Nothing
## ----setup, include=FALSE-----------------------------------------------------
knitr::opts_chunk$set(echo = TRUE)
## ----eval=TRUE----------------------------------------------------------------
#Load the library
library(phosphonormalizer)
#Enriched data overview
head(enriched.rd)
#Non-enriched data overview
head(non.enriched.rd)
## ----eval=FALSE---------------------------------------------------------------
# ## try http:// if https:// URLs are not supported
# if (!requireNamespace("BiocManager", quietly=TRUE))
# install.packages("BiocManager")
# BiocManager::install("phosphonormalizer")
## ----eval=TRUE, fig.height = 4, fig.width = 6, fig.align = "center"-----------
#Load the library
library(phosphonormalizer)
#Specify the column numbers of abundances in the original data.frame,
#from both enriched and non-enriched runs
samplesCols <- data.frame(enriched=3:17, non.enriched=3:17)
#Specify the column numbers of sequence and modification in the original data.frame,
#from both enriched and non-enriched runs
modseqCols <- data.frame(enriched = 1:2, non.enriched = 1:2)
#The samples and their technical replicates
techRep <- factor(x = c(1,1,1,2,2,2,3,3,3,4,4,4,5,5,5))
#If the paramter plot.fc set, the corresponding plots of Sample fold changes is produced
#Here, for demonstration, the fold change distributions are shown for samples 3 vs 1
plot.param <- list(control = c(1), samples = c(3))
#Call the function
norm <- normalizePhospho(enriched = enriched.rd, non.enriched = non.enriched.rd,
samplesCols = samplesCols, modseqCols = modseqCols, techRep = techRep,
plot.fc = plot.param)
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