Quick start of CytoTree

knitr::opts_chunk$set(echo = TRUE, cache = FALSE, eval = TRUE,
                      warning = TRUE, message = TRUE,
                      fig.width = 6, fig.height = 5)

Introduction

Although multidimensional single-cell-based flow and mass cytometry have been increasingly applied to microenvironmental composition and stem-cell research, integrated analysis workflows to facilitate the interpretation of experimental cytometry data remain underdeveloped. We present CytoTree, a comprehensive R package designed for the analysis and interpretation of flow and mass cytometry data. We applied CytoTree to mass cytometry and time-course flow cytometry data to demonstrate the usage and practical utility of its computational modules. CytoTree is a reliable tool for multidimensional cytometry data workflows and produces compelling results for trajectory construction and pseudotime estimation.

See the detailed tutorial of CytoTree, please visit Tutorial of CytoTree.

Overview of Workflow

The CytoTree package is developed to complete the majority of standard analysis and visualization workflow for FCS data. In CytoTree workflow, an S4 object in R is built to implement the statistical and computational approach, and all computational functionalities are integrated into one single channel which only requires a specified input data format. Computational functionalities of CytoTree can be divided into four main parts (Fig. 2.1): preprocessing, trajectory, analysis and visualization.

Figure 1 Workflow of CytoTree

Installation

GitHub

This requires the devtools package to be pre-installed first.

``` {r eval = FALSE}

If not already installed

install.packages("devtools") devtools::install_github("JhuangLab/CytoTree")

library(CytoTree)

The link of `CytoTree` on GitHub can be visited at https://github.com/JhuangLab/CytoTree.

### Bioconductor

This requires the `BiocManager` package to be pre-installed first, and make sure the version of Bioc is 3.12.

To install this package, start R (version "4.0") and enter:

``` {r eval = FALSE}

if (!requireNamespace("BiocManager", quietly = TRUE))
    install.packages("BiocManager")

BiocManager::install("CytoTree")

The link of CytoTree on Bioconductor can be visited at https://bioconductor.org/packages/CytoTree/.

Quick-start code

To run CytoTree, the first step is to build a CYT object. Here are the main functions in CytoTree. This figure describes the available functionalities: preprocessing, trajectory, analysis, visualization, and set operations. A short description (black font) and the corresponding function (blue font) are provided for each function. The CytoTree workflow begins with the reading of the FCS data. Compensation, filtration, concatenation, and normalization are included in the preprocessing part. A clean matrix after preprocessing is required to build a CYT object, and the analysis workflows of all other functionalities are all based on the CYT object. The trajectory module contains functions used to perform clustering and dimensionality reduction for cells. The analysis module is based on calculation results from the trajectory part. The visualization part includes functions to generate publication-quality plots from the CYT object. The set operations part includes a function for subsetting a CYT object based on user-defined cells or fetching meta information for clusters and cells during the analysis.

``` {r eval = TRUE}

Loading packages

suppressMessages({ library(CytoTree) })

Read fcs files

fcs.path <- system.file("extdata", package = "CytoTree") fcs.files <- list.files(fcs.path, pattern = '.FCS$', full = TRUE)

Using runExprsMerge for multip FCS files

Or using runExprsExtract for one single FCS file

fcs.data <- runExprsMerge(fcs.files, comp = FALSE, transformMethod = "none")

Build the CYT object

cyt <- createCYT(raw.data = fcs.data, normalization.method = "log")

See information

cyt

Running CytoTree in one line code

Run without dimensionality reduction steps

Run CytoTree as pipeline and visualize as tree

cyt <- cyt %>% runCluster() %>% processingCluster() %>% buildTree() plotTree(cyt)

Or you can run with dimensionality reduction steps

Run CytoTree as pipeline and visualize as tree

cyt <- cyt %>% runCluster() %>% processingCluster() %>% runFastPCA() %>% runTSNE() %>% runDiffusionMap() %>% runUMAP() %>% buildTree() plot2D(cyt, item.use = c("UMAP_1", "UMAP_2"))

Here we provied the running template of trajectory inference using CYT object is as follows:

``` {r eval = TRUE}

# Cluster cells by SOM algorithm
set.seed(1)
cyt <- runCluster(cyt)

# Processing Clusters
cyt <- processingCluster(cyt)

# This is an optional step
# run Principal Component Analysis (PCA)
cyt <- runFastPCA(cyt)

# This is an optional step
# run t-Distributed Stochastic Neighbor Embedding (tSNE)
cyt <- runTSNE(cyt)

# This is an optional step
# run Diffusion map
cyt <- runDiffusionMap(cyt)

# This is an optional step
# run Uniform Manifold Approximation and Projection (UMAP)
cyt <- runUMAP(cyt)

# build minimum spanning tree
cyt <- buildTree(cyt)

# DEGs of different branch
diff.list <- runDiff(cyt)

# define root cells
cyt <- defRootCells(cyt, root.cells = c(32,26))

# run pseudotime
cyt <- runPseudotime(cyt)

# define leaf cells
cyt <- defLeafCells(cyt, leaf.cells = c(30))

# run walk between root cells and leaf cells
cyt <- runWalk(cyt)

# Save object
if (FALSE) {
  saveRDS(cyt, file = "Path to you output directory")
}

Visualization

The running template of visualization is as follows:

# Plot 2D tSNE. And cells are colored by cluster id
plot2D(cyt, item.use = c("tSNE_1", "tSNE_2"), color.by = "cluster.id", 
       alpha = 1, main = "tSNE", category = "categorical", show.cluser.id = TRUE)

# Plot 2D UMAP. And cells are colored by cluster id
plot2D(cyt, item.use = c("UMAP_1", "UMAP_2"), color.by = "cluster.id", 
       alpha = 1, main = "UMAP", category = "categorical", show.cluser.id = TRUE)

# Plot 2D tSNE. And cells are colored by cluster id
plot2D(cyt, item.use = c("tSNE_1", "tSNE_2"), color.by = "branch.id", 
       alpha = 1, main = "tSNE", category = "categorical", show.cluser.id = TRUE)

# Plot 2D UMAP. And cells are colored by cluster id
plot2D(cyt, item.use = c("UMAP_1", "UMAP_2"), color.by = "branch.id", 
       alpha = 1, main = "UMAP", category = "categorical", show.cluser.id = TRUE)

# Plot 2D tSNE. And cells are colored by stage
plot2D(cyt, item.use = c("tSNE_1", "tSNE_2"), color.by = "stage", 
       alpha = 1, main = "UMAP", category = "categorical")

# Plot 2D UMAP. And cells are colored by stage
plot2D(cyt, item.use = c("UMAP_1", "UMAP_2"), color.by = "stage", 
       alpha = 1, main = "UMAP", category = "categorical")

# Tree plot
plotTree(cyt, color.by = "D0.percent", show.node.name = TRUE, cex.size = 1)

# Tree plot
plotTree(cyt, color.by = "FITC-A<CD43>", show.node.name = TRUE, cex.size = 1) 


# plot clusters
plotCluster(cyt, item.use = c("tSNE_1", "tSNE_2"), category = "numeric",
            size = 100, color.by = "BV510-A<CD45RA>") 

# plot pie tree
plotPieTree(cyt, cex.size = 3, size.by.cell.number = TRUE)

# plot pie cluster
plotPieCluster(cyt, item.use = c("tSNE_1", "tSNE_2"), cex.size = 40) 

# plot heatmap of clusters
plotClusterHeatmap(cyt)

# plot heatmap of branches
plotBranchHeatmap(cyt)

# Violin plot
plotViolin(cyt, color.by = "cluster.id", marker = "BV510-A<CD45RA>", text.angle = 90)

# Violin plot
plotViolin(cyt, color.by = "branch.id", marker = "BV510-A<CD45RA>", text.angle = 90)

# UMAP plot colored by pseudotime
plot2D(cyt, item.use = c("UMAP_1", "UMAP_2"), category = "numeric",
            size = 1, color.by = "pseudotime")

# tSNE plot colored by pseudotime
plot2D(cyt, item.use = c("tSNE_1", "tSNE_2"), category = "numeric",
            size = 1, color.by = "pseudotime") 

# denisty plot by different stage
plotPseudotimeDensity(cyt, adjust = 1) 
# Tree plot
plotTree(cyt, color.by = "pseudotime", cex.size = 1.5) 

# Violin plot
plotViolin(cyt, color.by = "cluster.id", order.by = "pseudotime",
           marker = "BV650-A<CD49f>", text.angle = 90)

# trajectory value
plotPseudotimeTraj(cyt, var.cols = TRUE)

# Heatmap plot
plotHeatmap(cyt, downsize = 1000, cluster_rows = TRUE, clustering_method = "ward.D",
            color = colorRampPalette(c("#00599F","#EEEEEE","#FF3222"))(100))

# plot cluster
plotCluster(cyt, item.use = c("tSNE_1", "tSNE_2"), color.by = "traj.value.log", 
            size = 10, show.cluser.id = TRUE, category = "numeric") 

References

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CytoTree documentation built on Nov. 10, 2020, 2 a.m.