In this document, the user is presented with an analysis that DepecheR has been written to perform. There are lots of tweaks to this general outline, so the user is encouraged to read the help files for each function individually in addition. In cases where bugs are identified, feedback is most welcome, primarily on the github site github.com/theorell/DepecheR. Now let us get started.
This is how to install the package, if that has not already been done:
if(!requireNamespace("BiocManager", quietly = TRUE))
install.packages("BiocManager")
BiocManager::install("DepecheR")
The data used in this example is a semi-simulated dataset, consisting of 1000 cytotoxic lymphocytes from each of 20 individuals. These have been categorized into two groups, and after this, alterations have been added to the sizes of some cell populations in both groups. This means that the groups can be separated based onthe sizes of certain cell types in the data. And this excersize will show how to identify these, and tell us what markers that define the separating cell types in question.
Importantly, DepecheR does not provide any pre-processing tools, such as for compensation/spectral unmixing of flow cytometry files. The clustering function does have an internal algorithm to detect data with extreme tails, but this does not circumvent the need to transform flow- or mass cytometry data. This can be done using either commercially available software or with R packages, such as Biocpkg(“flowSpecs”), Biocpkg(“flowCore”) or Biocpkg(“flowVS”).
library(DepecheR)
data('testData')
str(testData)
## 'data.frame': 20000 obs. of 16 variables:
## $ ids : int 1 1 1 1 1 1 1 1 1 1 ...
## $ SYK : num 11.2 21.3 23.7 22.1 24.8 ...
## $ FcER1g: num 15.4 19.8 18.7 17.9 28.2 ...
## $ CD16 : num 27.4 23.7 17.9 19.2 19.8 ...
## $ CD57 : num 6.45 5.55 9.65 17.41 86.38 ...
## $ EAT.2 : num 21.2 18.2 23.6 39.6 25.9 ...
## $ CD4 : num 80.7 82.6 88.2 89.6 12.7 ...
## $ TCRgd : num 17.5 21.6 20.2 29 14.3 ...
## $ CD8 : num 21.2 17.6 16.4 -11.4 78.3 ...
## $ iCD3 : num 88.9 86.7 82.7 90.6 87.6 ...
## $ NKG2C : num 21.2 56.3 36.5 62.9 21.5 ...
## $ CD2 : num 43.2 64.6 73.6 14.7 75.6 ...
## $ CD45RO: num 34.9 34.1 27.3 59.5 22.5 ...
## $ CD3 : num 83.3 90.7 91.5 103.4 76.2 ...
## $ CD56 : num 21.1 39.7 28.3 15.5 69.5 ...
## $ label : int 0 0 0 0 0 0 0 0 0 0 ...
As can be noted here, the expected input format is either a dataframe or a matrix with cells as rows and markers/variables as columns. This is in accordance with the .fcs file convention. In this case, however, the different samples (coming from donors) should be added to the same dataframe, and a donor column should specify which cells that belong to which donor. If you have .fcs files, you can do this conversion easily using the “flowSet2LongDf” function in Biocpkg(“flowSpecs”).
With the depeche clustering function, all necessary scaling and parameter selection is performed under the hood, so all we have to do, when we have the file of interest in the right format, is to run the function on the variables that we want to cluster on.
testDataDepeche <- depeche(testData[, 2:15])
## [1] "Files will be saved to ~/Desktop"
## [1] "As the dataset has less than 100 columns, peak centering is applied."
## [1] "Set 1 with 7 iterations completed in 14 seconds."
## [1] "Set 2 with 7 iterations completed in 6 seconds."
## [1] "Set 3 with 7 iterations completed in 6 seconds."
## [1] "The optimization was iterated 21 times."
str(testDataDepeche)
## List of 4
## $ clusterVector : int [1:20000] 2 2 2 2 6 3 5 2 1 1 ...
## $ clusterCenters : num [1:8, 1:14] 0 0 0 40.2 0 ...
## ..- attr(*, "dimnames")=List of 2
## .. ..$ : chr [1:8] "1" "2" "3" "4" ...
## .. ..$ : chr [1:14] "SYK" "FcER1g" "CD16" "CD57" ...
## $ essenceElementList:List of 8
## ..$ 1: chr [1:3] "CD4" "NKG2C" "CD45RO"
## ..$ 2: chr [1:5] "CD4" "iCD3" "NKG2C" "CD2" ...
## ..$ 3: chr [1:3] "CD57" "CD8" "CD2"
## ..$ 4: chr [1:10] "SYK" "FcER1g" "CD16" "CD57" ...
## ..$ 5: chr [1:3] "CD57" "CD8" "CD45RO"
## ..$ 6: chr [1:4] "CD57" "CD8" "CD2" "CD56"
## ..$ 7: chr [1:6] "SYK" "FcER1g" "iCD3" "CD2" ...
## ..$ 8: chr [1:4] "TCRgd" "CD2" "CD45RO" "CD56"
## $ penaltyOptList :List of 2
## ..$ :'data.frame': 1 obs. of 2 variables:
## .. ..$ bestPenalty: num 16
## .. ..$ k : num 30
## ..$ :'data.frame': 11 obs. of 2 variables:
## .. ..$ ARI : num [1:11] 0.59 0.581 0.683 0.689 0.857 ...
## .. ..$ nClust: num [1:11] 29.4 28 27.1 24.3 20.4 ...
As can be seen above, the output from the function is a relatively complex list. If the names of each list element is not suficiently self explanatory, see (?depeche) for information about each slot.
Two graphs are part of the output from the depeche function.
This graph shows how internally reproducible the results were for each of the tested penalties. An Adjusted Rand Index of 1 shows that if any random subset of observations is clustered two times, each observation will be assigned to the same cluster both times. Conversely, an Adjusted Rand Index of 0 indicates the opposite, i.e. totally random distribution. The adjustment in “Adjusted” Rand index takes the divering probabilities of ending up with a high or low overlap in the special cases of very few and very many clusters into consideration.
This graph shows in a heatmap format where the cluster center is located for each of the markers that are defined for the cluster in question. A light color indicates a high expression, whereas a dark color indicates low or absent expression. Grey color, on the other hand, indicates that the cluster in question did not contribute to defining the cluster in question. In some cases, the results might seem strange, as a cluster might have an expression very close to the center of the full dataset, but this expression still defined the cluster. This is due to an internal, and for stability reasons necessary, effect of the algotihm: a specific penalty will have a larger effect on a cluster with fewer observations, than on a cluster with many observations.
To be able to visualize the results, we need to generate a two-dimensional representation of the data used to generate the depeche clustering. Any sutiable method, such as tSNE or UMAP can be used for this purpose. I would today use uwot::umap, mainly as it in its R implementation is considerably faster than tSNE, but we will keep the tSNE here, as it well represents the data.
library(Rtsne)
testDataSNE <- Rtsne(testData[,2:15], pca=FALSE)
Now, we want to evaluate how the different clusters are distributed on the 2D representation. To do this, we need to generate a color vector from the cluster vector in the testDataDepeche. This cluster vector is then overlayed over the tSNE, and to make things easier to interpret, a separate legend is included as well. The reason that the legend is in a separate plot is for making it easier to use the plots for publication purposes. For file size reasons, it has namely been necessary to use PNG and not PDF for the plot files.
NB! The resolution of the files normally generated by DepecheR is considerably higher than in this vinjette, due to size restrictions.
dColorPlot(colorData = testDataDepeche$clusterVector, xYData = testDataSNE$Y,
colorScale = "dark_rainbow", plotName = "Cluster")
## png
## 2
Here, we once again use the dColorPlot function, with different settings. Note that titles are included in this case. As they are then becoming embedded in the png picture, this is not the standard, for publication reasons. It is also worth noting, that nothing is printed to screen, but rather all graphics are saved as separate files. This is done to save some computational time and effort.
dColorPlot(colorData = testData[2], xYData = testDataSNE$Y)
## png
## 2
Now, we are getting into separating the groups from each other. The first thing we want to do is to visually compare the densities of the groups. This is done in the following way. First, the density for all events are plotted. This is followed by plotting of the first and second group of individuals, but keeping the density contours from the full dataset.
densContour <- dContours(testDataSNE$Y)
dDensityPlot(xYData = testDataSNE$Y, plotName = 'All_events',
colorScale="purple3", densContour = densContour)
## png
## 2
#Here the data for the first group is plotted
dDensityPlot(xYData = testDataSNE$Y[testData$label==0,], plotName = 'Group_0',
colorScale="blue", densContour = densContour)
## png
## 2
#And here comes the second group
dDensityPlot(xYData = testDataSNE$Y[testData$label==1,], plotName = 'Group_1',
colorScale="red", densContour = densContour)
## png
## 2
Now, we have arrived at a crucial point: we are now going to see which clusters that separate the two groups from each other. There are three functions in the DepecheR package that can help us do this. The first one is the dResidualPlot.
dResidualPlot(
xYData = testDataSNE$Y, groupVector = testData$label,
clusterVector = testDataDepeche$clusterVector)
## png
## 2
This function shows the difference on a per-group/per-cluster basis. This means that it is non-statistical, and thus applicable even if the groups consist of only one or a few samples each. However, it cannot distinguish between a rare but very pronounced phenotype and a common difference: i.e., an individual donor can be responsible for the full difference noted. To circumvent this, and to get some statistical inferences, two other functions are available: the dWilcox and the dSplsda. These functions have identical input, but where the former performs a Wilcoxon rank-sum test (also called Mann-whitney U test) on a per-cluster basis and thus results in multiple comparisons, the latter (based on sparse projection to latent structures (aka partial least squares) discriminant analysis) instead identifies the angle through the multi-dimensional datacloud created by the individual donor frequencies in each cluster that most optimally separates the groups. It then internally checks how well the groups are separated along this vector, and plots the clusters that contribute to this separation with colors relative to how well the groups are separated. As this method is a sparse version of the method, it, like depeche, only identifies clusters that contribute robustly to separating the clusters, and has its internal tuning algorithm to define how the penalty term should be set. For both methods, there are paired alternatives. In this case, however, the data is not paired, and thus, the normal methods will be used. The standard use of the methods are:
dWilcoxResult <- dWilcox(
xYData = testDataSNE$Y, idsVector = testData$ids,
groupVector = testData$label, clusterVector = testDataDepeche$clusterVector)
sPLSDAObject <- dSplsda(xYData = testDataSNE$Y, idsVector = testData$ids,
groupVector = testData$label,
clusterVector = testDataDepeche$clusterVector)
## Saving 3 x 3 in image
## [1] "The separation of the datasets was perfect, with no overlap between
## the groups"
## [1] "Files were saved at /Users/jakthe/Labbet/GitHub/DepecheR/vignettes"
The object rendered by the dSplsda function is inherited from the mixOmics package. The object rendered by the dWilcox function is a matrix containing information about the cluster number, the median in each group, the Wilcoxon statistic, the p-value and a p-value corrected for multiple comparisons. In addition to the graphs, the dWilcox and the dSplsda functions also output result files. See ?dSplsda and ?dWilcox for more information.
When investigating the results from the sPLS-DA or the dWilcox analysis, it was clear that half of the clusters were highly significantly different between the groups in this case.
This function is especially useful to view the cluster distributions for specific clusters of interest, such as the significant clusters from the previousstep. dViolins serves as a compliment to the cluster center heatmap (see step 2). In this function, the sparsityMatrix from the depeche run is used. The function will in addition to producing all the graphs also produce a hierarchy of folders where the graphs are placed. EDIT 2019-09-12: This function currently does not support most CyTOF data, as the zero-peak is so dominant, which would make the interpretation of the plots impossible. This will be fixed in the near future, by reducing the negative population.
dViolins(testDataDepeche$clusterVector, inDataFrame = testData,
plotClusters = 3, plotElements = testDataDepeche$essenceElementList)
## [[1]]
## png
## 2
In this document, a typical analysis of a cytometry dataset is shown. There are however very many other possibilities with this package. One of the major ones is that it accuratly classifies scRNAseq data, and in that process reduces the complexity of the data up to 1000-fold, as very few transcripts actually define each cluster. For further information on how to do this, the reader is currently encouraged to read the publication connected to this package: https://journals.plos.org/plosone/article?id=10.1371/journal.pone.0203247.
sessionInfo()
## R version 4.2.0 RC (2022-04-19 r82224)
## Platform: x86_64-pc-linux-gnu (64-bit)
## Running under: Ubuntu 20.04.4 LTS
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## Matrix products: default
## BLAS: /home/biocbuild/bbs-3.15-bioc/R/lib/libRblas.so
## LAPACK: /home/biocbuild/bbs-3.15-bioc/R/lib/libRlapack.so
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## [5] LC_MONETARY=en_US.UTF-8 LC_MESSAGES=en_US.UTF-8
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## [9] LC_ADDRESS=C LC_TELEPHONE=C
## [11] LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=C
##
## attached base packages:
## [1] stats graphics grDevices utils datasets methods base
##
## other attached packages:
## [1] DepecheR_1.12.0 knitr_1.38 BiocStyle_2.24.0
##
## loaded via a namespace (and not attached):
## [1] ggrepel_0.9.1 Rcpp_1.0.8.3 lattice_0.20-45
## [4] tidyr_1.2.0 FNN_1.1.3 corpcor_1.6.10
## [7] snow_0.4-4 gtools_3.9.2 assertthat_0.2.1
## [10] digest_0.6.29 foreach_1.5.2 utf8_1.2.2
## [13] RSpectra_0.16-1 plyr_1.8.7 R6_2.5.1
## [16] ellipse_0.4.2 evaluate_0.15 ggplot2_3.3.5
## [19] pillar_1.7.0 gplots_3.1.3 rlang_1.0.2
## [22] gdata_2.18.0 jquerylib_0.1.4 gmodels_2.18.1
## [25] Matrix_1.4-1 rmarkdown_2.14 moments_0.14
## [28] rARPACK_0.11-0 BiocParallel_1.30.0 stringr_1.4.0
## [31] igraph_1.3.1 munsell_0.5.0 compiler_4.2.0
## [34] xfun_0.30 pkgconfig_2.0.3 htmltools_0.5.2
## [37] doSNOW_1.0.20 tidyselect_1.1.2 tibble_3.1.6
## [40] gridExtra_2.3 bookdown_0.26 codetools_0.2-18
## [43] matrixStats_0.62.0 viridisLite_0.4.0 fansi_1.0.3
## [46] crayon_1.5.1 dplyr_1.0.8 MASS_7.3-57
## [49] bitops_1.0-7 grid_4.2.0 jsonlite_1.8.0
## [52] gtable_0.3.0 lifecycle_1.0.1 DBI_1.1.2
## [55] magrittr_2.0.3 scales_1.2.0 KernSmooth_2.23-20
## [58] cli_3.3.0 stringi_1.7.6 reshape2_1.4.4
## [61] viridis_0.6.2 robustbase_0.95-0 bslib_0.3.1
## [64] ellipsis_0.3.2 generics_0.1.2 vctrs_0.4.1
## [67] RColorBrewer_1.1-3 iterators_1.0.14 mixOmics_6.20.0
## [70] tools_4.2.0 glue_1.6.2 DEoptimR_1.0-11
## [73] purrr_0.3.4 parallel_4.2.0 fastmap_1.1.0
## [76] yaml_2.3.5 colorspace_2.0-3 BiocManager_1.30.17
## [79] caTools_1.18.2 beanplot_1.3.1 sass_0.4.1