Hi guys, could you suggest me a way to normalize Illumina expression beadchip data?

For example, starting from the GSE32025_non-normalized.txt.gz file, could you suggest me some few steps (preferentially in R) to finally obtain a normalized data matrix as for Affymetrix RMA normalisation? I suppose this is an intensity "count" matrix. When I started reading it using limma and the following instruction: idata <- read.ilmn("GSE32025_non-normalized.txt",probeid = "ID_REF",expr="SKBR"), the following error appeared:

Error in readGenericHeader(fname, columns = expr, sep = sep) : 
  Specified column headings not found in file
In addition: Warning message:
In grep(a, txt) : input string 1 is invalid in this locale

I don't know how to deal with this error since this is the first time for me that I analyse this kind of data.

Can anyone help me please?

Thank you in advance

e.

You can download the already-normalised data with:

library(Biobase)
library(GEOquery)

# load series and platform data from GEO
gset <- getGEO("GSE32025", GSEMatrix =TRUE, getGPL=FALSE)
if (length(gset) > 1) idx <- grep("GPL6885", attr(gset, "names")) else idx <- 1
gset <- gset[[idx]]

dev.new(width=4+dim(gset)[[2]]/5, height=6)
par(mar=c(2+round(max(nchar(sampleNames(gset)))/2),4,2,1))
title <- paste ("GSE32025", '/', annotation(gset), " selected samples", sep ='')
boxplot(exprs(gset), boxwex=0.7, notch=T, main=title, outline=FALSE, las=2)

Kevin