knitr::opts_chunk$set(message = FALSE, warning = FALSE)
Illumina Infinium HumanMethylation 450K BeadChip assay has become a standard tool to analyse methylation in human samples. Developed in 2011, it has already been used in projects such as The Cancer Genome Atlas (TCGA). Their 450.000 probes provide a good overall image of the methylation state of the genome, being one of the reasons of its success.
Given its complex design^[More information can be found at this minfi tutorial], many Bioconductor packages have been developed to assess normalization and pre-processing issues (e.g. r Biocpkg("minfi")
[@Aryee2014] or r Biocpkg("lumi")
[@Du2008]). In addition, these packages can detect differentially methylated probes (DMPs) and differentially methylated regions (DMRs). However, the interfaces are not very intuitive and several scripting steps are usually required.
r Biocpkg("MEAL")
aims to facilitate the analysis of Illumina Methylation 450K chips. We have included two methods to analyze DMPs (Differentially Methylated Probes), that test differences in means (limma) or differences in variance (DiffVar). We have included three DMRs (Differentially Methylated Regions) detection algorithms (bumphunter, blockFinder and DMRcate) and a new method to test differences in methylation in a target region (RDA). Finally, we have prepared plots for all these analyses as well as a wrapper to run all the analyses in the same dataset.
r Biocpkg("MEAL")
is meant to analyze methylation data already preprocessed. All our functions accept a GenomicRatioSet
as input, which is a class from r Biocpkg("minfi")
package designed to manage preprocessed methylation data. Users willing to preprocess their own data are encouraged to take a look to minfi's vignette
In this vignette, we will use methylation data from r Biocpkg("minfiData")
package.
library(MEAL) library(MultiDataSet) library(minfiData) library(minfi) library(ggplot2) data("MsetEx")
MsetEx
is a MethylationRatioSet
that contains measurements for 485512 CpGs and 6 samples, as well as some phenotypic variables such as age or sex. The first step will be to convert it to a GenomicRatioSet
. Then, we will add some extra features annotation. Finally, we will remove probes not measuring methylation, with SNPs or with NAs. For the sake of speed, we will select a subset of CpGs:
meth <- mapToGenome(ratioConvert(MsetEx)) rowData(meth) <- getAnnotation(meth)[, -c(1:3)] ## Remove probes measuring SNPs meth <- dropMethylationLoci(meth) ## Remove probes with SNPs meth <- dropLociWithSnps(meth) ## Remove probes with NAs meth <- meth[!apply(getBeta(meth), 1, function(x) any(is.na(x))), ] ## Select a subset of samples set.seed(0) meth <- meth[sample(nrow(meth), 100000), ]
The function runPipeline
run all methods included in r Biocpkg("MEAL")
to the same dataset. We only need to pass to this function a GenomicRatioSet
and the name of our variable of interest. In our case, we will analyze the effect of cancer on methylation:
res <- runPipeline(set = meth, variable_names = "status")
runPipeline
includes several parameters to customize the analyses. The most important parameters are covariable_names
, betas
and sva
. covariable_names
is used to include covariates in our models. betas
allows the user choosing between running the analyis with beta (TRUE) or M-values (FALSE). If sva
is TRUE, Surrogate Variable Analysis is run and surrogate variables are included in the models. Finally, some parameters modify the behaviour of the methods included in the wrapper and they will be covered later on. More information about the parameters can be found in the documentation (by typing ?runPipeline).
We will run a new analysis including age as covariate:
resAdj <- runPipeline(set = meth, variable_names = "status", covariable_names = "age", analyses = c("DiffMean", "DiffVar")) resAdj
runPipeline
generates a ResultSet
object. ResultSet
is a class designed to encapsulate different results from the same dataset. It contains the results of the different methods, the feature data and other data required to get tables or plots. We can examine the analyses included in a ResultSet
with the function names
:
names(resAdj)
Both objects contains five analyses. DiffMean is an analysis of difference of means performed with r Biocpkg("limma")
while the others are named with the method name (DiffVar, bumphunter, blockFinder and dmrcate).
We can use the function getAssociation
to get a data.frame with the results, independent of the original method. This function has two main arguments: object
and rid
. object
is the ResultSet
with our data and rid
is the name or the index of the analysis we want to extract.
head(getAssociation(resAdj, "DiffMean")) head(getAssociation(resAdj, "DiffVar"))
DiffMean and DiffVar are internally stored as a MArrayLM, the class from r Biocpkg("limma")
results. This class allows testing different constrasts or evaluating different variables simultaneously. The function getProbeResults
helps the user performing these operations. It also has the arguments object
and rid
from getAssociation
. coef
is a numeric with the index of the coefficient from which we want the results. If we did not pass a custom model to runPipeline
, the first coefficient (coef = 1) is the intercept and the second coefficient (coef = 2) is the first variable that we included in variable_names
. We can evaluate different coefficients simultaneously by passing a vector to coef
. contrast
is a matrix with the contrasts that we want to evaluate. This option is useful when our variable of interest is a factor with several levels and we want to do all the different comparisons. Finally, the argument fNames
is used to select the variables from features annotation that will be added to the tables.
To exemplify the use of this function, we will evaluate our whole adjusted model, including age coefficient. We will also add some annotation of the CpGs:
head(getProbeResults(resAdj, rid = 1, coef = 2:3, fNames = c("chromosome", "start")))
When more than one coefficient is evaluated, a estimate for each coefficient is returned and the t-statistic is substituted by a F-statistic. More information about linear models, including a detailed section of how to create a constrast matrix can be found in limma users' guide.
Finally, we can obtain the results of CpGs mapped to some genes with the function getGeneVals
. This function accepts the same arguments than getProbeResults
but includes the arguments gene
and genecol
to pass the names of the genes to be selected and the column name of feature data containing gene names.
We will retrieve the difference in variance results for all CpGs mapped to ARMS2. We can see in the rowData of meth
that gene names are in the column 'UCSC_RefGene_Name':
getGeneVals(resAdj, "ARMS2", genecol = "UCSC_RefGene_Name", fNames = c("chromosome", "start"))
We can easily get Manhattan plots, Volcano plots and QQ-plots for the probes results (DiffMean and DiffVar) using plot
method. Our extension of plot
method to ResultSet
includes the arguments rid
or coef
that were already present in getProbeResult
. In addition, the argument type
allows choosing between a Manhattan plot ("manhattan"), a Volcano plot ("volcano") or a qq-plot ("qq").
We can customize different aspects of a Manhattan plot. We can highlight the CpGs of a target region by passing a GenomicRanges
to the argument highlight
. Similarly, we can get a Manhattan plot with only the CpGs of our target region passing a GenomicRanges
to the argument subset
. It should be noticed that the GenomicRange
should have the chromosome as a number (1-24).
We will show these capabilities by highlighting and subsetting a region of ten Mb in chromosome X:
targetRange <- GRanges("23:13000000-23000000") plot(resAdj, rid = "DiffMean", type = "manhattan", highlight = targetRange) plot(resAdj, rid = "DiffMean", type = "manhattan", subset = targetRange)
We can also change the height of lines marking different levels of significance. Height of blue line can be set with suggestiveline
parameter and red line with genomewideline
parameter. It should be noticed that these values are expressed as -log10 of p-value. Finally, as our Manhattan plot is done with base
framework, we can customize the plot using base
plotting functions such as points
, lines
or text
or arguments of plot
function like main
:
plot(resAdj, rid = "DiffMean", type = "manhattan", suggestiveline = 3, genomewideline = 6, main = "My custom Manhattan") abline(h = 13, col = "yellow")
In our Volcano plot, we can also customize the thresholds for statistical significance and magnitude of the effect using the arguments tPV
and tFC
. As in the previous case, tPV
is expressed as -log10 of p-value. On the other hand, tFC
units will change depending if we used beta or M-values. show.labels
can turn on and turn off the labelling of significant features. Finally, Volcano plot is based on r CRANpkg("ggplot2")
so we can further customize the plot adding new layers:
plot(resAdj, rid = "DiffMean", type = "volcano", tPV = 14, tFC = 0.4, show.labels = FALSE) + ggtitle("My custom Volcano")
Our QQplot include the computation of the lambda, a measure of the inflation of the p-values. We can remove this value with the parameter show.lambda
.
Our qqplot is also based on r CRANpkg("ggplot2")
so we will add a title to customize it:
plot(resAdj, rid = "DiffMean", type = "qq") + ggtitle("My custom QQplot")
r Biocpkg("MEAL")
incorporates the function plotFeature
to plot the beta values distribution of a CpG. plotFeature
has three main arguments. set
is the GenomicRatioSet
with the methylation data. feat
is the index or name of our target CpG. variables
is a character vector with the names of the variables used in the plot. We can include two variables in our plot.
In the next line, we will plot a CpG with high difference in means between cases and controls (cg25104555) and a CpG with high difference in variance (cg11847929) vs cancer status. As plotFeature is based on r CRANpkg("ggplot2")
, we can customize it:
plotFeature(set = meth, feat = "cg09383816", variables = "status") + ggtitle("Diff Means") plotFeature(set = meth, feat = "cg11847929", variables = "status") + ggtitle("Diff Vars")
We can simultaneously plot the different results in a target region along with gene and CpG annotation with the function plotRegion
. This function has two main arguments. rset
is the ResultSet
and range
is a GenomicRanges
with our target region.
We will plot a region of 1 Mb in chromosome X:
targetRange <- GRanges("chrX:13000000-14000000") plotRegion(resAdj, targetRange)
Our plot has three main parts. The top contains the annotation of the regional genes and the CpGs included in the analysis. The middle part contains the results of the DMR detection methods (Bumphunter, blockFinder and DMRcate). The bottom part contains the results of the single probe analyses (differential mean and differential variance). Each analysis has two parts: the coefficients and the p-values. The line in the p-values plot marks the significance threshold.
By default,plotRegion
includes all analyses run in the plot. However, we can plot only few analyses with the parameter results
. We can also modify the height of the p-value line with the parameter tPV
(units are -log10 of p-value):
plotRegion(resAdj, targetRange, results = c("DiffMean"), tPV = 10)
r Biocpkg("MEAL")
includes wrappers to run the different methods of the pipeline individually. All these functions accept a GenomicRatioSet
as input and can return the results in a ResultSet
. Consequently, functionalities described in the above section for the results of the pipeline also apply for the results of a single method.
We can test if a phenotype causes changes in methylation means using the runDiffMeanAnalysis
. This function is a wrapper of lmFit
function from r Biocpkg("limma")
and requires two arguments: set
and model
. set
contains the methylation data, either in a GenomicRatioSet
or a matrix. model
can be a matrix with the linear model or a formula indicating the model. In the former case, set
must be a GenomicRatioSet
and the variables included in the model must be present in the colData of our set.
We exemplify the use of this function by running the same linear model than in our pipeline:
resDM <- runDiffMeanAnalysis(set = meth, model = ~ status)
runDiffMeanAnalysis
also has other parameters to customize the analysis. If set
is a GenomicRatioSet
, the parameter betas
allows us choosing between betas (TRUE) and M-values (FALSE). We can also run a robust linear model changing the parameter method
to "robust". Finally, resultSet
indicates if the function will return a ResultSet
(TRUE) or a MArrayLM
(FALSE).
All these parameters can be set in the runPipeline
function with the argument DiffMean_params
.
We can test if a phenotype causes changes in methylation variance using the runDiffVarAnalysis
. This function is a wrapper of varFit
function from r Biocpkg("missMethyl")
and requires three arguments: set
, model
and coefficient
. set
contains the methylation data in a GenomicRatioSet
. model
can be a matrix with the linear model or a formula indicating the model. In the former case, the variables included in the model must be present in the colData of our set. coefficient
indicates the variables of the linear model for which the difference of variance will be computed. By default, all discrete variables will be included.
We exemplify the use of this function by running the same model than in our pipeline:
resDV <- runDiffVarAnalysis(set = meth, model = ~ status, coefficient = 2)
runDiffVarAnalysis
also has the parameter resultSet
that allows returning a MArrayLM
object instead of a ResultSet
. Finally, we can change other parameters of varFit
function using the ...
argument. These parameters can also be set in the runPipeline
function passing them to the argument DiffVar_params
.
We can determine if a genomic region is differentially methylated with RDA (Redundancy Analysis). This analysis can be run with the function runRDA
that requires three arguments: set
, model
and range
. As in the previous functions, set
is a GenomicRatioSet
with the methylation data and model
contains the linear model either in a matrix or in a formula. range
is a GenomicRanges
with the coordinates of our target region.
We will exemplify the use of this function by running RDA
in a region of chromosome X:
targetRange <- GRanges("chrX:13000000-23000000") resRDA <- runRDA(set = meth, model = ~ status, range = targetRange)
runRDA
also has other parameters to customize the analysis. The parameter betas
allows us choosing between betas (TRUE) and M-values (FALSE). num_vars
selects the number of columns in model matrix considered as variables. The remaining columns will be considered as covariates. num_permutations
indicates the number of permutations run to compute p-values. resultSet
allows returning a rda
object from r CRANpkg("vegan")
package instead of a ResultSet
.
We can run RDA in our pipeline when we are a priori interested in a target genomic range. In this case, we will pass our target region to the argument range
of runPipeline
. We can pass other parameters of runRDA
using the argument rda_params
.
We can retrieve RDA results using the function getAssociation
:
getAssociation(resRDA, rid = "RDA")
RDA results are encapsulated in a rda object from r CRANpkg("vegan")
package. We can get a summary of RDA results with the function getRDAresults
:
getRDAresults(resRDA)
This function returns four values: R2, pval, global.R2 and global.pval. R2 is the ammount of variance that the model explains in our target region. pval is the probability of finding this ammount of variance of higher by change. global.R2 is the ammount of variance that our model explains in the whole genome. global.pval is the probability of finding a region with the same number of probes explaining the same or more variance than our target region. With these values, we can determine if our target region is differentially methylated and if this phenomena is local or global.
The function topRDAhits
returns a data.frame with features associated to first two RDA components. This functions computes a Pearson correlation test between the methylation values and the RDA components. Only CpGs with a p-value lower than tPV
parameter (by default 0.05) with any of the components are included in the data.frame:
topRDAhits(resRDA)
Finally, we can plot the first two dimensions of our RDA with the function plotRDA
. This function makes a biplot of samples and features. We can color the samples using categorical variables by passing in a data.frame to argument pheno
.
We will plot RDA using status variable of our sets colData:
plotRDA(object = resRDA, pheno = colData(meth)[, "status", drop = FALSE])
The RDA plot prints a label at the center of each group and the summary of RDA results (R^2^ and p-value) in the legend. plotRDA
has two additional arguments. main
is a character vector with the plot's title. n_feat
is a numeric with the number of feats that will have a label in the text. Only the n_feat
features most associated to each of the components will be displayed.
plotRDA
relies on base
paradigm, so we can add layers using functions from this infrastructure (e.g. lines
, points
...):
plotRDA(object = resRDA, pheno = colData(meth)[, "status", drop = FALSE]) abline(h = -1)
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