calcCounts: Calculate cluster cell counts
In diffcyt: Differential discovery in high-dimensional cytometry via high-resolution clustering
Description
Usage
Arguments
Details
Value
Examples
Description
Calculate number of cells per cluster-sample combination
Usage
1
calcCounts(d_se)
Arguments
d_se
Data object from previous steps, in SummarizedExperiment
format, containing cluster labels as a column in the row meta-data (from
generateClusters).
Details
Calculate number of cells per cluster-sample combination (referred to as cluster cell
'counts', 'abundances', or 'frequencies').
The cluster cell counts are required for testing for differential abundance of cell
populations, and are also used for weights and filtering when testing for differential
states within cell populations.
Results are returned as a new SummarizedExperiment object, where rows =
clusters, columns = samples, assay = values (counts). (Note that this structure
differs from the input data object.)
Value
d_counts: SummarizedExperiment object, where rows =
clusters, columns = samples, assay = values (counts).
Examples
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# For a complete workflow example demonstrating each step in the 'diffcyt' pipeline,
# see the package vignette.
# Function to create random data (one sample)
d_random <- function(n = 20000, mean = 0, sd = 1, ncol = 20, cofactor = 5) {
d <- sinh(matrix(rnorm(n, mean, sd), ncol = ncol)) * cofactor
colnames(d) <- paste0("marker", sprintf("%02d", 1:ncol))
d
}
# Create random data (without differential signal)
set.seed(123)
d_input <- list(
sample1 = d_random(),
sample2 = d_random(),
sample3 = d_random(),
sample4 = d_random()
)
experiment_info <- data.frame(
sample_id = factor(paste0("sample", 1:4)),
group_id = factor(c("group1", "group1", "group2", "group2")),
stringsAsFactors = FALSE
)
marker_info <- data.frame(
channel_name = paste0("channel", sprintf("%03d", 1:20)),
marker_name = paste0("marker", sprintf("%02d", 1:20)),
marker_class = factor(c(rep("type", 10), rep("state", 10)),
levels = c("type", "state", "none")),
stringsAsFactors = FALSE
)
# Prepare data
d_se <- prepareData(d_input, experiment_info, marker_info)
# Transform data
d_se <- transformData(d_se)
# Generate clusters
d_se <- generateClusters(d_se)
# Calculate counts
d_counts <- calcCounts(d_se)
diffcyt documentation built on Nov. 8, 2020, 6:37 p.m.
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Description Usage Arguments Details Value Examples
Description
Calculate number of cells per cluster-sample combination
Usage
1 | calcCounts(d_se)
|
Arguments
d_se |
Data object from previous steps, in |
Details
Calculate number of cells per cluster-sample combination (referred to as cluster cell 'counts', 'abundances', or 'frequencies').
The cluster cell counts are required for testing for differential abundance of cell populations, and are also used for weights and filtering when testing for differential states within cell populations.
Results are returned as a new SummarizedExperiment object, where rows =
clusters, columns = samples, assay = values (counts). (Note that this structure
differs from the input data object.)
Value
d_counts: SummarizedExperiment object, where rows =
clusters, columns = samples, assay = values (counts).
Examples
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 | # For a complete workflow example demonstrating each step in the 'diffcyt' pipeline,
# see the package vignette.
# Function to create random data (one sample)
d_random <- function(n = 20000, mean = 0, sd = 1, ncol = 20, cofactor = 5) {
d <- sinh(matrix(rnorm(n, mean, sd), ncol = ncol)) * cofactor
colnames(d) <- paste0("marker", sprintf("%02d", 1:ncol))
d
}
# Create random data (without differential signal)
set.seed(123)
d_input <- list(
sample1 = d_random(),
sample2 = d_random(),
sample3 = d_random(),
sample4 = d_random()
)
experiment_info <- data.frame(
sample_id = factor(paste0("sample", 1:4)),
group_id = factor(c("group1", "group1", "group2", "group2")),
stringsAsFactors = FALSE
)
marker_info <- data.frame(
channel_name = paste0("channel", sprintf("%03d", 1:20)),
marker_name = paste0("marker", sprintf("%02d", 1:20)),
marker_class = factor(c(rep("type", 10), rep("state", 10)),
levels = c("type", "state", "none")),
stringsAsFactors = FALSE
)
# Prepare data
d_se <- prepareData(d_input, experiment_info, marker_info)
# Transform data
d_se <- transformData(d_se)
# Generate clusters
d_se <- generateClusters(d_se)
# Calculate counts
d_counts <- calcCounts(d_se)
|
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