hi Hernando, I suggest you have a read of: J. N. McClintick & H. J. Edenberg. Effects of filtering by Present call on analysis of microarray experiments.. BMC Bioinformatics, 2006 (7): 49. there's no standard cutoff, but if you plot histograms of normalised data, then can help you choose a cutoff cheers, mark On 07/07/2010, at 11:22 PM, Naomi Altman wrote: > Isn't filtering on spread like pretesting for differential expression? Maybe not such a good idea. > > When using MAS5, it is traditional to use the Affy presence/absence score. (Not necessarily optimal ...) > > --Naomi > > At 06:53 AM 7/7/2010, Yuan Hao wrote: >> Usually it can be filtered based on IQR and/or variance across >> samples, which might be worthy of thinking besides 'average' >> >> Yuan >> >> On 7 Jul 2010, at 11:47, Sean Davis wrote: >> >>> On Wed, Jul 7, 2010 at 6:28 AM, Hernando Mart?nez <hernybiotec at="" gmail.com="">wrote: >>> >>>> Hi, I need to remove genes with low expression values from a >>>> expression >>>> matrix. I would like to remove those with an average of expression >>>> values >>>> less than a certain cut-off. I was thinking in computing the >>>> average for >>>> each row, create a list with the gene names for which their average >>>> is less >>>> than the cut-off, and remove those genes from the initial matrix. >>>> However, >>>> I >>>> have a couple of doubts that maybe you can help me with. Is there any >>>> package or function that makes this easier? And, does anyone know >>>> which >>>> cut-off to use for data normalized with RMA and for data normalized >>>> with >>>> MAS5? Thanks, >>>> >>> Take a look at the genefilter package. However, what you describe >>> can be >>> done easily with standard R. >>> >>> I don't think there is such a thing as a "standard" cutoff for >>> microarray >>> data. >>> >>> Sean >>> >>> [[alternative HTML version deleted]] >>> >>> _______________________________________________ >>> Bioconductor mailing list >>> Bioconductor at stat.math.ethz.ch >>> https://stat.ethz.ch/mailman/listinfo/bioconductor >>> Search the archives: http://news.gmane.org/gmane.science.biology.informatics.conductor >> >> _______________________________________________ >> Bioconductor mailing list >> Bioconductor at stat.math.ethz.ch >> https://stat.ethz.ch/mailman/listinfo/bioconductor >> Search the archives: http://news.gmane.org/gmane.science.biology.informatics.conductor > > Naomi S. Altman 814-865-3791 (voice) > Associate Professor > Dept. of Statistics 814-863-7114 (fax) > Penn State University 814-865-1348 (Statistics) > University Park, PA 16802-2111 > > _______________________________________________ > Bioconductor mailing list > Bioconductor at stat.math.ethz.ch > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: http://news.gmane.org/gmane.science.biology.informatics.conductor

Hi, On Wed, Jul 7, 2010 at 6:22 AM, Naomi Altman <naomi at="" stat.psu.edu=""> wrote: > Isn't filtering on spread like pretesting for differential expression? > ?Maybe not such a good idea. No it isn't like pretesting and it is quite often a good idea. Please have a look at: Independent filtering increases detection power for high-throughput experiments. Bourgon R, Gentleman R, Huber W. Proc Natl Acad Sci U S A. 2010 May 25;107(21):9546-51. Epub 2010 May 11. Where the reasons why it is not like a pretest are given and the potential benefits are laid out. > > When using MAS5, it is traditional to use the Affy presence/absence score. > ?(Not necessarily optimal ...) > > --Naomi > > At 06:53 AM 7/7/2010, Yuan Hao wrote: >> >> Usually it can be filtered based on IQR and/or variance across >> samples, which might be worthy of thinking besides 'average' >> >> Yuan >> >> On 7 Jul 2010, at 11:47, Sean Davis wrote: >> >>> On Wed, Jul 7, 2010 at 6:28 AM, Hernando Mart?nez <hernybiotec at="" gmail.com="">>> >wrote: >>> >>>> Hi, I need to remove genes with low expression values from a >>>> expression >>>> matrix. I would like to remove those with an average of expression >>>> values >>>> less than a certain cut-off. I was thinking in computing the >>>> average for >>>> each row, create a list with the gene names for which their average >>>> is less >>>> than the cut-off, and remove those genes from the initial matrix. >>>> However, >>>> I >>>> have a couple of doubts that maybe you can help me with. Is there any >>>> package or function that makes this easier? And, does anyone know >>>> which >>>> cut-off to use for data normalized with RMA and for data normalized >>>> with >>>> MAS5? Thanks, >>>> >>> Take a look at the genefilter package. ?However, what you describe >>> can be >>> done easily with standard R. >>> >>> I don't think there is such a thing as a "standard" cutoff for >>> microarray >>> data. >>> >>> Sean >>> >>> ? ? ? ?[[alternative HTML version deleted]] >>> >>> _______________________________________________ >>> Bioconductor mailing list >>> Bioconductor at stat.math.ethz.ch >>> https://stat.ethz.ch/mailman/listinfo/bioconductor >>> Search the archives: >>> http://news.gmane.org/gmane.science.biology.informatics.conductor >> >> _______________________________________________ >> Bioconductor mailing list >> Bioconductor at stat.math.ethz.ch >> https://stat.ethz.ch/mailman/listinfo/bioconductor >> Search the archives: >> http://news.gmane.org/gmane.science.biology.informatics.conductor > > Naomi S. Altman ? ? ? ? ? ? ? ? ? ? ? ? ? ? ? ?814-865-3791 (voice) > Associate Professor > Dept. of Statistics ? ? ? ? ? ? ? ? ? ? ? ? ? ? ?814-863-7114 (fax) > Penn State University ? ? ? ? ? ? ? ? ? ? ? ? 814-865-1348 (Statistics) > University Park, PA 16802-2111 > > _______________________________________________ > Bioconductor mailing list > Bioconductor at stat.math.ethz.ch > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: > http://news.gmane.org/gmane.science.biology.informatics.conductor > > -- Robert Gentleman rgentlem at gmail.com

Hi Jim, Unfortunately, we did not use the mask file when scanning the chip. So there is not a single NA in the PM values. So I will go back to the dat file and try to generate a new cel file. Thanks a lot and kind regards, Mike -----Urspr?ngliche Nachricht----- Von: "James W. MacDonald" <jmacdon at="" med.umich.edu=""> Gesendet: 08.07.2010 15:43:26 An: Mike Walter <michael_walter at="" email.de=""> Betreff: Re: [BioC] Yeast 2.0 Arrays >Hi Mike, > >On 7/8/2010 8:40 AM, Mike Walter wrote: >> Hi there, >> >> I have a question on Affymetrix Yeast 2.0 arrays. These arrays >> contain about 5000 probesets for budding and fission yeast, >> respectively. We hybridized budding yeast sample and now I'd like to >> get rid of all the fission yeast probes before normalization. There >> is a mask file outlining which probesets belong to which organism. >> However, when I use ReadAffy(..., rm.mask=T) the number of probes >> does not change (s. below). Is there a way to specify a mask file >> during the affybatch import? > >I assume you are using the mask file when scanning the chip? > >If so, the probes for fission yeast should all be NA, which your test >below will not detect (having a bunch of NA probes won't affect the >dimension of your pm matrices). Something like > >pms <- pm(d1, LISTRUE = TRUE) > >length(pms) - sum(sapply(pms, function(x) allis.na(x))) > >or now that I think about it, > >apply(pm(d1), 2, function(x) sum(!is.na(x))) > >should give you a measure of how many non NA probesets remain. > >Best, > >Jim > > >> >> Any hints are welcome. >> >> Mike >> >>> d1<- ReadAffy(celfile.path=celfile, filenames=filenames, >>> rm.mask=F) d2<- ReadAffy(celfile.path=celfile, filenames=filenames, >>> rm.mask=T) dim(pm(d1)) >> [1] 120855 5 >>> dim(pm(d2)) >> [1] 120855 5 >>> sessionInfo() >> R version 2.10.1 (2009-12-14) i386-pc-mingw32 >> >> locale: [1] LC_COLLATE=German_Germany.1252 >> LC_CTYPE=German_Germany.1252 [3] LC_MONETARY=German_Germany.1252 >> LC_NUMERIC=C [5] LC_TIME=German_Germany.1252 >> >> attached base packages: [1] stats graphics grDevices utils >> datasets methods base >> >> other attached packages: [1] yeast2cdf_2.5.0 affyQCReport_1.24.0 >> lattice_0.18-3 [4] RColorBrewer_1.0-2 affyPLM_1.22.0 >> preprocessCore_1.8.0 [7] xtable_1.5-6 simpleaffy_2.22.0 >> gcrma_2.18.1 [10] genefilter_1.28.2 affy_1.24.2 >> Biobase_2.6.1 >> >> loaded via a namespace (and not attached): [1] affyio_1.14.0 >> annotate_1.24.1 AnnotationDbi_1.8.2 [4] Biostrings_2.14.12 >> DBI_0.2-5 grid_2.10.1 [7] IRanges_1.4.16 RSQLite_0.9-1 >> splines_2.10.1 [10] survival_2.35-8 tools_2.10.1 >>> >> > >-- >James W. MacDonald, M.S. >Biostatistician >Douglas Lab >University of Michigan >Department of Human Genetics >5912 Buhl >1241 E. Catherine St. >Ann Arbor MI 48109-5618 >734-615-7826 >********************************************************** >Electronic Mail is not secure, may not be read every day, and should not be used for urgent or sensitive issues

Hi Jim, I thought of two workarounds to mask the S pombe probes with the code attached below. However, in both attempt R crashes, when I call the rma() function either with the NAs introduced in the Affybatch or the subset option. I guess this would also happen, when I use the mask file to generate the cel file and use rm.mask=T in the ReadAffy() call? Do you (or anyone else) have any explanation for the breakdown of R? Btw, mas5() also gives an error on option 1 due to NAs. Kind regards, Mike Code for 1st Option: library(affy) celfile = "X:\\affy\\array\\2010\\E10R027" filenames = list.files(path=celfile) filenames = filenames[grep(".CEL", filenames)] filenames d1 = ReadAffy(celfile.path=celfile, filenames=filenames) msk=read.table("F:/Auswertung/Array Annotationen/Affy/s_cerevisiae.msk", header=F, skip=2, row.names=1) pombe = c(as.vector(unlist(pmindex(d1)[rownames(msk)])), as.vector(unlist(mmindex(d1)[rownames(msk)]))) exprs(d1)[pombe,]=NA apply(pm(d1), 2, function(x) sum(!is.na(x))) #drops from 120855 to 65552 features d1n = rma(d1) #R crashes completely with following error information: AppName: rgui.exe AppVer: 2.100.50208.0 ModName: preprocesscore.dll ModVer: 0.0.0.0?? ? Offset: 00017253 Code for 2nd Option: d2 = ReadAffy(celfile.path=celfile, filenames=filenames) msk.sp=read.table("F:/Auswertung/Array Annotationen/Affy/s_pombe.msk", header=F, skip=2, row.names=1) head(msk.sp) d2n = rma(d2, subset=rownames(msk.sp)) #again R crashes completely!!! AppName: rgui.exe AppVer: 2.101.50720.0 ModName: preprocesscore.dll ModVer: 0.0.0.0 Offset: 00017253 > sessionInfo() R version 2.10.1 (2009-12-14) i386-pc-mingw32 locale: [1] LC_COLLATE=German_Germany.1252 LC_CTYPE=German_Germany.1252 [3] LC_MONETARY=German_Germany.1252 LC_NUMERIC=C [5] LC_TIME=German_Germany.1252 attached base packages: [1] stats graphics grDevices utils datasets methods base other attached packages: [1] yeast2cdf_2.5.0 affy_1.24.2 Biobase_2.6.1 loaded via a namespace (and not attached): [1] affyio_1.14.0 preprocessCore_1.8.0 tools_2.10.1 -- MFT?Services University?of?T?bingen Calwerstr.?7 72076??T?bingen/GERMANY Tel.:?+49 7071?29?83210 Fax.?+?49 7071?29?5228 web: www.mft-services.de Confidentiality?Note: This?message?is?intended?only?for?the?use?of?the?named?recipient(s)?an d?may contain?confidential?and/or?proprietary?information.?If?you?are?not?th e?intended recipient,?please?contact?the?sender?and?delete?the?message.?Any?unaut horized use?of?the?information?contained?in?this?message?is?prohibited. -----Urspr?ngliche Nachricht----- Von: "James W. MacDonald" <jmacdon at="" med.umich.edu=""> Gesendet: 08.07.2010 15:43:26 An: Mike Walter <michael_walter at="" email.de=""> Betreff: Re: [BioC] Yeast 2.0 Arrays >Hi Mike, > >On 7/8/2010 8:40 AM, Mike Walter wrote: >> Hi there, >> >> I have a question on Affymetrix Yeast 2.0 arrays. These arrays >> contain about 5000 probesets for budding and fission yeast, >> respectively. We hybridized budding yeast sample and now I'd like to >> get rid of all the fission yeast probes before normalization. There >> is a mask file outlining which probesets belong to which organism. >> However, when I use ReadAffy(..., rm.mask=T) the number of probes >> does not change (s. below). Is there a way to specify a mask file >> during the affybatch import? > >I assume you are using the mask file when scanning the chip? > >If so, the probes for fission yeast should all be NA, which your test >below will not detect (having a bunch of NA probes won't affect the >dimension of your pm matrices). Something like > >pms <- pm(d1, LISTRUE = TRUE) > >length(pms) - sum(sapply(pms, function(x) allis.na(x))) > >or now that I think about it, > >apply(pm(d1), 2, function(x) sum(!is.na(x))) > >should give you a measure of how many non NA probesets remain. > >Best, > >Jim > > >> >> Any hints are welcome. >> >> Mike >> >>> d1<- ReadAffy(celfile.path=celfile, filenames=filenames, >>> rm.mask=F) d2<- ReadAffy(celfile.path=celfile, filenames=filenames, >>> rm.mask=T) dim(pm(d1)) >> [1] 120855 5 >>> dim(pm(d2)) >> [1] 120855 5 >>> sessionInfo() >> R version 2.10.1 (2009-12-14) i386-pc-mingw32 >> >> locale: [1] LC_COLLATE=German_Germany.1252 >> LC_CTYPE=German_Germany.1252 [3] LC_MONETARY=German_Germany.1252 >> LC_NUMERIC=C [5] LC_TIME=German_Germany.1252 >> >> attached base packages: [1] stats graphics grDevices utils >> datasets methods base >> >> other attached packages: [1] yeast2cdf_2.5.0 affyQCReport_1.24.0 >> lattice_0.18-3 [4] RColorBrewer_1.0-2 affyPLM_1.22.0 >> preprocessCore_1.8.0 [7] xtable_1.5-6 simpleaffy_2.22.0 >> gcrma_2.18.1 [10] genefilter_1.28.2 affy_1.24.2 >> Biobase_2.6.1 >> >> loaded via a namespace (and not attached): [1] affyio_1.14.0 >> annotate_1.24.1 AnnotationDbi_1.8.2 [4] Biostrings_2.14.12 >> DBI_0.2-5 grid_2.10.1 [7] IRanges_1.4.16 RSQLite_0.9-1 >> splines_2.10.1 [10] survival_2.35-8 tools_2.10.1 >>> >> > >-- >James W. MacDonald, M.S. >Biostatistician >Douglas Lab >University of Michigan >Department of Human Genetics >5912 Buhl >1241 E. Catherine St. >Ann Arbor MI 48109-5618 >734-615-7826 >********************************************************** >Electronic Mail is not secure, may not be read every day, and should not be used for urgent or sensitive issues