A brief introduction of ENmix R package for DNA methylation data analysis.
ENmix 1.43.1
The ENmix package provides a set of quality control, preprocessing/correction and data analysis tools for Illumina Methylation Beadchips. It includes functions to read in raw idat data, background correction, dye bias correction, probe-type bias adjustment, along with a number of additional tools. These functions can be used to remove unwanted experimental noise and thus to improve accuracy and reproducibility of methylation measures. ENmix functions are flexible and transparent. Users have option to choose a single pipeline command to finish all data pre-processing steps (including quality control, background correction, dye-bias adjustment, between-array normalization and probe-type bias correction) or to use individual functions sequentially to perform data pre-processing in a more customized manner. In addition the ENmix package has selectable complementary functions for efficient data visualization (such as QC plots, data distribution plot, manhattan plot and Q-Q plot), quality control (identifing and filtering low quality data points, samples, probes, and outliers, along with imputation of missing values), identification of probes with multimodal distributions due to SNPs or other factors, exploration of data variance structure using principal component regression analysis plot, preparation of experimental factors related surrogate control variables to be adjusted in downstream statistical analysis, an efficient algorithm oxBS-MLE to estimate 5-methylcytosine and 5-hydroxymethylcytosine level; estimation of celltype proporitons; methlation age calculation and differentially methylated region (DMR) analysis.
Most ENmix package can also support the data structure used by several other related R packages, such as minfi, wateRmelon and ChAMP, providing straightforward integration of ENmix-corrected datasets for subsequent data analysis.
ENmix readidat function does not depend on array annotation R packages. It can directly read in Illuminal manifest file, which makes it easier to work with newer array, such as MethylationEPICv2.0 and mouse Beadchip.
The software is designed to support large scale data analysis, and provides multi-processor parallel computing options for most functions.
Data acquisition
readidat()
: Read idat files into R
readmanifest()
: Read array manifest file into R
Quality control
QCinfo()
: Extract and visualize QC information
plotCtrl()
: Generate internal control plots
getCGinfo()
: Extract CpG probe annotation information
calcdetP()
: Compute detection P values
qcfilter()
: Remove low quality values, samples or CpGs; remove outlier samples and perform imputation
nmode()
: Identify “gap” probes, i.e. those with multimodal distribution from underlying caused by underlying SNPs
dupicc()
: Calculate Introclass correlation coefficient (ICC) using data for duplicates
freqpoly()
: Frequency polygon plot for single variable
multifreqpoly()
: Frequency polygon plot for multiple variables
Preprocessing
mpreprocess()
: Preprocessing pipeline
preprocessENmix()
: ENmix background correction and dye bias correction
relic()
: RELIC dye bias correction
norm.quantile()
: Quantile normalization
rcp()
: RCP probe design type bias correction
Differential methylated region (DMR) analysis
ipdmr()
: ipDMR differentially methylated region analysis
combp()
: Combp differentially methylated region analysis
Other functions
oxBS.MLE()
: MLE estimates of 5-methylcytosine (5mC) and 5-hydroxymethylcytosine (5hmC)
estimateCellProp()
: Estimate white blood cell type proportions
methyAge()
: Calculate methylation age
methscore()
: calculate various methylation predictors, including DNA methylation age, exposures and plasma protein levels.
predSex()
: Estimate sample sex
ctrlsva()
: Derive surrogate variables to control for experimental confounding using non-negative internal control probes
pcrplot()
: Principal component regression plot
mhtplot()
: P value manhattan plot
p.qqplot()
: P value Q-Q plot
B2M()
: Convert Beta value to M value
M2B()
: Convert M value to Beta value
ENmix organizes data with two different classes.
rgDataSet
contains raw data (including internal control probes) from IDAT file, CpG annotation from Illumina manifest file and/or sample inforamtion (plate, array, and phenotypes) provided by users. Array intensity data is organized by probe (not CpG locus) at red and green channel.
methDataSet
contains methylated and unmethylated intensity values (organized by CpG), CpG annotation from Illumina manifest file and/or sample inforamtion (plate, array, and phenotypes) provided by users.
The following examples are brief demonstrations on how to perform DNA methylation analysis using ENmix functions.
The pipeline function mpreprocess()
can be used to perform quality
control and data preprocessing.
rgSet <- readidat(datapath)
beta=mpreprocess(rgSet)
These can achieve the following tasks:
The following is an executable example.
library(ENmix)
#read in data
require(minfiData)
#read in IDAT files
path <- file.path(find.package("minfiData"),"extdata")
rgSet <- readidat(path = path,recursive = TRUE)
#data pre-processing
beta=mpreprocess(rgSet,nCores=6)
#quality control, data pre-processing and imputation
beta=mpreprocess(rgSet,nCores=6,qc=TRUE,fqcfilter=TRUE,
rmcr=TRUE,impute=TRUE)
#CpG information (from Illumina manifest file) is self-contained in rgDataSet or methDataSet
cginfo=getCGinfo(rgSet)
#It has the same infomation if extracted from methDataSet
meth=getmeth(rgSet)
cginfo1=rowData(meth)
#Probe information for internal controls
ictrl=getCGinfo(rgSet,type="ctrl")
The example code below is basically doing the same thing as in example 1, but has more customized options.
library(ENmix)
#read in data
path <- file.path(find.package("minfiData"),"extdata")
rgSet <- readidat(path = path,recursive = TRUE)
#QC info
qc<-QCinfo(rgSet)
#background correction and dye bias correction
#if qc info object is provided, the low quality or outlier samples
# and probes will be excluded before background correction
mdat<-preprocessENmix(rgSet, bgParaEst="oob", dyeCorr="RELIC",
QCinfo=qc, nCores=6)
#between-array normalization
mdat<-norm.quantile(mdat, method="quantile1")
#probe-type bias adjustment
beta<-rcp(mdat,qcscore=qc)
#set low quality and outlier data points as NA (missing value)
#remove samples and probes with too many (eg. >5%) missing data
#perform imputation to replace missing values
beta <- qcfilter(beta,qcscore=qc,rmcr=TRUE,impute=TRUE)
#remove suffix and combine duplicated CpGs with rm.cgsuffix(), for EPIC v2
#beta2=rm.cgsuffix(beta)
This example is a brief demonstration of major functions in ENmix. Getting detailed information about data quality, SNP-like/gap probes, excluding user-specified probes and/or samples, principal component regression analysis, low quality or outlier sample or probe removal, sex prediction, cell type proportion estimation, methylation age estimation, differentially methylated region analysis and surrogate variables for batch effect, etc.
library(ENmix)
#read in data
path <- file.path(find.package("minfiData"),"extdata")
rgSet <- readidat(path = path,recursive = TRUE)
#attach some phenotype info for later use
sheet <- read.metharray.sheet(file.path(find.package("minfiData"),
"extdata"),pattern = "csv$")
rownames(sheet)=paste(sheet$Slide,sheet$Array,sep="_")
colData(rgSet)=as(sheet[colnames(rgSet),],"DataFrame")
#generate internal control plots to inspect quality of experiments
plotCtrl(rgSet)
#generate quality control (QC) information and plots,
#identify outlier samples in data distribution
#if set detPtype="negative", recommend to set depPthre to <= 10E-6
#if set detPtype="oob", depPthre of 0.01 or 0.05 may be sufficient
#see Heiss et al. PMID: 30678737 for details
qc<-QCinfo(rgSet,detPtype="negative",detPthre=0.000001)
###data preprocessing
#background correction and dye bias correction
mdat<-preprocessENmix(rgSet, bgParaEst="oob", dyeCorr="RELIC",
QCinfo=qc, nCores=6)
#between-array normalization
mdat<-norm.quantile(mdat, method="quantile1")
#attach phenotype data for later use
colData(mdat)=as(sheet[colnames(mdat),],"DataFrame")
#probe-type bias adjustment
beta<-rcp(mdat,qcscore=qc)
#Search for multimodal CpGs, so called gap probes
#beta matrix before qcfilter() step should be used for this purpose
nmode<-nmode(beta, minN = 3, modedist=0.2, nCores = 6)
#filter low quality and outlier data points for each probe
#rows and columns with too many missing values will be removed if specify
#Imputation will be performed to fill missing data if specify.
beta <- qcfilter(beta,qcscore=qc,rmcr=TRUE, rthre=0.05,
cthre=0.05,impute=TRUE)
#If for epigenetic mutation analysis, outliers should be kept
beta <- qcfilter(beta,qcscore=qc,rmoutlier=FALSE,rmcr=TRUE, rthre=0.05,
cthre=0.05,impute=FALSE)
#remove suffix and combine duplicated CpGs with rm.cgsuffix(), for EPIC v2
#beta2=rm.cgsuffix(beta)
##Principal component regression analysis plot to check data variance structure
#phenotypes to be studied in the plot
cov<-data.frame(group=colData(mdat)$Sample_Group,
slide=factor(colData(mdat)$Slide))
#missing data is not allowed in the analysis!
pcrplot(beta, cov, npc=6)
#Non-negative control surrogate variables, which can be used in
# downstream association analysis to control for batch effects.
csva<-ctrlsva(rgSet)
#estimate cell type proportions
#rgDataset or methDataSet can also be used for the estimation
celltype=estimateCellProp(userdata=beta,
refdata="FlowSorted.Blood.450k",
nonnegative = TRUE,normalize=TRUE)
#predic sex based on rgDataSet or methDataset
sex=predSex(rgSet)
sex=predSex(mdat)
#Methylation predictors (>150), including methylation age calculation
pheno=data.frame(SampleID=colnames(beta),Age=c(23,45,52,36,58,43),Female=c(1,0,1,1,0,1))
mscore=methscore(datMeth=beta,datPheno=pheno)
#ICC analysis can be performed to study measurement reliability if
# have duplicates, see manual
#dupicc()
#After association analysis, the P values can be used for DMR analysis
#simulate a small example file in BED format
dat=simubed()
#using ipdmr method, low seed value (0.01 or 0.05) should be used in real study.
ipdmr(data=dat,seed=0.1)
#using comb-p method
combp(data=dat,seed=0.1)
The first step is to import array raw data files (*.idat)
to create an object of rgDataSet
, which is similar to
RGChannelSetExtended
in minfi package, but with probe annotation
integrated, and it has smaller data size (about 1/3 smaller). Alternatively, User can also
use minfi package to read in idat files and create
RGChannelSetExtended
. Most functions in ENmix support
RGChannelSetExtended
and RGChannelSet
.
Some array types and corresponding manifestfiles can be guessed by the program based on the number of probes per array. However, we recommend users provide the correct manifest file (.csv format) directly for their types of array, which can be easily downloaded from Illumina website, see below for some examples. This option also allows the function to read in data from newer array, such as mouse array.
library(ENmix)
rgSet <- readidat(path = "directory path for idat files",
recursive = TRUE)
#Download manifestfile for HumanMethylation450 beadchip
system("wget https://webdata.illumina.com/downloads/productfiles/humanmethylation450/humanmethylation450_15017482_v1-2.csv")
mf="HumanMethylation450_15017482_v1-2.csv"
rgSet <- readidat(path = "path to idat files",manifestfile=mf,recursive = TRUE)
When methylation IDAT raw data files are not available, such as for some
publicly available datasets, users can use methylated (M) and unmethylated
(U) intensity data to create an object of MethylSet
. MethylSet
is also supported by most functions in ENmix.
M<-matrix_for_methylated_intensity
U<-matrix_for_unmethylated_intensity
pheno<-as.data.frame(cbind(colnames(M), colnames(M)))
names(pheno)<-c("Basename","filenames")
rownames(pheno)<-pheno$Basename
pheno<-AnnotatedDataFrame(data=pheno)
anno<-c("IlluminaHumanMethylation450k", "ilmn12.hg19")
names(anno)<-c("array", "annotation")
mdat<-MethylSet(Meth = M, Unmeth = U, annotation=anno,
phenoData=pheno)
Both Illumina 450k and EPIC array incorporate 15 different types of internal control
probes (total of 848 probes for 450K and 635 probes for EPIC). The control
plots from ENmix function plotCtrl()
are similar to the control plots generated
by Illumina GenomeStudio software. See Illumina Infinium HD Methylation Assay for
detailed description on how to interpret these control figures.
plotCtrl(rgSet)
Below is a list of internal control types and number of probes for each type.
Control types | 450K | EPIC v1 | EPIC v2 |
Sample-Independent Controls | |||
STAINING | 4 | 6 | 4 |
EXTENSION | 4 | 4 | 4 |
HYBRIDIZATION | 3 | 3 | 3 |
TARGET REMOVAL | 2 | 2 | 2 |
RESTORATION | 1 | 1 | 1 |
Sample-Dependent Controls | |||
BISULFITE CONVERSION I | 12 | 10 | 10 |
BISULFITE CONVERSION II | 4 | 4 | 4 |
SPECIFICITY I | 12 | 12 | 12 |
SPECIFICITY II | 3 | 3 | 3 |
NON-POLYMORPHIC | 4 | 9 | 9 |
NORM_A | 32 | 27 | 27 |
NORM_C | 61 | 58 | 58 |
NORM_G | 32 | 27 | 27 |
NORM_T | 61 | 58 | 58 |
NEGATIVE | 613 | 411 | 411 |
These controls can be plotted in user specified order to check how experimental factors affect methylation measures, such as batch, plate, array or array location.
path <- file.path(find.package("minfiData"),"extdata")
rgSet <- readidat(path = path,recursive = TRUE)
sheet <- read.metharray.sheet(file.path(find.package("minfiData"),
"extdata"), pattern = "csv$")
rownames(sheet)=paste(sheet$Slide,sheet$Array,sep="_")
colData(rgSet)=as(sheet[colnames(rgSet),],"DataFrame")
#control plots
IDorder=rownames(colData(rgSet))[order(colData(rgSet)$Slide,
colData(rgSet)$Array)]
plotCtrl(rgSet,IDorder)
Methylation intensity or beta value distribution plots are
very useful for data summary, visual inspection and identification of
outlier samples. Density plots are routinely generated using R function
multidensity()
. However, the function is computationally intensive,
and can take several hours to produce density plots for a large methylation
dataset.
Frequency polygon plot is an alternative figure for inspection of data distribution. Similar to histogram, it can accurately reflect data distribution and easy to understand. The function is also much faster, and only takes a few minutes to produce a distribution plot for >1000 samples.
mraw <- getmeth(rgSet)
#total intensity plot is userful for data quality inspection
#and identification of outlier samples
multifreqpoly(assays(mraw)$Meth+assays(mraw)$Unmeth,
xlab="Total intensity")
#Compare frequency polygon plot and density plot
beta<-getB(mraw)
anno=rowData(mraw)
beta1=beta[anno$Infinium_Design_Type=="I",]
beta2=beta[anno$Infinium_Design_Type=="II",]
library(geneplotter)
jpeg("dist.jpg",height=900,width=600)
par(mfrow=c(3,2))
multidensity(beta,main="Multidensity")
multifreqpoly(beta,main="Multifreqpoly",xlab="Beta value")
multidensity(beta1,main="Multidensity: Infinium I")
multifreqpoly(beta1,main="Multifreqpoly: Infinium I",
xlab="Beta value")
multidensity(beta2,main="Multidensity: Infinium II")
multifreqpoly(beta2,main="Multifreqpoly: Infinium II",
xlab="Beta value")
dev.off()
See the following figures generated from the above code. When type I and type II probes are plotted separately bottom 4 panels, the difference in modes between type I and II probes can be appreciated. But when all probes are plotted together (top panel), the multidensity plot obscures these differences, while they remain readily apparent in the multifreqpoly plot. In addition, the multidensity plots appear to suggest that probes range in value from <0 to >1, whereas multifreqpoly correctly show the range from 0 to 1.
Data quality measures, including detection P values, average intensities for
bisulfite conversion probes and number of
beads for each methylation read
can be extracted or estimated using the
function QCinfo()
from an object of rgDataSet
or
RGChannelSetExtended
. Based on default or user specified
quality score thresholds, the QCinfo()
will identify
a list of low quality samples and CpG probes as wells as outlier samples based on
total intensity or beta value distribution. These samples and probes
should be excluded before
further analysis. Data quality score figures “qc_sample.jpg” and “qc_CpG.jpg” from
QCinfo()
can be used to guide the selection of quality score
thresholds. Low quality samples and probes
are listed as “badsample” and “badCpG” in QCinfo object, and also marked
in red in figure “freqpolygon_beta_beforeQC.jpg”.
qc<-QCinfo(rgSet)
#QCinfo returns "detP","nbead","bisul","badsample","badCpG","outlier_sample"
#Samples with low quality data
qc$badsample
#CpGs with low quality data
qc$badCpG
#outlier samples
qc$outlier_sample
#Low quality samples and probes should be excluded before data preprocesssing
#by specifying `QCinfo` in `preprocessENmix()`
mdat<-preprocessENmix(rgSet, QCinfo=qc, nCores=6)
After excluding low quality samples and probes, as well as outlier samples.
we can still have many low quality and outlier data points for many CpGs.
These small percentage of data points can have big impact on downstream
association statistical tests for individual CpGs.
Function qcfilter()
can be used to filter out these
data points and replace them with missing value NA. Outliers are defined as
values smaller than 3 times IQR from the lower quartile or larger than
3 times IQR from the upper quartile. Some statistical methods do not allow
missing values,(e.g. principal component analysis), so
argument in the function can be
specified to impute missing data using k-nearest neighbors method.
#filter outlier values only
b1=qcfilter(beta)
#filter low quality and outlier values
b2=qcfilter(beta,qcscore=qc)
#filter low quality and outlier values, remove rows
#and columns with too many missing values
b3=qcfilter(beta,qcscore=qc,rmcr=TRUE)
#filter low quality and outlier values, remove rows and
#columns with too many (rthre=0.05,cthre=0.05, 5% in default) missing values,
# and then do imputation
b3=qcfilter(beta,qcscore=qc,rmcr=TRUE,rthre=0.05,
cthre=0.05,impute=TRUE)
Function preprocessENmix()
incorporates a model-based background
correction method ENmix
, which models methylation signal intensities
with a flexible exponential-normal mixture distribution, together
with a truncated normal distribution to model background noise.
Argument “dyeCorr”
can be used to specify a method for dye-bias correction, the default is RELIC.
Refer the following papers for the detailed description of related methods:
Zongli Xu, et. al. ENmix: a novel background correction method for Illumina HumanMethylation450 BeadChip, Nucleic Acids Research, 2015
Xu Z, Langie SA, De Boever P, Taylor JA, Niu L. RELIC: a novel dye-bias correction method for Illumina Methylation BeadChip. BMC Genomics. 2017
If argument QCinfo is specified, the low quality samples and probes identified
by function QCinfo()
will be excluded before ENmix background correction.
Using argument exSample
and exCpG
, User can also specify a list
of samples or probes to be excluded before background correction.
qc=QCinfo(rgSet)
mdat<-preprocessENmix(rgSet, bgParaEst="oob", dyeCorr="RELIC",
QCinfo=qc, exCpG=NULL, nCores=6)
Function norm.quantile()
can be used to perform quantile
normalization on methylation intensity values.
mdat<-norm.quantile(mdat, method="quantile1")
The majority of probes on Illumina 450K and EPIC BeadChips are type II probes. Although type II probes facilitate increased array genome coverage, they were shown to have decreased dynamic range and reproducibility compared to type I probes. Taking advantage of the high spatial correlation of DNA methylation levels along the human genome, The RCP (Regression on Correlated Probes) method utilizes nearby (<25 bp) type I and II probe pairs to derive the quantitative relationship between probe types and then recalibrates type II probe measurements using type I probes as referents.
beta<-rcp(mdat)
Refer the following publication for the detailed description of the method:
Niu L, Xu Z, Taylor JA. RCP: a novel probe design bias correction method for Illumina Methylation BeadChip. Bioinformatics, 2016
Function ctrlsva()
can be used to estimate surrogate variables for batch
effects and unknown experimental confounders using intensity data for non-negative
internal control probes. These surrogate variables can then be modeled as covariables in
downstream association analysis to adjust for experimental variation.
sva<-ctrlsva(rgSet)
First, principal component analysis will be performed on the standardized beta value
matrix (standardized probe by probe), and then the specified number of top
principal components (that explain most data variation) will be used to perform
linear regression with each specified variables, such as batch or phenotype
variables. Regression P values will be
plotted to explore methylation data variance structure and to identify possible
confounding variables to guide association statistical analysis. Principal
components are ordered according to the percentage of variance they explained
from large to small. PCA will not allow for missing values, so specify impute=true
in preprocessing (qcfilter()
) if there is missing data.
require(minfiData)
mdat <- preprocessRaw(RGsetEx)
beta=getBeta(mdat, "Illumina")
group=pData(mdat)$Sample_Group
slide=factor(pData(mdat)$Slide)
cov=data.frame(group,slide)
pcrplot(beta,cov,npc=6)
Function nmode()
uses an empirical approach to identify
CpGs whose methylation values are multimodal distributed
(SNP-like or gap probes). When measured in a population of people
the majority of CpGs on the Illumina HumanMethylation450 BeadChip have
unimodal distributions of DNA methylation values with relatively small
between-person variation. However, some CpGs may have multimodal
distributions of methylation values with sizeable differences between
modes and large between-person variation.
These multimodal distributed data are usually caused by SNP effect in the probe region, problematic probe design or other unknown artifacts rather than by actual difference in methylation level and thus should be excluded from DNA methylation analysis. Researchers have often excluded CpGs based simply on SNP annotation information (e.g. reported SNPs in or near probe sequences). However, because SNP frequency and annotation always depends on population origin, we find that this approach alone may exclude many well-distributed (unimodal) CpGs, while still failing to identify other problematic multi-modal CpGs. We developed an empirical approach to identify CpGs that are obviously not uni-modally distributed, so that researchers can make more informed decisions about whether to exclude them in their particular study populations and analyses.
See online supplementary materials of the following paper for
an evaluation of the method using published EWAS data.
Zongli Xu, Liang Niu, Leping Li and Jack A. Taylor ENmix: a novel background correction method for Illumina HumanMethylation450 BeadChip, Nucleic Acids Research, 2015
nmode<- nmode(beta, minN = 3, modedist=0.2, nCores = 5)
Whole blood samples are often used in EWAS, however, whole blood has
mixed cell types and methylation level can be widely different between
different cell types. Function estimateCellProp()
can be used
to estimate cell types based on reference dataset. Users should select
a reference that is most resemble to their own study samples. Currently
there are 6 publicly deposited reference datasets:
“FlowSorted.Blood.450k”,
“FlowSorted.DLPFC.450k”,“FlowSorted.CordBlood.450k”,
“FlowSorted.CordBloodCombined.450k”,
“FlowSorted.CordBloodNorway.450k” or “FlowSorted.Blood.EPIC”.
require(minfidata)
path <- file.path(find.package("minfiData"),"extdata")
#based on rgDataset
rgSet <- readidat(path = path,recursive = TRUE)
celltype=estimateCellProp(userdata=rgSet,
refdata="FlowSorted.Blood.450k",
nonnegative = TRUE,normalize=TRUE)
The input data can be in one of the follow format: rgDataSet
,
methDataSet
, MethylSet
,
RGChannelSet
or methylation beta value matrix.
Methylation age can reflect a person’s biological age, which may be more
related to the person’s health status than chronological age. Several
types of methylation age can be estimated using
methyAge()
. The more comprehensive function is methsocre()
, which calculate more than 150 methylation predictors, including all predictors from methyAge()
require(minfidata)
path <- file.path(find.package("minfiData"),"extdata")
#based on rgDataset
rgSet <- readidat(path = path,recursive = TRUE)
meth=getmeth(rgSet)
beta=getB(meth)
mage=methyAge(beta)
pheno=data.frame(SampleID=colnames(beta),Age=c(23,45,52,36,58,43),Female=c(1,0,1,1,0,1))
mscore=methscore(datMeth=beta,datPheno=pheno)
EWAS is usually done probe by probe. However, in the human genome, nearby
CpGs often have similar methylation status, so combined statistics from nearby
CpGs can potentially increase association signal. Functions ipdmr()
and
combp()
can utilize P values from EWAS to identify
differentially methylated regions (DMRs). The argument “seed” in these two functions
indicate the FDR threshold for initial selection of DMR regions, but we
note that same value of seed do not appear to have the same effect in these
two functions. It is often more stringent in ipdmr than combp. For more information see:
Xu Z, Xie C, Taylor JA, Niu L. ipDMR: identification of differentially methylated regions with interval P-values. Bioinformatics. 2021 May 5;37(5):711-713. doi: 10.1093/bioinformatics/btaa732. PMID: 32805005; PMC8248314.
There is no true DMR in the following example data, we set less stringent seed threshold is only for demostration purpose to show what the output looks like when DMRs were detected.
dat=simubed()
names(dat)
ipdmr(data=dat,seed=0.1)
combp(data=dat,seed=0.1)
Several studies have showen that a large percentage of CpGs on Illumina arrays
have poor reliability, i.e. they have low correlation between replicate measures
in a same set of samples. Measurement of the reliability of individual CpGs
can be assessed by calculating intraclass
correlation coefficients (ICC) using methylation from duplicate samples. Function
dupicc()
can be used for this purpose.
require(minfiData)
path <- file.path(find.package("minfiData"),"extdata")
rgSet <- readidat(path = path,recursive = TRUE)
mdat=getmeth(rgSet)
beta=getB(mdat,"Illumina")
#assuming list in id1 are corresponding duplicates of id2
dupidx=data.frame(id1=c("5723646052_R02C02","5723646052_R04C01",
"5723646052_R05C02"),
id2=c("5723646053_R04C02","5723646053_R05C02",
"5723646053_R06C02"))
iccresu<-dupicc(dat=beta,dupid=dupidx)
Studies showed that 5-Methylcytosine and 5-hydroxymethylcytosine can have very different
function. However, traditional bisulfite (BS) treatment commonly used in genome-wide
methylation studies can not distinguish 5mC from 5hmC. Sequencing or array data from
paired DNA samples (bisulfite and oxidative bisulfite conversion) are needed for the
separate estimation. Bisulfite converted DNA can be used to estimate the proportion
of 5mC+5hmC and oxidative bisulfite (oxBS) converted DNA can be used to estimate
the proportion of 5mC. Function oxBS.MLE()
can be used to generate the
maximum Likelihood Estimate (MLE) of 5mC and 5hmC using sequencing or array data from
paired experiments (Xu et al. Bioinformatics 2016).
load(system.file("oxBS.MLE.RData",package="ENmix"))
resu<-oxBS.MLE(beta.BS,beta.oxBS,N.BS,N.oxBS)
dim(resu[["5mC"]])
dim(resu[["5hmC"]])
Zongli Xu, Liang Niu, Leping Li and Jack A. Taylor, ENmix: a novel background correction method for Illumina HumanMethylation450 BeadChip. Nucleic Acids Research, 2015
Liang Niu, Zongli Xu and Jack A. Taylor, RCP: a novel probe design bias correction method for Illumina Methylation BeadChip. Bioinformatics 2016
Zongli Xu, Jack A. Taylor, Yuet-Kin Leung, Shuk-Mei Ho and Liang Niu, oxBS-MLE: An efficient method to estimate 5-methylcytosine and 5-hydroxymethylcytosine in paired bisulfite and oxidative bisulfite treated DNA. Bioinformatics 2016
Zongli Xu, Sabine A. S. Langie, Patrick De Boever, Jack A. Taylor1 and Liang Niu, RELIC: a novel dye-bias correction method for Illumina Methylation BeadChip. BMC Genomics 2017
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## R Under development (unstable) (2024-10-21 r87258)
## Platform: x86_64-pc-linux-gnu
## Running under: Ubuntu 24.04.1 LTS
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## Matrix products: default
## BLAS: /home/biocbuild/bbs-3.21-bioc/R/lib/libRblas.so
## LAPACK: /usr/lib/x86_64-linux-gnu/lapack/liblapack.so.3.12.0
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## locale:
## [1] LC_CTYPE=en_US.UTF-8 LC_NUMERIC=C
## [3] LC_TIME=en_GB LC_COLLATE=C
## [5] LC_MONETARY=en_US.UTF-8 LC_MESSAGES=en_US.UTF-8
## [7] LC_PAPER=en_US.UTF-8 LC_NAME=C
## [9] LC_ADDRESS=C LC_TELEPHONE=C
## [11] LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=C
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## time zone: America/New_York
## tzcode source: system (glibc)
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## attached base packages:
## [1] stats graphics grDevices utils datasets methods base
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## other attached packages:
## [1] BiocStyle_2.35.0
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## loaded via a namespace (and not attached):
## [1] digest_0.6.37 R6_2.5.1 bookdown_0.41
## [4] fastmap_1.2.0 xfun_0.49 cachem_1.1.0
## [7] knitr_1.49 htmltools_0.5.8.1 rmarkdown_2.29
## [10] lifecycle_1.0.4 cli_3.6.3 sass_0.4.9
## [13] jquerylib_0.1.4 compiler_4.5.0 tools_4.5.0
## [16] evaluate_1.0.1 bslib_0.8.0 yaml_2.3.10
## [19] BiocManager_1.30.25 jsonlite_1.8.9 rlang_1.1.4