are stored under rowData attribute. As we can see in the R console, the new attribute rowData is added into the SummarizedExperiment object. Similar to the data stored under other attributes, this data can also be accessed using the function rowData() from the SummarizedExperiment package, as follows:
# Extract the differential analysis result
affyDEResults <- SummarizedExperiment::rowData(affyDEExperiment)
Users can display the result in R console by running head(affyDEResults, c(3,5))
:
> head(affyDEResults, c(3,5))
DataFrame with 3 rows and 5 columns
PROBEID ID p.value statistic logFC
<character> <character> <numeric> <numeric> <numeric>
55101 45828_at 55101 1.53869e-23 -11.8894 -0.465108
92840 226597_at 92840 3.56762e-23 -11.7546 -0.661995
727957 227778_at 727957 3.55473e-22 -11.3858 -0.525213
For GSE61196 dataset, the samples have two conditions: normal and Alzheimer’s, which are defined in the source_name_ch1 column.
# GSE61196
colData(agilDataset)$condition <- ifelse(grepl("healthy", colData(agilDataset)$source_name_ch1), "normal", "alzheimer")
colData(agilDataset)$condition <- factor(colData(agilDataset)$condition)
Next, we define the design matrix and contrast matrix for differential expression analysis. For this dataset, we define the design matrix to include the condition, and similarly, the contrast matrix to compare the alzheimer condition versus the normal condition.
# GSE61196
agilDesign <- model.matrix(~0 + condition, data = colData(agilDataset))
agilContrast <- limma::makeContrasts("conditionalzheimer-conditionnormal", levels=agilDesign)
As an example of expected output, here we show a part of constructed design and contrast matrices for GSE61196:
head(agilDesign)
conditionalzheimer conditionnormal
GSM1499379 0 1
GSM1499380 0 1
GSM1499381 0 1
GSM1499382 0 1
GSM1499383 0 1
GSM1499384 0 1
head(agilContrast)
Contrasts
Levels conditionalzheimer-conditionnormal
conditionalzheimer 1
conditionnormal -1
Next, we define the mapping between the ID of the assay in the SummarizedExperiment object and Entrez ID. The annotation argument can accept a supported GEO platform ID or a data frame with two columns: FROM and TO. If a GEO platform ID is provided, the function will automatically download the available annotation from Bioconductor. Users can use the function RCPA::getSupportedPlatforms() to get the list of supported GEO platform IDs. For GSE61196, since the platform GPL4133 is not supported by Bioconductor, we need to manually download the annotation from GEO as follows.
# GSE61196
GPL4133Anno <- GEOquery::dataTable(GEOquery::getGEO("GPL4133"))@table
GPL4133GeneMapping <- data.frame(FROM = GPL4133Anno$SPOT_ID, TO = as.character(GPL4133Anno$GENE), stringsAsFactors = F)
GPL4133GeneMapping <- GPL4133GeneMapping[!is.na(GPL4133GeneMapping$TO), ]
The mapping output is a dataframe as:
head(GPL4133GeneMapping)
FROM TO
A_24_P66027 9582
A_23_P212522 23200
A_24_P934473 100132006
A_24_P9671 3301
A_24_P801451 10919
A_32_P30710 9349
Finally, we perform differential expression analysis using the runDEAnalysis function. We still use limma for differential expression analysis since the data are from microarray experiments.
# GSE61196
agilDEExperiment <- RCPA::runDEAnalysis(agilDataset, method = "limma", design = agilDesign, contrast = agilContrast, annotation = GPL4133GeneMapping)
For GSE153873, the samples have two conditions: normal and Alzheimer’s, which are defined in the characteristics_ch1.1 column.
# GSE153873
colData(RNASeqDataset)$condition <- ifelse(grepl("Alzheimer", colData(RNASeqDataset)$characteristics_ch1.1), "alzheimer", "normal")
Next, we define the design matrix and contrast matrix for differential expression analysis. For GSE153873 dataset, we define the design matrix to include the condition, and similarly, the contrast matrix to compare the alzheimer condition versus the normal condition.
# GSE61196
agilDesign <- model.matrix(~0 + condition, data = colData(agilDataset))
agilContrast <- limma::makeContrasts("conditionalzheimer-conditionnormal", levels=agilDesign)
# GSE153873
RNASeqDesign <- model.matrix(~0 + condition, data = colData(RNASeqDataset))
RNASeqContrast <- limma::makeContrasts("conditionalzheimer-conditionnormal", levels=RNASeqDesign)
For GSE153873, the IDs are Gene SYMBOL, we can use the org.Hs.eg.db package to map Human Gene SYMBOL to Entrez ID as follows:
# GSE153873
if (!require("org.Hs.eg.db", quietly = TRUE)) {
BiocManager::install("org.Hs.eg.db")
}
library(org.Hs.eg.db)
ENSEMBLMapping <- AnnotationDbi::select(org.Hs.eg.db, keys = rownames(RNASeqDataset), columns = c("SYMBOL", "ENTREZID"), keytype = "SYMBOL")
colnames(ENSEMBLMapping) <- c("FROM", "TO")
The first rows of generated mapping dataframe are as:
head(ENSEMBLMapping)
FROM TO
SGIP1 84251
NECAP2 55707
AZIN2 113451
AGBL4 84871
CLIC4 25932
SLC45A1 50651
Finally, we perform differential expression analysis using the runDEAnalysis function. For GSE153873 dataset, we use DESeq2 for differential expression analysis since the data are counts data from RNA-Seq experiments.
# GSE153873
RNASeqDEExperiment <- RCPA::runDEAnalysis(RNASeqDataset, method = "DESeq2", design = RNASeqDesign, contrast = RNASeqContrast, annotation = ENSEMBLMapping)
User can also use edgeR for GSE153873 dataset by setting the method argument to edgeR:
# GSE153873
RNASeqDEExperiment <- RCPA::runDEAnalysis(RNASeqDataset, method = "edgeR", design = RNASeqDesign, contrast = RNASeqContrast, annotation = ENSEMBLMapping)
It is important to examine the differential analysis results before further analysis. This will help to identify potential issues in the analysis as well as to determine the suitable downstream analysis methods and parameters. Two common approaches are MA plot and volcano plot.
We have implemented three functions, plotMA, plotVolcano, and plotVennDE. Each of the mentioned functions returns a ggplot object that can be further customized using the ggplot2 package.
The code below shows how to generate the MA plots for three datasets:
# MA plots
p1 <- RCPA::plotMA(rowData(affyDEExperiment), logFCThreshold = 0.5) + ggplot2::ggtitle("Affymetrix - GSE5281")
p2 <- RCPA::plotMA(rowData(agilDEExperiment), logFCThreshold = 0.5) + ggplot2::ggtitle("Agilent - GSE61196")
p3 <- RCPA::plotMA(rowData(RNASeqDEExperiment), logFCThreshold = 0.5) + ggplot2::ggtitle("RNASeq - GSE153873")
gridExtra::grid.arrange(p1, p2, p3, ncol = 3)
A normal MA plot will have most of the points centered around the zero log fold change line, If all points are shifted up or down, it indicates a systematic bias in the data that needs to be corrected. The obtained plots are:
Similarly, we can have volcano plot for the three datasets, as well:
# Volcano plots
p1 <- RCPA::plotVolcanoDE(rowData(affyDEExperiment), logFCThreshold = 0.5) + ggplot2::ggtitle("Affymetrix - GSE5281")
p2 <- RCPA::plotVolcanoDE(rowData(agilDEExperiment), logFCThreshold = 0.5) + ggplot2::ggtitle("Agilent - GSE61196")
p3 <- RCPA::plotVolcanoDE(rowData(RNASeqDEExperiment), logFCThreshold = 0.5) + ggplot2::ggtitle("RNASeq - GSE153873")
gridExtra::grid.arrange(p1, p2, p3, ncol = 3)
A normal volcano plot will have points that are relatively symmetrical around the y-axis of zero log fold change. The generated plots are:
It is also important to check the intersection of DE genes between different datasets. This will help to identify potential issues in the analysis design. To this aim, we can use the function plotVennDE to generate the Venn diagram of DE genes among datasets as follows:
# All DE genes
DEResults <- list(
"Affymetrix - GSE5281" = rowData(affyDEExperiment),
"Agilent - GSE61196" = rowData(agilDEExperiment),
"RNASeq - GSE153873" = rowData(RNASeqDEExperiment)
)
# Up-regulated genes
DEResultUps <- lapply(DEResults, function(df) df[!is.na(df$logFC) & df$logFC > 0,])
# Down-regulated genes
DEResultDowns <- lapply(DEResults, function(df) df[!is.na(df$logFC) & df$logFC < 0,])
p1 <- RCPA::plotVennDE(DEResults) + ggplot2::ggtitle("All DE Genes")
p2 <- RCPA::plotVennDE(DEResultUps) + ggplot2::ggtitle("Up-regulated DE Genes")
p3 <- RCPA::plotVennDE(DEResultDowns) + ggplot2::ggtitle("Down-regulated DE Genes")
gridExtra::grid.arrange(p1, p2, p3, ncol = 3)
and the generated Venn diagrams are:
In this pipeline, we have implemented eight widely used and reliable approaches for pathway analysis, which assist users in identifying significantly enriched functional categories. We categorize these approaches into two subgroups: non-topology-based and topology-based pathway analysis tools.
The included geneset enrichment analysis methods in RCPA package are ORA, FGSEA, GSA, KS (Kolmogorov–Smirnov), and Wilcox tests, which do not account for gene interactions within a pathway.
To start with this analysis, beside the SummarizedExperiment object generated by differential analysis, users need to prepare genesets information beforehand. In this protocol, we have implemented getGeneSets function to retrieve gene sets from two databases, including KEGG and GO, for a given organism. The below code retrieves genesets definitions from KEGG for human organism:
genesets <- RCPA::getGeneSets(database = "KEGG", org = "hsa")
The returned object is a named list of length three, including, genesets definitions, names of genesets, and the size of genesets.
If users wish to use their own genesets in the analysis, they can prepare a geneset object with the same format as the returned object from getGeneSets function. We recommend using Entreze gene IDs as the gene identifiers in the genesets object, as we provided helper functions to retrieve the gene symbols and descriptions from the NCBI database, which will be used in the downstream analysis and visualization.
After preparing the genesets object, users can proceed to the enrichment analysis. The analysis can be initiated by calling the runGeneSetAnalysis function, which will execute the gene set analysis procedure based on the selected method.
To run the function with fgsea as method, for three datasets, the code is:
#The list of additional arguments passed to fgsea function
fgseaArgsList <- list(minSize = 10, maxSize = Inf)
#Geneset enrichment analysis
affyFgseaResult <- runGeneSetAnalysis(affyDEExperiment, genesets,
method = "fgsea", FgseaArgs = fgseaArgsList)
agilFgseaResult <- runGeneSetAnalysis(agilDEExperiment, genesets,
method = "fgsea", FgseaArgs = fgseaArgsList)
RNASeqFgseaResult <- runGeneSetAnalysis(RNASeqDEExperiment, genesets,
method = "fgsea", FgseaArgs = fgseaArgsList)
For ORA and affyDEExperiment object, we can use:
affyORAResult <- runGeneSetAnalysis(affyDEExperiment, genesets,
method = "ora", ORAArgs = list(pThreshold = 0.05))
For GSA and affyDEExperiment object, we can use:
affyGSAResult <- runGeneSetAnalysis(affyDEExperiment, genesets, method = "gsa")
For KS test and affyDEExperiment object, we can use:
affyKSResult <- runGeneSetAnalysis(affyDEExperiment, genesets, method = "ks")
For Wilcox test and affyDEExperiment object, we can use:
affyKSResult <- runGeneSetAnalysis(affyDEExperiment, genesets, method = "wilcox")
The output of the runGeneSetAnalysis function is a dataframe containing the results of the enrichment analysis. We can see a part of the output after running the function using fgsea method for affyDEExperiment:
> head(RNASeqFgseaResult)
ID p.value score normalizedScore sampleSize name
1 path:hsa05014 1.69e-35 -0.584 -2.78 30 Amyotrophic lateral sclerosis
2 path:hsa05016 9.76e-33 -0.597 -2.78 30 Huntington disease
3 path:hsa05012 2.84e-29 -0.607 -2.78 30 Parkinson disease
4 path:hsa05020 9.29e-29 -0.598 -2.74 30 Prion disease
5 path:hsa00190 8.11e-28 -0.743 -3.07 30 Oxidative phosphorylation
6 path:hsa05022 3.86e-25 -0.487 -2.37 30 Pathways of neurodegeneration - multiple diseases
pFDR pathwaySize
1 5.73e-33 364
2 1.65e-30 306
3 3.21e-27 266
4 7.87e-27 272
5 5.50e-26 134
6 2.18e-23 476
The methods for pathway enrichment analysis in RCPA are SPIA, CePa ORA, and CePa GSA, which consider the topology and interconnections between genes within a pathway. We have implemented the runPathwayAnalysis function to perform pathway enrichment analysis using one of the mentioned methods.
For each of these methods, we need to pass a network object which contains the pathways network information from the KEGG database. To elaborate, the getSPIAKEGGNetwork function generates the necessary network for SPIA, while the getCePaPathwayCatalogue function produces the pathway catalog object required by both CePa ORA and CePa GSA.
We start with the process of running SPIA. First, we call the getSPIAKEGGNetwork to get network for human organism:
spiaNetwork <- RCPA::getSPIAKEGGNetwork(org = "hsa", updateCache = FALSE)
The generated network object is a list of length three which are network definitions of pathways, names of patwhays, and the size of pathways.
Now, we can call runPathwayAnalysis function:
affySpiaResult <- runPathwayAnalysis(affyDEExperiment, spiaNetwork, method = "spia")
agilSpiaResult <- runPathwayAnalysis(agilDEExperiment, spiaNetwork, method = "spia")
RNASeqSpiaResult <- runPathwayAnalysis(RNASeqDEExperiment, spiaNetwork, method = "spia")
To run any of the CePa ORA, or CePa GSA, we need first get the pathway network using getCePaPathwayCatalogue function, as:
cepaNetwork <- RCPA::getCePaPathwayCatalogue(org = "hsa", updateCache = FALSE)
Similar to getSPIAKEGGNetwork, the generated network catalogue is a list of length three with the same structure.
Then, we can utilize the generated network to call runPathwayAnalysis function. To call the function using affyDEExperiment object and with CePa ORA as method:
affyCepaORAResult <- runPathwayAnalysis(affyDEExperiment, cepaNetwork, method = "cepaORA")
and similarly, to call function using affyDEExperiment object and with CePa GSA as method:
affyCepaGSAResult <- runPathwayAnalysis(affyDEExperiment, cepaNetwork, method = "cepaGSA")
The runPathwayAnalysis function returns a dataframe the same as the output of the runGeneSetAnalysis function. Below, the top rows of obtained results using SPIA and affyDEExperiment object is shown:
> head(RNASeqSpiaResult)
ID p.value score normalizedScore sampleSize
1 path:hsa05016 1.836417e-28 33.48486 -1.3614702 30
2 path:hsa05014 8.015966e-27 68.44187 -1.0164137 30
3 path:hsa05020 1.771357e-24 43.61561 -1.0511215 30
4 path:hsa00190 2.024686e-24 46.89983 4.7167369 30
5 path:hsa05022 3.590430e-23 213.46961 0.7301322 30
6 path:hsa05010 5.217307e-23 130.11774 -0.5420581 30
name pFDR pathwaySize
1 Huntington disease 5.215424e-26 306
2 Amyotrophic lateral sclerosis 1.138267e-24 364
3 Prion disease 1.437527e-22 272
4 Oxidative phosphorylation 1.437527e-22 134
5 Pathways of neurodegeneration - multiple diseases 2.039364e-21 476
6 Alzheimer disease 2.469525e-21 384
For gene-level meta-analysis, RCPA provides the function named runDEMetaAnalysis to perform meta-analysis using DE analysis results. Users can pick one of the fisher, stouffer, addCLT, geoMean, and minP methods to perform meta-analysis. Besides the p-values, the fold-changes also are combined using SMD method. In the following code, we call this function utilizing three obtained DE results from stage 2:
#Preparing the input list of DE results
DEResults <- list(
"Affymetrix - GSE5281" = rowData(affyDEExperiment),
"Agilent - GSE61196" = rowData(agilDEExperiment),
"RNASeq - GSE153873" = rowData(RNASeqDEExperiment)
)
#Calling the runDEMetaAnalysis with 'stouffer' as the selected method to combine PValues
metaDEResult <- RCPA::runDEMetaAnalysis(DEResults, method = "stouffer")
The output is a dataframe containing combined p-value, pFDR, log fold change, and log fold change standard error. In the below table, we show six top rows of the generated dataframe:
> head(metaDEResult)
ID p.value pFDR logFC logFCSE
1 84964 1.541734e-19 2.585333e-15 -0.4693914 0.04721164
2 10106 6.840827e-16 4.219658e-12 0.3273123 0.03915734
3 7108 8.988938e-16 4.219658e-12 -0.3681265 0.04798479
4 4713 1.006538e-15 4.219658e-12 -0.5306827 0.06044290
5 10382 1.766204e-15 5.923497e-12 -0.6648832 0.07334485
6 396 2.202702e-15 6.156186e-12 -0.3427080 0.03925764
Users can perform meta-analysis of pathway analysis results, using the runPathwayMetaAnalysis function. sers can pick one of the fisher, stouffer, addCLT, geoMean, and minP methods to perform meta-analysis. Besides the p-values, the scores also are combined using SMD method. In the following code, we call this function utilizing three obtained enrichment analysis results of the FGSEA method in stage 3 to conduct meta-analysis based on Stouffer’s method:
#Preparing the input list of enrichment results
PAResults <- list(
"Affymetrix - GSE5281" = affyFgseaResult,
"Agilent - GSE61196" = agilFgseaResult,
"RNASeq - GSE153873" = RNASeqFgseaResult
)
#Calling the runPathwayMetaAnalysis with 'stouffer' as the selected method to combine PValues
metaPAResult <- RCPA::runPathwayMetaAnalysis(PAResults, method = "stouffer")
The output of meta-analysis is a dataframe containing combined p-value, score, and normalized score. In the below table, we show six top rows of the obtained results after performing meta-analysis:
ID name p.value pFDR score
1 path:hsa05012 Parkinson disease 7.123092e-46 2.393359e-43 -2.467830
2 path:hsa05016 Huntington disease 3.763897e-44 6.323347e-42 -2.430244
3 path:hsa05014 Amyotrophic lateral sclerosis 9.552510e-44 1.069881e-41 -2.393301
4 path:hsa00190 Oxidative phosphorylation 6.473335e-40 5.437601e-38 -2.691299
5 path:hsa05020 Prion disease 1.291475e-37 8.678712e-36 -2.402497
6 path:hsa05022 Pathways of neurodegeneration - multiple diseases 9.036272e-34 5.060312e-32 -2.119561
normalizedScore pathwaySize
1 -2.467830 266
2 -2.430244 306
3 -2.393301 364
4 -2.691299 134
5 -2.402497 272
6 -2.119561 476
To start with consensus analysis, users can call the runConsensusAnalysis function with either weightedZMean or RRA to conduct consensus analysis. In the following code, we call runConsensusAnalysis to perform consensus analysis based on weightedZMean utilizing two obtained enrichment analysis results for Affymetrix-GSE5281 dataset by FGSEA, and SPIA methods:
PAResults <- list(
"fgsea" = affyFgseaResult,
"spia" = affySpiaResult
)
consensusPAResult <- RCPA::runConsensusAnalysis(PAResults, method = "weightedZMean")
The output of runConsensusAnalysis function, is a dataframe containing combined p-value, and pFDR. In the below table, we show six top rows of the generated dataframe:
> head(consensusPAResult)
ID p.value name pathwaySize pFDR
1 path:hsa05022 8.213205e-09 Pathways of neurodegeneration - multiple diseases 476 8.213205e-09
2 path:hsa05014 7.783738e-07 Amyotrophic lateral sclerosis 364 7.783738e-07
3 path:hsa05016 1.933887e-06 Huntington disease 306 1.933887e-06
4 path:hsa05020 3.727841e-06 Prion disease 272 3.727841e-06
5 path:hsa04723 7.422680e-06 Retrograde endocannabinoid signaling 148 7.422680e-06
6 path:hsa00190 7.736429e-06 Oxidative phosphorylation 134 7.736429e-06
In this section, we demonstrate how to visualize the results of the pathway analysis and integrative analysis. RCPA includes several state-of-the-art plots, which can be used to visualize and interpret results more efficiently. It is notable that since consensus analysis results do not report any score, the results can be visualized using plotting functions in RCPA that employ the p-value or pFDR.
We can plot the Venn diagram for enrichment analysis results using plotVennPathway function. The below code generates three Venn diagrams of all significant pathways, significant up-regulated pathways, and significant down-regulated pathways utilizing results obtained by fgsea method. The definition of up/down regulation depends on the method which we are using to analyze data.
PAResults <- list(
"Affymetrix - GSE5281" = affyFgseaResult,
"Agilent - GSE61196" = agilFgseaResult,
"RNASeq - GSE153873" = RNASeqFgseaResult,
"Meta-analysis" = metaPAResult
)
PAREsultUps <- lapply(PAResults, function(df) df[df$normalizedScore > 0,])
PAREsultDowns <- lapply(PAResults, function(df) df[df$normalizedScore < 0,])
p1 <- RCPA::plotVennPathway(PAResults, pThreshold = 0.05) + ggplot2::ggtitle("All Significant Pathways")
p2 <- RCPA::plotVennPathway(PAREsultUps, pThreshold = 0.05) + ggplot2::ggtitle("Significantly Up-regulated Pathways")
p3 <- RCPA::plotVennPathway(PAREsultDowns, pThreshold = 0.05) + ggplot2::ggtitle("Significantly Down-regulated Pathways")
gridExtra::grid.arrange(p1, p2, p3, ncol = 3)
The generated Venn diagram is as:
Using the volcano plot, we can have a quick overview of the results of the enrichment analysis, as well as the general trend of the pathway regulation for each dataset. The following code use the plotVolcanoPathway function from RCPA to plot four volcano plots, including 3 plots for the analysis of the 3 datasets and one for the meta-analysis, all using the FGSEA method.
p1 <- RCPA::plotVolcanoPathway(affyFgseaResult, sideToLabel = "left") + ggtitle("Affymetrix - GSE5281")
p2 <- RCPA::plotVolcanoPathway(agilFgseaResult, sideToLabel = "left") + ggtitle("Agilent - GSE61196")
p3 <- RCPA::plotVolcanoPathway(RNASeqFgseaResult, sideToLabel = "left") + ggtitle("RNASeq - GSE153873")
p4 <- RCPA::plotVolcanoPathway(metaPAResult, sideToLabel = "left") + ggtitle("Meta-analysis")
gridExtra::grid.arrange(p1, p2, p3, p4, ncol = 4)
The generated volcano plot is as:
To plot the bar chart, users can use the plotBarChart function. In the following code, we plot the bar chart for the analysis of the FGSEA method using the 3 datasets along with the meta-analysis result. To limit the number of pathways to plot, we only plot the 17 pathways belonging to the categories Neurodegenerative disease and Nervous system of KEGG pathways.
selectedPathways <- c("path:hsa05010", "path:hsa05012", "path:hsa05014", "path:hsa05016", "path:hsa05017", "path:hsa05020", "path:hsa05022", "path:hsa04724", "path:hsa04727", "path:hsa04725", "path:hsa04728", "path:hsa04726", "path:hsa04720", "path:hsa04730", "path:hsa04723", "path:hsa04721", "path:hsa04722")
resultsToPlot <- lapply(PAResults, function(df) df[df$ID %in% selectedPathways,])
RCPA::plotBarChart(resultsToPlot) + ggplot2::ggtitle("FGSEA Analysis Results")
The generated bar plot is as:
The forest plot displays the enrichment score along with their confidence interval as individual points along a horizontal line. When multiple datasets are analyzed, datasets are appended along the x-axis. The following code generates a forest plot using plotForest function, displaying the FGSEA analysis results for two categories Neurodegenerative disease and Nervous system of KEGG pathways on the selected three datasets:
RCPA::plotForest(resultsToPlot, yAxis = "name", statLims = c(-3.5, 3.5))
The generated forest plot is as:
The pathway heatmap shows three pieces of information for each pathway within each input study. These information are: (i) the magnitude of the enrichment score, (ii) the regulation direction, and (iii) the significance of the enrichment score. In RCPA this plot can be generated using plotPathwayHeatmap function. The following code generates a pathway heatmap for KEGG pathways from two categories, Neurodegenerative disease and Nervous system, using the resutls from the FGSEA method on the selected three datasets.
RCPA::plotPathwayHeatmap(resultsToPlot, yAxis = "name")
The generated heatmap for pathways is as:
The gene heatmap shows log fold changes of the genes in the pathway along with their significance across different datasets. The following code plots the gene heatmap using plotDEGeneHeatmap in RCPA for top 50 genes in Alzheimer’s disease pathway that are differentially expressed in meta-analysis.
alzheimerGenes <- genesets$genesets[["path:hsa05010"]]
genesToPlot <- head(metaDEResult[metaDEResult$ID %in% alzheimerGenes, ], 50)$ID
genesAnnotation <- RCPA::getEntrezAnnotation(genesToPlot)
labels <- genesAnnotation[genesToPlot, "Description"]
genesOrderByFC <- order(metaDEResult[match(genesToPlot, metaDEResult$ID), "logFC"])
resultsToPlot <- c(DEResults, list(metaDEResult))
names(resultsToPlot) <- c(names(DEResults), "Meta-analysis")
RCPA::plotDEGeneHeatmap(resultsToPlot, genesToPlot[genesOrderByFC],
labels = labels[genesOrderByFC], negLog10pValueLims = c(0, 5), logFCLims = c(-1, 1)
)
The generated heatmap for genes is as:
The KEGG pathway map shows the expression changes of the genes in the pathway on the KEGG pathway map. The following code plots the KEGG pathway map for Alzheimer’s disease pathway by calling plotKEGGMap function implemented in RCPA.
pltObj <- RCPA::plotKEGGMap(DEResults, "hsa05010", stat = "logFC", pThreshold = 1, statLimit = 1)
pltObj$plot
The generated KEGG map for the selected pathway is as:
The pathway network shows each pathway as a node and the relationship (e.g., common genes) among the pathways as edges. This plot is useful for understanding the relationships among the pathways and identifying the modules of related pathways that are impacted together. In the below code, we use the plotPathwayNetwork to generate the network plot of top 30 significantly enriched pathways in the meta-analysis result obtained in stage 4.
genesetsToPlot <- metaPAResult$ID[order(metaPAResult$pFDR)][1:30]
pltHtml <- RCPA::plotPathwayNetwork(
PAResults,
genesets = genesets,
selectedPathways = genesetsToPlot,
edgeThreshold = 0.75,
mode = "continuous",
statistic = "normalizedScore"
)
The generated pathway network for the selected set of pathways is as:
R version 4.3.1 (2023-06-16)
Platform: aarch64-apple-darwin23.0.0 (64-bit)
Running under: macOS Sonoma 14.0
Matrix products: default
BLAS: /System/Library/Frameworks/Accelerate.framework/Versions/A/Frameworks/vecLib.framework/Versions/A/libBLAS.dylib
LAPACK: /opt/homebrew/Cellar/r/4.3.1/lib/R/lib/libRlapack.dylib; LAPACK version 3.11.0
locale:
[1] en_US.UTF-8/en_US.UTF-8/en_US.UTF-8/C/en_US.UTF-8/en_US.UTF-8
time zone: America/Chicago
tzcode source: internal
attached base packages:
[1] grid stats4 stats graphics grDevices utils datasets methods base
other attached packages:
[1] RCPA_0.2.1 tidyr_1.3.0 RCyjs_2.24.0
[4] BrowserViz_2.24.0 httpuv_1.6.12 jsonlite_1.8.7
[7] RCurl_1.98-1.12 png_0.1-8 XML_3.99-0.15
[10] gridExtra_2.3 ggvenn_0.1.10 dplyr_1.1.3
[13] ggplot2_3.4.4 meta_6.5-0 hgu133plus2.db_3.13.0
[16] ROntoTools_2.30.0 Rgraphviz_2.46.0 KEGGgraph_1.62.0
[19] KEGGREST_1.42.0 boot_1.3-28.1 graph_1.80.0
[22] GSA_1.03.2 fgsea_1.28.0 DESeq2_1.42.0
[25] GenomicRanges_1.54.1 org.Hs.eg.db_3.18.0 AnnotationDbi_1.64.0
[28] IRanges_2.36.0 Biobase_2.62.0 BiocGenerics_0.48.0
[31] SummarizedExperiment_1.32.0 S4Vectors_0.40.1
loaded via a namespace (and not attached):
[1] mathjaxr_1.6-0 rstudioapi_0.15.0 magrittr_2.0.3 rmarkdown_2.25
[5] farver_2.1.1 nloptr_2.0.3 zlibbioc_1.48.0 vctrs_0.6.4
[9] gridpattern_1.1.1 memoise_2.0.1 minqa_1.2.6 base64enc_0.1-3
[13] CompQuadForm_1.4.3 htmltools_0.5.6.1 S4Arrays_1.2.0 curl_5.1.0
[17] SparseArray_1.2.0 KernSmooth_2.23-22 cachem_1.0.8 lifecycle_1.0.3
[21] pkgconfig_2.0.3 Matrix_1.6-1.1 R6_2.5.1 fastmap_1.1.1
[25] GenomeInfoDbData_1.2.11 RobustRankAggreg_1.2.1 MatrixGenerics_1.14.0 digest_0.6.33
[29] numDeriv_2016.8-1.1 colorspace_2.1-0 ggnewscale_0.4.9 RSQLite_2.3.2
[33] labeling_0.4.3 metadat_1.2-0 fansi_1.0.5 httr_1.4.7
[37] abind_1.4-5 compiler_4.3.1 proxy_0.4-27 bit64_4.0.5
[41] withr_2.5.2 metafor_4.4-0 BiocParallel_1.36.0 DBI_1.1.3
[45] R.utils_2.12.2 MASS_7.3-60 DelayedArray_0.28.0 classInt_0.4-10
[49] units_0.8-4 tools_4.3.1 R.oo_1.25.0 glue_1.6.2
[53] promises_1.2.1 nlme_3.1-163 sf_1.0-14 generics_0.1.3
[57] gtable_0.3.4 ggpattern_1.0.1 tzdb_0.4.0 class_7.3-22
[61] R.methodsS3_1.8.2 data.table_1.14.8 hms_1.1.3 xml2_1.3.5
[65] utf8_1.2.4 XVector_0.42.0 ggrepel_0.9.4 pillar_1.9.0
[69] stringr_1.5.0 limma_3.58.0 later_1.3.1 splines_4.3.1
[73] lattice_0.22-5 bit_4.0.5 GEOquery_2.70.0 tidyselect_1.2.0
[77] locfit_1.5-9.8 Biostrings_2.70.1 knitr_1.45 edgeR_4.0.1
[81] xfun_0.40 statmod_1.5.0 matrixStats_1.0.0 stringi_1.7.12
[85] yaml_2.3.7 evaluate_0.22 codetools_0.2-19 tibble_3.2.1
[89] BiocManager_1.30.22 cli_3.6.1 munsell_0.5.0 Rcpp_1.0.11
[93] GenomeInfoDb_1.38.0 parallel_4.3.1 readr_2.1.4 blob_1.2.4
[97] bitops_1.0-7 lme4_1.1-35.1 e1071_1.7-13 scales_1.2.1
[101] purrr_1.0.2 crayon_1.5.2 rlang_1.1.1 cowplot_1.1.1
[105] fastmatch_1.1-4
These binaries (installable software) and packages are in development.
They may not be fully stable and should be used with caution. We make no claims about them.