This is an introductory guide to integration analysis between exposome and omics data with R package omicRexposome. The document illustrates two types of analysis: 1) Association analysis, that are performed between exposome and a single omic data-set; and 2) Integration analysis where multiple data-sets, including exposome data, are analysed at the same time.
omicRexposome 1.22.0
omicRexposome
is an R package designed to work join with rexposome
. The aim of omicRexposome
is to perform analysis joining exposome and omic data with the goal to find the relationship between a single or set of exposures (external exposome) and the behavior of a gene, a group of CpGs, the level of a protein, etc. Also to provide a series of tools to analyse exposome and omic data using standard methods from Biocondcutor.
omicRexposome
is currently in development and not available from CRAN nor Bioconductor. Anyway, the package can be installed by using devtools R package and taking the source from Bioinformatic Research Group in Epidemiology’s GitHub repository.
This can be done by opening an R session and typing the following code:
devtools::install_github("isglobal-brge/omicRexposome")
User must take into account that this sentence do not install the packages’ dependencies.
Two different types of analyses can be done with omicRexposome
:
Analysis | omicRexposome function |
---|---|
Association Study | association |
Integration Study | crossomics |
Both association and integration studies are based in objects of class MultiDataSet
. A MultiDataSet
object is a contained for multiple layers of sample information. Once the exposome data and the omics data are encapsulated in a MultiDataSet
the object can be used for both association and integration studies.
The method association
requires a MultiDataSet
object having to types of information: the exposome data from an ExposomeSet
object and omic information from objects of class ExpressionSet
, MethylationSet
, SummarizedExperiment
or others. ExposomeSet
objects are created with functions read_exposome
and load_exposome
from rexposome
R package (see next section Loading Exposome Data) and encapsulates exposome data. The method crossomics
expects a MultiDataSet
with any number of different data-sets (at last two). Compared with association
method, crossomics
do not requires an ExposomeSet
.
In order to illustrate the capabilities of omicRexposome
and the exposome-omic analysis pipeline, we will use the data from BRGdata
package. This package includes different omic-sets including methylation, transcriptome and proteome data-sets and an exposome-data set.
omicRexposome
and MultiDataSet
R packages are loaded using the standard library command:
library(omicRexposome)
## Warning: replacing previous import 'utils::findMatches' by
## 'S4Vectors::findMatches' when loading 'AnnotationDbi'
library(MultiDataSet)
The association studies are performed using the method association
. This method requires, at last four, augments:
object
should be filled with a MultiDataSet
object.formula
should be filled with an expression containing the covariates used to adjust the model.expset
should be filled with the name that the exposome-set receives in the MultiDataSet
object.omicset
should be filled with the name that the omic-set receives in the MultiDataSet
object.The argument formula
should follow the pattern: ~sex+age
. The method association
will fill the formula placing the exposures in the ExposomeSet
m between ~
and the covariates sex+age
.
association
implements the limma
pipeline using lmFit
and eBayes
in the extraction methods from MultiDataSet
. The method takes care of the missing data in exposures, outcomes and omics data and locating and is subsets both data-sets, exposome data and omic data, by common samples. The argument method
allows to select the fitting method used in lmFit
. By default it takes the value "ls"
for least squares but it can also takes "robust"
for robust regression.
The following subsections illustrates the usage of association
with different types of omics data: methylome, transcriptome and proteome.
First we get the exposome data from BRGdata
package that we will use in the whole section.
data("brge_expo", package = "brgedata")
class(brge_expo)
## [1] "ExposomeSet"
## attr(,"package")
## [1] "rexposome"
The aim of this analysis is to perform an association test between the gene expression levels and the exposures. So the first point is to obtain the transcriptome data from the brgedata
package.
data("brge_gexp", package = "brgedata")
The association studies between exposures and transcriptome are done in the same way that the ones with methylome. The method used is association
, that takes as input an object of MultiDataSet
class with both exposome and expression data.
mds <- createMultiDataSet()
mds <- add_genexp(mds, brge_gexp)
mds <- add_exp(mds, brge_expo)
gexp <- association(mds, formula=~Sex+Age,
expset = "exposures", omicset = "expression")
We can have a look to the number of hits and the lambda score of each analysis with the methods tableHits
and tableLambda
, seen in the previous section.
hit <- tableHits(gexp, th=0.001)
lab <- tableLambda(gexp)
merge(hit, lab, by="exposure")
## exposure hits lambda
## 1 BPA_p 19 0.9072377
## 2 BPA_t1 27 0.8807316
## 3 BPA_t3 56 0.9391129
## 4 Ben_p 19 0.8013466
## 5 Ben_t1 12 0.8234104
## 6 Ben_t2 9 0.8393350
## 7 Ben_t3 21 0.8301203
## 8 NO2_p 32 1.0281960
## 9 NO2_t1 16 0.7942881
## 10 NO2_t2 35 1.1482314
## 11 NO2_t3 31 0.8770931
## 12 PCB118 59 0.9308472
## 13 PCB138 38 1.0726221
## 14 PCB153 51 1.1743989
## 15 PCB180 17 0.9790750
Since most of all models have a lambda under one, we should consider use Surrogate Variable Analysis. This can be done using the same association
method but by setting the argument sva
to "fast"
so the pipeline of isva
and SmartSVA
R packages is applied. If sva
is set to "slow"
the applied. pipeline is the one from sva
R package.
gexp <- association(mds, formula=~Sex+Age,
expset = "exposures", omicset = "expression", sva = "fast")
We can re-check the results creating the same table than before:
hit <- tableHits(gexp, th=0.001)
lab <- tableLambda(gexp)
merge(hit, lab, by="exposure")
## exposure hits lambda
## 1 BPA_p 50 0.9874152
## 2 BPA_t1 51 0.9453795
## 3 BPA_t3 61 0.9842216
## 4 Ben_p 76 1.0117733
## 5 Ben_t1 64 1.0115515
## 6 Ben_t2 71 1.0089834
## 7 Ben_t3 59 0.9969123
## 8 NO2_p 78 1.0117151
## 9 NO2_t1 68 1.0056950
## 10 NO2_t2 69 1.0210000
## 11 NO2_t3 49 0.9802407
## 12 PCB118 129 1.0518170
## 13 PCB138 67 1.0094139
## 14 PCB153 58 0.9924482
## 15 PCB180 67 0.9973381
The objects of class ResultSet
have a method called plotAssociation
that allows to create QQ Plots (that are another useful way to see if there are some inflation/deflation in the P-Values).
gridExtra::grid.arrange(
plotAssociation(gexp, rid="Ben_p", type="qq") +
ggplot2::ggtitle("Transcriptome - Pb Association"),
plotAssociation(gexp, rid="BPA_p", type="qq") +
ggplot2::ggtitle("Transcriptome - THM Association"),
ncol=2
)
Following this line, the same method plotAssociation
can be used to create volcano plots.
gridExtra::grid.arrange(
plotAssociation(gexp, rid="Ben_p", type="volcano", tPV=-log10(1e-04)) +
ggplot2::ggtitle("Transcriptome - Pb Association"),
plotAssociation(gexp, rid="BPA_p", type="volcano", tPV=-log10(1e-04)) +
ggplot2::ggtitle("Transcriptome - THM Association"),
ncol=2
)
The proteome data-set included in brgedata
has 47 proteins for 90 samples.
data("brge_prot", package="brgedata")
brge_prot
## ExpressionSet (storageMode: lockedEnvironment)
## assayData: 47 features, 90 samples
## element names: exprs
## protocolData: none
## phenoData
## sampleNames: x0001 x0002 ... x0090 (90 total)
## varLabels: age sex
## varMetadata: labelDescription
## featureData
## featureNames: Adiponectin_ok Alpha1AntitrypsinAAT_ok ...
## VitaminDBindingProte_ok (47 total)
## fvarLabels: chr start end
## fvarMetadata: labelDescription
## experimentData: use 'experimentData(object)'
## Annotation:
The association analysis between exposures and proteome is also done using association
.
mds <- createMultiDataSet()
mds <- add_eset(mds, brge_prot, dataset.type ="proteome")
mds <- add_exp(mds, brge_expo)
prot <- association(mds, formula=~Sex+Age,
expset = "exposures", omicset = "proteome")
The tableHits
indicates that no association was found between the 47 proteins and the exposures.
tableHits(prot, th=0.001)
## exposure hits
## Ben_p Ben_p 0
## Ben_t1 Ben_t1 0
## Ben_t2 Ben_t2 0
## Ben_t3 Ben_t3 0
## BPA_p BPA_p 0
## BPA_t1 BPA_t1 0
## BPA_t3 BPA_t3 0
## NO2_p NO2_p 0
## NO2_t1 NO2_t1 1
## NO2_t2 NO2_t2 0
## NO2_t3 NO2_t3 0
## PCB118 PCB118 0
## PCB138 PCB138 0
## PCB153 PCB153 0
## PCB180 PCB180 0
This is also seen in the Manhattan plot for proteins that can be obtained from plotAssociation
.
gridExtra::grid.arrange(
plotAssociation(prot, rid="Ben_p", type="protein") +
ggplot2::ggtitle("Proteome - Cd Association") +
ggplot2::geom_hline(yintercept = 1, color = "LightPink"),
plotAssociation(prot, rid="NO2_p", type="protein") +
ggplot2::ggtitle("Proteome - Cotinine Association") +
ggplot2::geom_hline(yintercept = 1, color = "LightPink"),
ncol=2
)
NOTE: A real Manhattan plot can be draw with plot
method for ResultSet
objects by setting the argument type
to "manhattan"
.
## used (Mb) gc trigger (Mb) max used (Mb)
## Ncells 8203328 438.2 12356621 660.0 12356621 660.0
## Vcells 22132499 168.9 378563032 2888.3 473198342 3610.3
omicRexposome
allows to study the relation between exposures and omic-features from another perspective, different from the association analyses. The integration analysis can be done, in omicRexposome
using multi canonical correlation analysis or using multiple co-inertia analysis. The first methods is implemented in R package PMA
(CRAN) and the second in omicade4
R package (Bioconductor). The two methods are encapsulated in the crossomics
method.
The differences between association
and crossomics
are that the first method test association between two complete data-sets, by removing the samples having missing values in any of the involved data-sets, and the second try to find latent relationships between two or more sets.
Hence, we need to explore the missing data in the exposome data-set. This can be done using the methods plotMissings
and tableMissings
from rexposome
R package.
library(rexposome)
plotMissings(brge_expo, set = "exposures")
From the plot we can see that more of the exposures have up to 25% of missing values. Hence the first step in the integration analysis is to avoid missing values. so, we perform a fast imputation on the exposures side:
brge_expo <- imputation(brge_expo)
crossomics
function expects to obtain the different data-sets in a single labelled-list, in the argument called list
. The argument method
from crossomics
function can be set to mcia
(for multiple co-inertia analysis) or to mcca
(for multi canonical correlation analysis).
The following code shows how to perform the integration of the exposome and the proteome. The method crossomics
request a MultiDataSet
object as input, containing the data-set to be integrated.
mds <- createMultiDataSet()
mds <- add_genexp(mds, brge_gexp)
mds <- add_eset(mds, brge_prot, dataset.type = "proteome")
mds <- add_exp(mds, brge_expo)
cr_mcia <- crossomics(mds, method = "mcia", verbose = TRUE)
cr_mcia
## Object of class 'ResultSet'
## . created with: crossomics
## . sva:
## . method: mcia ( omicade4 )
## . #results: 1 ( error: 0 )
## . featureData: 3
## . expression: 67528x11
## . proteome: 47x3
## . exposures: 15x12
As can be seen, crossomics
returns an object of class ResultSet
. In the integration process, the different data-sets are subset by common samples. This is done taking advantage of MultiDataSet
capabilities.
The same is done when method is set to mcca
.
cr_mcca <- crossomics(mds, method = "mcca", permute=c(4, 2))
cr_mcca
We used an extra argument (permute
) into the previous call to crossomics
using multi canonical correlation analysis. This argument allows to set the internal argument corresponding to permutations
and iterations
, that are used to tune-up internal parameters.
When a ResultSet
is generated using crossomics
the methods plotHits
, plotLambda
and plotAssociation
can NOT be used. But the plotIntegration
will help us to understand what was done. This method allows to provide the colors to be used on the plots:
colors <- c("green", "blue", "red")
names(colors) <- names(mds)
The graphical representation of the results from a multiple co-inertia analysis is a composition of four different plots.
plotIntegration(cr_mcia, colors=colors)
The first plot (first row, first column) is the samples space. It illustrates how the different data-sets are related in terms of intra-sample variability (each data-set has a different color). The second plot (first row, second column) shows the feature space. The features of each set are drawn on the same components so the relation between each data-set can be seen (the features are colored depending of the set were they belong).
The third plot (second row, first column) shows the inertia of each component. The two first plots are drawn on the first and second component. Finally, the fourth plot shows the behavior of the data-sets.
A radar plots is obtained when plotIntegration
is used on a ResultSet
created though multi canonical correlation analysis.
plotIntegration(cr_mcca, colors=colors)
This plot shows the features of the three data-sets in the same 2D space.The relation between the features can be understood by proximity. This means that the features that clusters, or that are in the same quadrant are related and goes in a different direction than the features in the other quadrants.
rm(cr_mcia, cr_mcca)
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## tzcode source: system (glibc)
##
## attached base packages:
## [1] stats graphics grDevices utils datasets methods base
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## [1] rexposome_1.22.0 MultiDataSet_1.28.0 omicRexposome_1.22.0
## [4] Biobase_2.60.0 BiocGenerics_0.46.0 BiocStyle_2.28.0
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## [7] rpart_4.1.19 lifecycle_1.0.3
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