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inst/doc/steady-state-vignette.R
In flowTime: Annotation and analysis of biological dynamical systems using flow cytometry
## ---- echo = FALSE, message=FALSE---------------------------------------------
knitr::opts_chunk$set(collapse = TRUE, comment = "#>", tidy = TRUE)
library(flowCore)
library(flowTime)
library(ggplot2)
## -----------------------------------------------------------------------------
plate1<-read.flowSet(path=system.file("extdata", "ss_example",
package = "flowTime"), alter.names = TRUE)
# add plate numbers to the sampleNames
sampleNames(plate1)<-paste("1_", sampleNames(plate1), sep = "")
dat<-plate1
## ---- eval = F----------------------------------------------------------------
# plate2 <- read.flowSet(path = paste(experiment, "_2/", sep = ""),
# alter.names = TRUE)
# sampleNames(plate2) <- paste("2_", sampleNames(plate2), sep = "")
# dat <- rbind2(plate1, plate2)
## -----------------------------------------------------------------------------
annotation <- read.csv(system.file("extdata", "ss_example.csv",
package = "flowTime"))
head(annotation)
sampleNames(dat)
sampleNames(dat) == annotation$name
## ---- eval = F----------------------------------------------------------------
# annotation <- cbind(annotation, 'name' = sampleNames(dat))
# # or
# annotation <- createAnnotation(yourFlowSet = dat)
# write.csv(annotation, file = 'path/to/yourAnnotation.csv')
## -----------------------------------------------------------------------------
adat <- annotateFlowSet(yourFlowSet = dat, annotation_df = annotation,
mergeBy = 'name')
head(rownames(pData(adat)))
head(pData(adat))
## ---- eval = F----------------------------------------------------------------
# write.flowSet(adat, outdir = 'your/favorite/directory')
#
# # Read the flowSet with the saved experimental meta data
# read.flowSet('flowSet folder', path = 'your/flow/directory',
# phenoData = 'annotation.txt', alter.names = TRUE)
## ---- fig.width = 4, fig.height = 4-------------------------------------------
loadGates() # use the default included gateSet
dat.SS <- steadyState(flowset = adat, ploidy = 'diploid', only = 'singlets')
p <- ggplot(dat.SS, aes(x = as.factor(treatment), y = FL2.A, fill = AFB)) +
geom_boxplot(outlier.shape = NA) + facet_grid(IAA~AFB) +
theme_classic(base_family = 'Arial', base_size = 16) + ylim(c(-1000,10000)) +
xlab(expression(paste('Auxin (',mu,'M)',sep = ""))) +
ylab('Fluorescence (AU)') + theme(legend.position="none")
p
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flowTime documentation built on Nov. 8, 2020, 8:13 p.m.
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## ---- echo = FALSE, message=FALSE---------------------------------------------
knitr::opts_chunk$set(collapse = TRUE, comment = "#>", tidy = TRUE)
library(flowCore)
library(flowTime)
library(ggplot2)
## -----------------------------------------------------------------------------
plate1<-read.flowSet(path=system.file("extdata", "ss_example",
package = "flowTime"), alter.names = TRUE)
# add plate numbers to the sampleNames
sampleNames(plate1)<-paste("1_", sampleNames(plate1), sep = "")
dat<-plate1
## ---- eval = F----------------------------------------------------------------
# plate2 <- read.flowSet(path = paste(experiment, "_2/", sep = ""),
# alter.names = TRUE)
# sampleNames(plate2) <- paste("2_", sampleNames(plate2), sep = "")
# dat <- rbind2(plate1, plate2)
## -----------------------------------------------------------------------------
annotation <- read.csv(system.file("extdata", "ss_example.csv",
package = "flowTime"))
head(annotation)
sampleNames(dat)
sampleNames(dat) == annotation$name
## ---- eval = F----------------------------------------------------------------
# annotation <- cbind(annotation, 'name' = sampleNames(dat))
# # or
# annotation <- createAnnotation(yourFlowSet = dat)
# write.csv(annotation, file = 'path/to/yourAnnotation.csv')
## -----------------------------------------------------------------------------
adat <- annotateFlowSet(yourFlowSet = dat, annotation_df = annotation,
mergeBy = 'name')
head(rownames(pData(adat)))
head(pData(adat))
## ---- eval = F----------------------------------------------------------------
# write.flowSet(adat, outdir = 'your/favorite/directory')
#
# # Read the flowSet with the saved experimental meta data
# read.flowSet('flowSet folder', path = 'your/flow/directory',
# phenoData = 'annotation.txt', alter.names = TRUE)
## ---- fig.width = 4, fig.height = 4-------------------------------------------
loadGates() # use the default included gateSet
dat.SS <- steadyState(flowset = adat, ploidy = 'diploid', only = 'singlets')
p <- ggplot(dat.SS, aes(x = as.factor(treatment), y = FL2.A, fill = AFB)) +
geom_boxplot(outlier.shape = NA) + facet_grid(IAA~AFB) +
theme_classic(base_family = 'Arial', base_size = 16) + ylim(c(-1000,10000)) +
xlab(expression(paste('Auxin (',mu,'M)',sep = ""))) +
ylab('Fluorescence (AU)') + theme(legend.position="none")
p
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R Package Documentation
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We want your feedback!
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