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Lana Schaffer ★ 1.3k
@lana-schaffer-1056
Last seen 10.2 years ago
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@gregor-siegler-1366
Last seen 10.2 years ago
Dear list, I have encountered following problem and do not know how to solve it: After processing my data with RMA and filtering genes, that are not of interest I have performed SAM analysis. Here are the steps I took: cell <- ReadAffy() RMAcell <- rma(cell) after filtering my data set, I have the following: filtered Expression Set (exprSet) with 2271 genes 20 samples phenoData object with 1 variables and 20 cases varLabels sample: arbitrary numbering I now perform SAM anaylsis like this to extract the genes of interest (I want to have about 120 called genes): cl <- c(0,0,0,0,0,0,0,0,0,0,1,1,1,1,1,1,1,1,1,1) where 0 stands for the probes of group 0, 1 for the samples of group 1. c <- seq(1.3, 1.36, 0.01) sam(filtered, cl, delta=c, rand =123) SAM Analysis for the Two-Class Unpaired Case Assuming Unequal Variances Delta p0 False Called FDR 1 1.30 0.464 7.44 127 0.0272 2 1.31 0.464 7.30 126 0.0269 3 1.32 0.464 6.71 120 0.0260 4 1.33 0.464 6.41 117 0.0254 5 1.34 0.464 5.50 109 0.0234 6 1.35 0.464 5.50 109 0.0234 7 1.36 0.464 5.07 103 0.0229 now I summarize my results for delta= 1.32 : sumRMA <- summary(sam(filtered,cl, delta=1.32, rand=123)) and want to extract those 120 genes like this: top120RMA<-filtered[sumRMA at row.sig.genes,] top120RMA Expression Set (exprSet) with 0 genes 20 samples phenoData object with 1 variables and 20 cases varLabels sample: arbitrary numbering but as you can see, my expression set contains 0 genes out of my 20 samples. If I try the same steps but with GCRMA instead of RMA, everything works out well (of course with a different value for delta). Every kind of help would be very much appreciated. Thanks in advance! With best regards, gregor
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