-----Original Message----- From: bioconductor-bounces@stat.math.ethz.ch [mailto:bioconductor-bounces@stat.math.ethz.ch] On Behalf Of Maria Fookes Sent: 11 March 2004 11:05 To: bioconductor@stat.math.ethz.ch FAO Limma developers, I have started to use the limma package for a couple of two-colour hybridization slides RNA/RNA... can anybody tell me if I can still use it When I have features in the array at one spacing (controls) and other features at another spacing? Or do I have to modify my gpr file? (generated by genepix) Thank you very much in advance Mar?a _______________________________________________ Bioconductor mailing list Bioconductor@stat.math.ethz.ch https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor

Hi Maria, limma is set up to handle replicate spots which have constant spacing by default. The assumption when you fit a linear model with lmFit() is that the log-ratios from the duplicate spots on an array are correlated through being on the same array and being spatially separated by a constant amount (ie side-by-side, or one below the other). This assumption is violated if the spacing isn't constant. If the spacing is constant for your data (but different?) for the two classes of spots, you could always fit the linear model separately to the 2 subsets of spots after normalization. I've put a toy example below which might help. I wouldn't bother rearranging the gpr files. Best wishes, Matt Ritchie # Example - assume we have 2 replicate arrays, each with 6 genes printed in duplicate in a 3x4 grid # the control spots are side by side, however the genes are below each other genes <- data.frame(ID=c("Control1","Control1","Control2","Control2","AA1","AA2 ","AA3","AA4", "AA1", "AA2", "AA3", "AA4"), Name=c("Ratio 1","Ratio 1","House keeping 1","House keeping 1","Gene 1","Gene 2","Gene 3","Gene 4", "Gene1", "Gene2", "Gene3", "Gene4")) genes # The information stored in types would normally be kept in a spottypes file and read in using readSpotTypes() - see the limma user's guide for an example types <- data.frame(SpotType=c("Gene","Ratio","Housekeeping"),ID=c("*","Control *","Control*"),Name=c("*","Ratio*","House keeping*"),col=c("black","red","blue")) status <- controlStatus(types,genes) # randomly generate an MAList object for the 2 array MA <- new("MAList", list(M=matrix(rnorm(24), 12, 2), A=matrix(rnorm(24, 10, 2), 12, 2))) MA # calulate the duplicate correlation for the two groups (different for each because of the different spacing - note the different spacing arguments) corGene <- duplicateCorrelation(MA[status=="Gene",], ndups=2, spacing=4) corControl <- duplicateCorrelation(MA[status=="Ratio" | status=="Houeskeeping",], ndups=2, spacing=1) # now summarise the log-ratios for the genes and the controls fitGene <- lmFit(MA[status=="Gene",], ndups=2, spacing=4, correlation=corGene$cor) fitControl <- lmFit(MA[status=="Ratio"|status=="Housekeeping",], ndups=2, spacing=1, correlation=corControl$cor) > -----Original Message----- > From: bioconductor-bounces@stat.math.ethz.ch > [mailto:bioconductor-bounces@stat.math.ethz.ch] On Behalf Of Maria > Fookes > Sent: 11 March 2004 11:05 > To: bioconductor@stat.math.ethz.ch > > FAO Limma developers, > > I have started to use the limma package for a couple of two-colour > hybridization slides RNA/RNA... can anybody tell me if I can still use > it > When I have features in the array at one spacing (controls) and other > features at another spacing? Or do I have to modify my gpr file? > (generated by genepix) > > Thank you very much in advance > Mar?a