# NOT RUN {
#generate some example data
set.seed(100)
x<-matrix(rnorm(1000*20),ncol=20)
dd<-sample(1:1000,size=100)
u<-matrix(2*rnorm(100),ncol=10,nrow=100)
x[dd,11:20]<-x[dd,11:20]+u
y<-c(rep(1,10),rep(2,10))
data=list(x=x,y=y, geneid=as.character(1:nrow(x)),
genenames=paste("g",as.character(1:nrow(x)),sep=""), logged2=TRUE)
log2=function(x){log(x)/log(2)}
# run SAM first
samr.obj<-samr(data, resp.type="Two class unpaired", nperms=100)
# assess current sample size (20), assuming 1.5fold difference on the log base 2 scale
samr.assess.samplesize.obj<- samr.assess.samplesize(samr.obj, data, log2(1.5))
samr.assess.samplesize.plot(samr.assess.samplesize.obj)
# }
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