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James Anderson wrote: > Hi, > > I am analyzing about 30 agilent two color arrays. One simple question is that, in terms of the downstream analysis such as finding differentially expressed genes, what are the features should I use (such as log ratio, mean intensity of red and green, etc)? I have some experience in Affy, but almost no experience in agilent. > > In addition, I am trying to use arrayMagic from Bioconductor to do quality control and pre-processing of my agilent arrays. From the example arrayMagic gave in the manual, it seems that the format of the example data is somewhat different than agilent data format. > > I saw the following header file > > HEADER SPOT GRID TOP LEFT BOT RIGHT ROW COL CH1I CH1B CH1AB CH2I CH2B CH2AB SPIX BGPIX EDGE RAT2 MRAT REGR CORR LFRAT CH1GTB1 CH2GTB1 CH1GTB2 CH2GTB2 CH1EDGEA CH2EDGEA FLAG CH1KSD CH1KSP CH2KSD CH2KSP > While my agilent arrays has the following header information: > > FeatureNum Row Col Start Sequence ProbeUID ControlType ProbeName GeneName PositionX PositionY LogRatio LogRatioError PValueLogRatio gSurrogateUsed rSurrogateUsed gIsFound rIsFound gProcessedSignal rProcessedSignal gProcessedSigError rProcessedSigError gNumPixOLHi rNumPixOLHi gNumPixOLLo rNumPixOLLo gNumPix rNumPix gMeanSignal rMeanSignal gMedianSignal rMedianSignal gPixSDev rPixSDev gBGNumPix rBGNumPix gBGMeanSignal rBGMeanSignal gBGMedianSignal rBGMedianSignal gBGPixSDev rBGPixSDev gNumSatPix rNumSatPix gIsSaturated rIsSaturated PixCorrelation BGPixCorrelation gIsFeatNonUnifOL rIsFeatNonUnifOL gIsBGNonUnifOL rIsBGNonUnifOL gIsFeatPopnOL rIsFeatPopnOL > gIsBGPopnOL rIsBGPopnOL IsManualFlag gBGSubSignal rBGSubSignal gBGSubSigError rBGSubSigError BGSubSigCorrelation gIsPosAndSignif rIsPosAndSignif gPValFeatEqBG rPValFeatEqBG gNumBGUsed rNumBGUsed gIsWellAboveBG rIsWellAboveBG gBGUsed rBGUsed gBGSDUsed rBGSDUsed IsNormalization gDyeNormSignal rDyeNormSignal gDyeNormError rDyeNormError DyeNormCorrelation ErrorModel xDev gSpatialDetrendIsInFilteredSet rSpatialDetrendIsInFilteredSet gSpatialDetrendSurfaceValue rSpatialDetrendSurfaceValue > > How should I use arrayMagic on my data? > I haven't used arrayMagic for Agilent data. You can use limma and read.maimages() to load your data. As for what columns to use, the logRatio column of course contains a ratio, while the columns rProcessedSignal and gProcessedSignal probably contain the background-corrected intensities. You will probably want to glance at the Agilent technical manual about what the columns represent, in more detail. As for what columns you will want to use in your analysis, you will need to be specific about your experimental design. If you used a common reference, then you can simply treat the logRatio in the same way as your affymetrix arrays for the purposes of analysis. Sean