--- title: " Vignette illustrating the use of MOFA on the CLL data" author: "Britta Velten and Ricard Argelaguet" output: BiocStyle::html_document: toc: true package: MOFA vignette: > %\VignetteIndexEntry{MOFA: applications to a multi-omics data set of CLL patients} %\VignetteEngine{knitr::rmarkdown} %\VignetteEncoding{UTF-8} --- This vignette show how to use MOFA including initialization, training and down-stream analyses. For illustration we use the CLL data which is used in the MOFA publication. ```{r, warning=FALSE, message=FALSE} library(MultiAssayExperiment) library(MOFA) library(MOFAdata) ``` # Step 1: Load data and create MOFA object There are two options to input data to MOFA: * Option 1: base R approach using a list of matrices * Option 2: Bioconductor approach using the MultiAssayExperiment framework ## Option 1: base R approach If using the base R approach, you simply need to provide a list of matrices where features are rows and samples are columns. Importantly, the samples need to be aligned. Missing values/assays should be filled with NAs. ```{r} data("CLL_data") MOFAobject <- createMOFAobject(CLL_data) MOFAobject ``` ## Option 2: Bioconductor approach If using the Bioconductor approach, you need to provide or create a [MultiAssayExperiment](https://bioconductor.org/packages/release/bioc/html/MultiAssayExperiment.html) object and then use it to build the MOFA object. For example, starting from a list of matrices where features are rows and samples are columns, this can be easily constructed as follows: ```{r, warning=FALSE, message=FALSE} # Load data # import list with mRNA, Methylation, Drug Response and Mutation data. data("CLL_data") # check dimensionalities, samples are columns, features are rows lapply(CLL_data, dim) # Load sample metadata: Sex and Diagnosis data("CLL_covariates") head(CLL_covariates) # Create MultiAssayExperiment object mae_CLL <- MultiAssayExperiment( experiments = CLL_data, colData = CLL_covariates ) # Build the MOFA object MOFAobject <- createMOFAobject(mae_CLL) MOFAobject ``` ## Overview of training data The function `plotDataOverview` can be used to obtain an overview of the data stored in the object for training. For each sample it shows in which views data are available. The rows are the different views and columns are samples. Missing values are indicated by a grey bar. ```{r} plotDataOverview(MOFAobject) ``` # Step 2: Fit the MOFA model The next step is to fit the model. This part of the pipeline is implemented in Python, so first of all make sure you have the corresponding package installed (see installation instructions and read the FAQ if you have problems). ## Define options ### Define data options The most important options the user needs to define are: * **scaleViews**: logical indicating whether to scale views to have unit variance. As long as the scale of the different data sets is not too high, this is not required. Default is `FALSE`. * **removeIncompleteSamples**: logical indicating whether to remove samples that are not profiled in all omics. The model can cope with missing assays, so this option is not required. Default is `FALSE`. ```{r} DataOptions <- getDefaultDataOptions() DataOptions ``` ### Define model options Next, we define model options. The most important are: * **numFactors**: number of factors (default is 0.5 times the number of samples). By default, the model will only remove a factor if it explains exactly zero variance in the data. You can increase this threshold on minimum variance explained by setting `TrainOptions$dropFactorThreshold` to a value higher than zero. * **likelihoods**: likelihood for each view. Usually we recommend gaussian for continuous data, bernoulli for binary data and poisson for count data. By default, the model tries to guess it from the data. * **sparsity**: do you want to use sparsity? This makes the interpretation easier so it is recommended (Default is `TRUE`). ```{r} ModelOptions <- getDefaultModelOptions(MOFAobject) ModelOptions$numFactors <- 25 ModelOptions ``` ### Define training options Next, we define training options. The most important are: * **maxiter**: maximum number of iterations. Ideally set it large enough and use the convergence criterion `TrainOptions$tolerance`. * **tolerance**: convergence threshold based on change in the evidence lower bound. For an exploratory run you can use a value between 1.0 and 0.1, but for a "final" model we recommend a value of 0.01. * **DropFactorThreshold**: hyperparameter to automatically learn the number of factors based on a minimum variance explained criteria. Factors explaining less than `DropFactorThreshold` fraction of variation in all views will be removed. For example, a value of 0.01 means that factors that explain less than 1\% of variance in all views will be discarded. By default this it zero, meaning that all factors are kept unless they explain no variance at all. ```{r} TrainOptions <- getDefaultTrainOptions() # Automatically drop factors that explain less than 2% of variance in all omics TrainOptions$DropFactorThreshold <- 0.02 TrainOptions$seed <- 2017 TrainOptions ``` ## Prepare MOFA `prepareMOFA` internally performs a set of sanity checks and fills the `DataOptions`, `TrainOptions` and `ModelOptions` slots of the `MOFAobject` ```{r} MOFAobject <- prepareMOFA( MOFAobject, DataOptions = DataOptions, ModelOptions = ModelOptions, TrainOptions = TrainOptions ) ``` Optionally, we can choose to regress out some (technical) covariates before training, using a simple linear model. For example, here we can choose to remove the effect of sex. Ideally, all undesired sources of variation should be removed a priori from the model. The reason ebing that, if strong technical factors exist, the model will "focus" on capturing the variability driven by the technical factors, and small sources of biological variability could be missed. (Note: uncomment and running the function below will lead to a slight modification of the results) ```{r} # MOFAobject <- regressCovariates( # object = MOFAobject, # views = c("Drugs","Methylation","mRNA"), # covariates = MOFAobject@InputData$Gender # ) ``` ## Run MOFA Now we are ready to train the `MOFAobject`, which is done with the function `runMOFA`. This step can take some time (around 15 min with default parameters). For illustration we provide an existing trained `MOFAobject`. IMPORTANT NOTE: The software has evolved since the original publication and the results are not 100% reproducible with the last versions. Yet, the output should be very similar (if not improved) to the pre-existent model. ```{r, eval=FALSE} MOFAobject <- runMOFA(MOFAobject) ``` ```{r} # Loading an existing trained model filepath <- system.file("extdata", "CLL_model.hdf5", package = "MOFAdata") MOFAobject <- loadModel(filepath, MOFAobject) MOFAobject ``` # Step 3: Analyse a trained MOFA model After training, we can explore the results from MOFA. Here we provide a semi-automated pipeline to disentangle and characterize all the identified sources of variation (the factors). **Part 1: Disentangling the heterogeneity** Calculation of variance explained by each factor in each view. This is probably the most important plot that MOFA generates, as it summarises the entire heterogeneity of the dataset in a single figure. Here we can see in which view a factor explains variation which can guide further characterisation of the factors by investigating the weights in those views. **Part 2: Characterization of individual factors** * Inspection of top features with highest loadings: the loading is a measure of feature importance, so features with high loading are the ones driving the heterogeneity captured by the factor. * Feature set enrichment analysis (where set annotations are present, e.g. gene sets for mRNA views). * Ordination of samples by factors to reveal clusters and/or gradients: this is similar to what is traditionally done with Principal Component Analysis or t-SNE. Other analyses, including imputation of missing values and clustering of samples are also available. See below for a short illustration of these functionalities. In addition, the factors can be used in further analyses, for example as predictors, e.g. for predicting clinical outcome or classifying patients, or to control for unwanted sources of variation. Vignettes illustrating this are coming soon. ## Part 1: Disentangling the heterogeneity: calculation of variance explained by each factor in each view This is done by `calculateVarianceExplained` (to get the numerical values) and `plotVarianceExplained` (to get the plot). The resulting figure gives an overview of which factors are active in which view(s). If a factor is active in more than one view, this means that is capturing shared signal (co-variation) between features of different data modalities. Here, for example Factor 1 is active in all data modalities, while Factor 4 is specific to mRNA. ```{r} # Calculate the variance explained (R2) per factor in each view r2 <- calculateVarianceExplained(MOFAobject) r2$R2Total # Variance explained by each factor in each view head(r2$R2PerFactor) # Plot it plotVarianceExplained(MOFAobject) ``` ## Part 2: Characterisation of individual factors ### Inspection of top weighted features in the active views To get an overview of the weights across all factors in a given view you can use the `plotWeightsHeatmap` function. For example, here we plot all weights from all factors in the Mutations data: ```{r} plotWeightsHeatmap( MOFAobject, view = "Mutations", factors = 1:5, show_colnames = FALSE ) ``` We observe that Factors 1 and 2 have large non-zero weights. To explore a given factor in more detail we can plot all weights for a single factor using the `plotWeights` function. For example, here we plot all weights from Factor 1 in the Mutation data. With `nfeatures` we can set how many features should be labelled (`manual` let's you specify feautres manually to be labelled in the plot.) ```{r} plotWeights( MOFAobject, view = "Mutations", factor = 1, nfeatures = 5 ) plotWeights( MOFAobject, view = "Mutations", factor = 1, nfeatures = 5, manual = list(c("BRAF"),c("MED12")), color_manual = c("red","blue") ) ``` Features with large (absolute) weight on a given factor follow the pattern of covariation associated with the factor. In our case, this reveals a strong link to the IGHV status, hence recovering an important clinical marker in CLL (see our paper for details on the biological interpretation.) Note that the sign of the weight can only be interpreted relative to the signs of other weights and the factor values. If you are only interested in looking at only the top features you can use the `plotTopWeights` function. For example, here we plot the mutations with largest loadings on Factor 1. The sign on the right indicates the direction of the loading (positive/negative). ```{r} plotTopWeights( MOFAobject, view="Mutations", factor=1 ) ``` Again, features with large weight in a given factor means that they follow the pattern of covariation associated with the factor. For example, here the factor is associated with the B-cell of tumour's origin, consistent with a large weight on the IGHV status (see our manuscript for more details). From the previous plots, we can clearly see that Factor 1 is associated to IGHV status. As the variance decomposition above told us that this factor is also relevant on all the other data modalities we can investigate its weights on other modalities, e.g. mRNA, to make connections of the IGHV-linked axes of variation to other molecular layers. ```{r} plotTopWeights( MOFAobject, view = "mRNA", factor = 1 ) ``` Finally, instead of looking at an "abstract" weight, it is useful to observe the coordinated heterogeneity of the top features in the original data. This can be done using the `plotDataHeatmap` function. In this plot samples (in rows) are ordered according to their value on the factor (here Factor 1). Here, this shows clear patterns of the samples' gene expression in the 20 top weighted genes along the factor. ```{r} plotDataHeatmap( MOFAobject, view = "mRNA", factor = 1, features = 20, show_rownames = FALSE ) ``` ### Feature set enrichment analysis in the active views Sometimes looking at the loadings of single features can be challenging, and often the combination of signal from functionally related sets of features (i.e. gene ontologies) is required. Here we implemented a function for feature set enrichment analysis method (`runEnrichmentAnalysis`) derived from the [PCGSE package](https://cran.r-project.org/web/packages/PCGSE/index.html). The input of this function is a MOFA trained model (MOFAmodel), the factors for which to perform feature set enrichment (a character vector), the feature sets (a binary matrix) and a set of options regarding how the analysis should be performed, see also documentation of `runEnrichmentAnalysis` We illustrate the use of this function using the [reactome](http://reactome.org) annotations, which are contained in the package. Depending on your data other gene or feature sets might be useful and you can prepare your customized feature sets and specify it using the `feature.sets` argument of the function. ```{r} # Load reactome annotations data("reactomeGS") # binary matrix with feature sets in rows and features in columns # perform enrichment analysis gsea <- runEnrichmentAnalysis( MOFAobject, view = "mRNA", feature.sets = reactomeGS, alpha = 0.01 ) ``` The next step is to visualise the results of the Gene Set Enrichment Analysis. There are several ways: (a) Plot the number of enriched gene sets per factor ```{r} plotEnrichmentBars(gsea, alpha=0.01) ``` From this we find enriched at a FDR of 1% gene sets on Factors 3-6 and 8. To look into which gene sets these are we can choose a factor of interest and visualize the most enriched gene sets as follows: (b) Plot the top enriched pathways for every factor ```{r} interestingFactors <- 4:5 fseaplots <- lapply(interestingFactors, function(factor) { plotEnrichment( MOFAobject, gsea, factor = factor, alpha = 0.01, max.pathways = 10 # The top number of pathways to display ) }) cowplot::plot_grid(fseaplots[[1]], fseaplots[[2]], ncol = 1, labels = paste("Factor", interestingFactors)) ``` This shows us that Factor 4 is capturing variation related to immune response (possibly due to T-cell contamination of the samples) and Factor 5 is related to differences in stress response, as discussed in our paper. ## Ordination of samples by factors to reveal clusters and gradients in the sample space Samples can be visualized along factors of interest using the `plotFactorScatter` function. We can use features included in the model (such as IGHV or trisomy12) to color or shape the samples by. Alternatively, external covariates can also be used for this purpose. ```{r} plotFactorScatter( MOFAobject, factors = 1:2, color_by = "IGHV", # color by the IGHV values that are part of the training data shape_by = "trisomy12" # shape by the trisomy12 values that are part of the training data ) ``` Here we find again a clear separation of samples based on their IGHV status (color) along Factor 1 and by the absence or prescence of trisomy 12 (shape) along Factor 2 as indicated by the corresponding factor weights in the Mutations view. An overview of pair-wise sctterplots for all or a subset of factors is produced by the `plotFactorScatters` function ```{r} plotFactorScatters( MOFAobject, factors = 1:3, color_by = "IGHV" ) ``` A single factor can be visualised using the `plotFactorBeeswarm` function ```{r} plotFactorBeeswarm( MOFAobject, factors = 1, color_by = "IGHV" ) ``` ## Customized analysis For customized exploration of weights and factors, you can directly fetch the variables from the model using 'get' functions: `getWeights`, `getFactors` and `getTrainData`: ```{r} MOFAweights <- getWeights( MOFAobject, views = "all", factors = "all", as.data.frame = TRUE # if TRUE, it outputs a long dataframe format. If FALSE, it outputs a wide matrix format ) head(MOFAweights) ``` ```{r} MOFAfactors <- getFactors( MOFAobject, factors = c(1,2), as.data.frame = FALSE # if TRUE, it outputs a long dataframe format. If FALSE, it outputs a wide matrix format ) head(MOFAfactors) ``` ```{r} MOFAtrainData <- getTrainData( MOFAobject, as.data.frame = TRUE, views = "Mutations" ) head(MOFAtrainData) ``` # Further functionalities ## Prediction of views With the `predict` function, full views can be predicted based on the MOFA model with all or a subset of factors. ```{r} predictedDrugs <- predict( MOFAobject, view = "Drugs", factors = "all" )[[1]] # training data (incl. missing values) drugData4Training <- getTrainData(MOFAobject, view="Drugs")[[1]] pheatmap::pheatmap(drugData4Training[1:40,1:20], cluster_rows = FALSE, cluster_cols = FALSE, show_rownames = FALSE, show_colnames = FALSE) # predicted data pheatmap::pheatmap(predictedDrugs[1:40,1:20], cluster_rows = FALSE, cluster_cols = FALSE, show_rownames = FALSE, show_colnames = FALSE) ``` ## Imputation of missing observations With the `impute` function all missing values are imputed based on the MOFA model. The imputed data is then stored in the `ImputedData slot` of the MOFAobject and can be accessed via the `getImputedData` function. ```{r} MOFAobject <- impute(MOFAobject) imputedDrugs <- getImputedData(MOFAobject, view="Drugs")[[1]] # training data (incl. missing values) pheatmap::pheatmap(drugData4Training[1:40,1:20], cluster_rows = FALSE, cluster_cols = FALSE, show_rownames = FALSE, show_colnames = FALSE) # imputed data pheatmap::pheatmap(imputedDrugs[1:40,1:20], cluster_rows = FALSE, cluster_cols = FALSE, show_rownames = FALSE, show_colnames = FALSE) ``` ## Clustering of samples based on latent factors Samples can be clustered according to their values on some or all latent factors using the `clusterSamples` function. Clusters can for example be visualised using the `plotFactorScatters` function ```{r} set.seed(1234) clusters <- clusterSamples( MOFAobject, k = 2, # Number of clusters for the k-means function factors = 1 # factors to use for the clustering ) plotFactorScatter( MOFAobject, factors = 1:2, color_by = clusters ) ``` # SessionInfo ```{r} sessionInfo() ```