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This vignette shows how to use Signac with Seurat. There are three parts: Seurat, Signac and then visualization. We use an example PBMCs CITE-seq data set from 10X Genomics.
Start with the standard pre-processing steps for a Seurat object.
library(Seurat)
Download data from 10X Genomics.
dir.create("fls")
download.file("https://cf.10xgenomics.com/samples/cell-exp/3.0.0/pbmc_10k_protein_v3/pbmc_10k_protein_v3_filtered_feature_bc_matrix.h5",
destfile = "fls/pbmc_10k_protein_v3_filtered_feature_bc_matrix.h5")
Create a Seurat object, and then perform SCTransform normalization. Note:
# load dataset
= Read10X_h5(filename = "fls/pbmc_10k_protein_v3_filtered_feature_bc_matrix.h5")
E <- CreateSeuratObject(counts = E$`Gene Expression`, project = "pbmc")
pbmc
# run sctransform
<- SCTransform(pbmc)
pbmc
# optionally just normalize data pbmc <- NormalizeData(pbmc) pbmc <- FindVariableFeatures(pbmc)
# pbmc <- ScaleData(pbmc)
Perform dimensionality reduction by PCA and UMAP embedding. Note:
# These are now standard steps in the Seurat workflow for visualization and clustering
<- RunPCA(pbmc, verbose = FALSE)
pbmc <- RunUMAP(pbmc, dims = 1:30, verbose = FALSE)
pbmc <- FindNeighbors(pbmc, dims = 1:30, verbose = FALSE) pbmc
Load the package
require(SignacX)
Generate SignacX labels for the Seurat object. Note:
# Run Signac
<- Signac(pbmc, num.cores = 4)
labels = GenerateLabels(labels, E = pbmc) celltypes
Sometimes, training the neural networks takes a lot of time. To make Signac faster, we implemented SignacFast which uses an ensemble of pre-trained neural network models. Note:
# Run Signac
<- SignacFast(pbmc, num.cores = 12)
labels_fast = GenerateLabels(labels_fast, E = pbmc) celltypes_fast
B | MPh | TNK | Unclassified | |
---|---|---|---|---|
B | 550 | 0 | 0 | 0 |
MPh | 0 | 2178 | 0 | 0 |
TNK | 0 | 0 | 4914 | 0 |
Unclassified | 0 | 4 | 2 | 217 |
Now we can visualize the cell type classifications at many different levels: Immune and nonimmune
<- AddMetaData(pbmc, metadata = celltypes_fast$Immune, col.name = "immmune")
pbmc <- SetIdent(pbmc, value = "immmune")
pbmc png(filename = "fls/plot1_citeseq.png")
DimPlot(pbmc)
dev.off()
<- AddMetaData(pbmc, metadata = celltypes$L2, col.name = "celltypes")
pbmc <- SetIdent(pbmc, value = "celltypes")
pbmc png(filename = "fls/plot2_citeseq.png")
DimPlot(pbmc)
dev.off()
<- AddMetaData(pbmc, metadata = celltypes$CellTypes, col.name = "celltypes")
pbmc <- SetIdent(pbmc, value = "celltypes")
pbmc png(filename = "./fls/plot3_citeseq.png")
DimPlot(pbmc)
dev.off()
<- AddMetaData(pbmc, metadata = celltypes$CellTypes_novel, col.name = "celltypes_novel")
pbmc <- SetIdent(pbmc, value = "celltypes_novel")
pbmc png(filename = "./fls/plot4_citeseq.png")
DimPlot(pbmc)
dev.off()
<- AddMetaData(pbmc, metadata = celltypes$CellStates, col.name = "cellstates")
pbmc <- SetIdent(pbmc, value = "cellstates")
pbmc png(filename = "./fls/plot5_citeseq.png")
DimPlot(pbmc)
dev.off()
Identify differentially expressed genes between cell types.
<- SetIdent(pbmc, value = "celltypes")
pbmc
# Find markers for all clusters, and draw a heatmap
<- FindAllMarkers(pbmc, only.pos = TRUE, verbose = F, logfc.threshold = 1)
markers library(dplyr)
<- markers %>% group_by(cluster) %>% top_n(n = 5, wt = avg_logFC)
top5
png(filename = "./fls/plot9_citeseq.png", width = 640, height = 720)
DoHeatmap(pbmc, features = unique(top5$gene), angle = 90)
dev.off()
<- SetIdent(pbmc, value = "cellstates")
pbmc
# Find markers for all clusters, and draw a heatmap
<- FindAllMarkers(pbmc, only.pos = TRUE, verbose = F, logfc.threshold = 1)
markers <- markers %>% group_by(cluster) %>% top_n(n = 5, wt = avg_logFC)
top5
png(filename = "./fls/plot6_citeseq.png", width = 640, height = 720)
DoHeatmap(pbmc, features = unique(top5$gene), angle = 90)
dev.off()
Add protein expression information
"ADT"]] <- CreateAssayObject(counts = E$`Antibody Capture`[, colnames(E$`Antibody Capture`) %in%
pbmc[[colnames(pbmc)])
<- NormalizeData(pbmc, assay = "ADT", normalization.method = "CLR")
pbmc <- ScaleData(pbmc, assay = "ADT") pbmc
Identify differentially expressed proteins between clusters
DefaultAssay(pbmc) <- "ADT"
# Find protein markers for all clusters, and draw a heatmap
<- FindAllMarkers(pbmc, assay = "ADT", only.pos = TRUE, verbose = F)
adt.markers png(filename = "./fls/plot7_citeseq.png", width = 640, height = 720)
DoHeatmap(pbmc, features = unique(adt.markers$gene), angle = 90)
dev.off()
Save results
saveRDS(pbmc, file = "fls/pbmcs_signac_citeseq.rds")
saveRDS(celltypes, file = "fls/celltypes_citeseq.rds")
saveRDS(celltypes_fast, file = "fls/celltypes_fast_citeseq.rds")
## R version 4.0.3 (2020-10-10)
## Platform: x86_64-pc-linux-gnu (64-bit)
## Running under: Ubuntu 18.04.5 LTS
##
## Matrix products: default
## BLAS: /usr/lib/x86_64-linux-gnu/blas/libblas.so.3.7.1
## LAPACK: /usr/lib/x86_64-linux-gnu/lapack/liblapack.so.3.7.1
##
## locale:
## [1] LC_CTYPE=en_US.UTF-8 LC_NUMERIC=C
## [3] LC_TIME=en_US.UTF-8 LC_COLLATE=en_US.UTF-8
## [5] LC_MONETARY=en_US.UTF-8 LC_MESSAGES=en_US.UTF-8
## [7] LC_PAPER=en_US.UTF-8 LC_NAME=C
## [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
##
## loaded via a namespace (and not attached):
## [1] compiler_4.0.3 magrittr_2.0.1 formatR_1.7 htmltools_0.5.1.1
## [5] tools_4.0.3 yaml_2.2.1 stringi_1.5.3 rmarkdown_2.6
## [9] highr_0.8 knitr_1.30 stringr_1.4.0 digest_0.6.27
## [13] xfun_0.20 rlang_0.4.10 evaluate_0.14
These binaries (installable software) and packages are in development.
They may not be fully stable and should be used with caution. We make no claims about them.