A pseudobulk sample is formed by aggregating the expression values from a group of cells from the same individual. The cells are typically grouped by clustering or cell type assignment. Individual refers to the experimental unit of replication (e.g., the individual mice or patients).
Forming pseudobulk samples is important to perform accurate differential expression analysis. Cells from the same individual are more similar to each other than to cells from another individual. This means treating each cell as an independent sample leads to underestimation of the variance and misleadingly small p-values. Working on the level of pseudobulks ensures reliable statistical tests because the samples correspond to the units of replication.
We can use pseudobulks for example to find the expression changes between two conditions for one cell type.
I load a SingleCellExperiment
object containing gene expression counts from eight Lupus patient before and after interferon beta stimulation. The creator of the dataset has already annotated the cell types and if cell is a singlet.
library(SummarizedExperiment)
library(SingleCellExperiment)
sce <- muscData::Kang18_8vs8()
#> see ?muscData and browseVignettes('muscData') for documentation
#> loading from cache
# Keep only genes with more than 5 counts
sce <- sce[rowSums(counts(sce)) > 5,]
colData(sce)
#> DataFrame with 29065 rows and 5 columns
#> ind stim cluster cell multiplets
#> <integer> <factor> <integer> <factor> <factor>
#> AAACATACAATGCC-1 107 ctrl 5 CD4 T cells doublet
#> AAACATACATTTCC-1 1016 ctrl 9 CD14+ Monocytes singlet
#> AAACATACCAGAAA-1 1256 ctrl 9 CD14+ Monocytes singlet
#> AAACATACCAGCTA-1 1256 ctrl 9 CD14+ Monocytes doublet
#> AAACATACCATGCA-1 1488 ctrl 3 CD4 T cells singlet
#> ... ... ... ... ... ...
#> TTTGCATGCTAAGC-1 107 stim 6 CD4 T cells singlet
#> TTTGCATGGGACGA-1 1488 stim 6 CD4 T cells singlet
#> TTTGCATGGTGAGG-1 1488 stim 6 CD4 T cells ambs
#> TTTGCATGGTTTGG-1 1244 stim 6 CD4 T cells ambs
#> TTTGCATGTCTTAC-1 1016 stim 5 CD4 T cells singlet
The pseudobulk
functions emulates the group_by
and summarize
pattern popularized by the tidyverse
.
You provide the columns from the colData
that you want to use for grouping the data (akin to group_by
) and named arguments specifiying how you summarize the remaining columns (akin to summarize
). Using the aggregation_functions
you can set how the assay
’s and reducedDim
’s are summarized with a named list.
Here, I create a pseudobulk sample for each patient, condition, and cell type. This means for example that the counts of the 119 B-cells from patient 101 in the control condition are summed to one column in the reduced dataset.
The first argument is a SingleCellExperiment
object. The group_by
argument uses vars()
to quote the grouping columns The fraction_singlet
and n_cells
arguments demonstrate how additional columns from the colData
are summarized. For fraction_singlet
, I use the fact that mean
automatically coerces a boolean vector to zeros and ones and n_cells
demonstrates the n()
function that returns the number of cells that are aggregated for each group.
library(glmGamPoi)
reduced_sce <- pseudobulk(sce, group_by = vars(ind, condition = stim, cell),
fraction_singlet = mean(multiplets == "singlet"), n_cells = n())
#> Aggregating assay 'counts' using 'rowSums2'.
#> Aggregating reducedDim 'TSNE' using 'rowMeans2'.
colData(reduced_sce)
#> DataFrame with 132 rows and 5 columns
#> ind condition cell fraction_singlet
#> <integer> <factor> <factor> <numeric>
#> 107.ctrl.CD4 T cells 107 ctrl CD4 T cells 0.793970
#> 1016.ctrl.CD14+ Monocytes 1016 ctrl CD14+ Monocytes 0.800434
#> 1256.ctrl.CD14+ Monocytes 1256 ctrl CD14+ Monocytes 0.831557
#> 1488.ctrl.CD4 T cells 1488 ctrl CD4 T cells 0.867205
#> 1039.ctrl.Dendritic cells 1039 ctrl Dendritic cells 0.900000
#> ... ... ... ... ...
#> 1256.stim.Megakaryocytes 1256 stim Megakaryocytes 0.708333
#> 1244.stim.Megakaryocytes 1244 stim Megakaryocytes 0.764706
#> 107.stim.CD8 T cells 107 stim CD8 T cells 0.652174
#> 101.stim.Megakaryocytes 101 stim Megakaryocytes 1.000000
#> 1256.stim.NA 1256 stim NA 0.000000
#> n_cells
#> <integer>
#> 107.ctrl.CD4 T cells 199
#> 1016.ctrl.CD14+ Monocytes 461
#> 1256.ctrl.CD14+ Monocytes 469
#> 1488.ctrl.CD4 T cells 1363
#> 1039.ctrl.Dendritic cells 10
#> ... ...
#> 1256.stim.Megakaryocytes 24
#> 1244.stim.Megakaryocytes 17
#> 107.stim.CD8 T cells 23
#> 101.stim.Megakaryocytes 9
#> 1256.stim.NA 1
You can simulate the pseudobulk sample generation and check if you are using the correct arguments by calling dplyr::group_by
. Note that the order of the output differs because group_by
automatically sorts the keys.
library(dplyr, warn.conflicts = FALSE)
colData(sce) %>%
as_tibble() %>%
group_by(ind, condition = stim, cell) %>%
summarize(n_cells = n(), .groups = "drop")
#> # A tibble: 132 × 4
#> ind condition cell n_cells
#> <int> <fct> <fct> <int>
#> 1 101 ctrl B cells 119
#> 2 101 ctrl CD14+ Monocytes 247
#> 3 101 ctrl CD4 T cells 341
#> 4 101 ctrl CD8 T cells 99
#> 5 101 ctrl Dendritic cells 25
#> 6 101 ctrl FCGR3A+ Monocytes 96
#> 7 101 ctrl Megakaryocytes 16
#> 8 101 ctrl NK cells 84
#> 9 101 stim B cells 151
#> 10 101 stim CD14+ Monocytes 302
#> # ℹ 122 more rows
With the reduced data, we can conduct differential expression analysis the same way we would analyze bulk RNA-seq data (using tools like DESeq2
and edgeR
).
For example we can find the genes that change most upon treatment in the B-cells
# Remove NA's
reduced_sce <- reduced_sce[,!is.na(reduced_sce$cell)]
# Use DESeq2's size factor calculation procedure
fit <- glm_gp(reduced_sce, design = ~ condition*cell + ind, size_factor = "ratio", verbose = TRUE)
#> Calculate Size Factors (ratio)
#> Make initial dispersion estimate
#> Make initial beta estimate
#> Estimate beta
#> Estimate dispersion
#> Fit dispersion trend
#> Shrink dispersion estimates
#> Estimate beta again
res <- test_de(fit, contrast = cond(cell = "B cells", condition = "stim") - cond(cell = "B cells", condition = "ctrl"))
A volcano plot gives a quick impression of the overall distribution of the expression changes.
library(ggplot2, warn.conflicts = FALSE)
ggplot(res, aes(x = lfc, y = - log10(pval))) +
geom_point(aes(color = adj_pval < 0.01), size = 0.5)
Originally, glmGamPoi
’s API encouraged forming pseudobulks after fitting the model (i.e., within test_de()
). The advantage was that this reduced the number of functions. Yet, internally glmGamPoi
basically threw away the original fit and re-ran it on the aggregated data. This meant that computation time was wasted. Thus the original approach forming the pseudobulk in test_de
is now deprecated in favor of first calling pseudobulk()
and then proceed by calling glm_gp()
and test_de()
on the aggregated data.