modifyWeights Problem
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@gordon-smyth
Last seen 2 hours ago
WEHI, Melbourne, Australia
> Date: Wed, 3 Feb 2010 23:31:40 -0600 > From: stephen sefick <ssefick at="" gmail.com=""> > To: bioc-devel at stat.math.ethz.ch > Subject: [Bioc-devel] modifyWeights Problem > Content-Type: text/plain; charset=UTF-8 > > I am using the limma packages for the first time, and I need help with > the modifyWeights function. I have about three years of experience > with R programing, but this is the first time that I have run an > analysis with a bioconductor package. I have included the code below. > I know that this is not a reproducible example and I would gladly > give any more information requested. I am trying to modify the > weights of genes that I know are housekeeping genes (upweight). I can > not get the modifyWeights function to work to save my life. The > weights array is 6400, 6. The control status vector is 12800- that > seems like only two of the arrays are being represented??????? I > don't know what is wrong. Any help would be greatly appreciated > thanks, > > Stephen Sefick > > library(limma) > library(marray) > library(convert) > library(statmod) > #read in targets file > targets <- readTargets("targets.txt", row.names="Name") > #weight everything with flags !cutoff=0! > RG <- read.maimages(targets$FileName, source="genepix", > wt.fun=wtflags(cutoff=-50 weight=0)) > #read .gal file > #remove extra tab in file > > a <- readGAL() It is highly unlikely that you need to read a GAL file. The limma User's Guide tells you that you only need to do this with SPOT input, not with GenePix. It is obvious from the information you give that whatever GAL file you are reading, it doesn't match your GenePix files, because it has twice as many rows. > b <- a[,-6] > RG$genes<-b > #spot types file > spottypes <- readSpotTypes() > RG$genes$Status <- controlStatus(spottypes, RG$genes) > > ##################CHANGE weighting for spot types##################### > ###################################################################### > multiply <- c(1,0,2,0,1,0,1,1,1) > ###################################################################### > ###################################################################### > > a <- unique(RG$genes$ID) > status=RG$genes$Status > w <- modifyWeights(RG$weights, RG$genes$Status, a, c(0, 1)) Have you looked at the help page for modifyWeights? I'd think a quick read would tell you that your input arguments aren't the right dimensions, so there's no chance of this call working correctly. I also wonder what you're trying to achieve with modifyWeights, and whether you need it at all? This function is only needed for special situations. Best wishes Gordon > -- > Stephen Sefick ______________________________________________________________________ The information in this email is confidential and intend...{{dropped:4}}
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@stephen-sefick-3922
Last seen 8.1 years ago
There are housekeeping genes that should not be differentially expressed. I was trying to up weight these in the normalization process. Also, I am sorry if I am a bother, but what I am trying to recreate in the normalization process is this: background normalization two dimensional normalization for spatial and then print tip loess scale normalization between arrays #MA <- maNormMain(as(RG, "marrayRaw"), f.loc = list(maNorm2D(weights=w))) MA <- maNorm(as(RG, "marrayRaw"), norm="twoD") MA <- normalizeWithinArrays(as(MA, "MAList")) ################################################################## #MA <- normalizeWithinArrays(RG) #scale normalization between arrays WA <- normalizeBetweenArrays(as(MA, "MAList"), method="scale") I appreciate everyone's help. I will work on this tomorrow, and try to form my questions more coherently. thanks, Stephen On Thu, Feb 4, 2010 at 4:51 PM, Gordon K Smyth <smyth at="" wehi.edu.au=""> wrote: > > >> Date: Wed, 3 Feb 2010 23:31:40 -0600 >> From: stephen sefick <ssefick at="" gmail.com=""> >> To: bioc-devel at stat.math.ethz.ch >> Subject: [Bioc-devel] modifyWeights Problem >> Content-Type: text/plain; charset=UTF-8 >> >> I am using the limma packages for the first time, and I need help with >> the modifyWeights function. ?I have about three years of experience >> with R programing, but this is the first time that I have run an >> analysis with a bioconductor package. ?I have included the code below. >> I know that this is not a reproducible example and I would gladly >> give any more information requested. ?I am trying to modify the >> weights of genes that I know are housekeeping genes (upweight). ?I can >> not get the modifyWeights function to work to save my life. ?The >> weights array is 6400, 6. ?The control status vector is 12800- that >> seems like only two of the arrays are being represented??????? ?I >> don't know what is wrong. ?Any help would be greatly appreciated >> thanks, >> >> Stephen Sefick >> >> library(limma) >> library(marray) >> library(convert) >> library(statmod) >> #read in targets file >> targets <- readTargets("targets.txt", row.names="Name") >> #weight everything with flags !cutoff=0! >> RG <- read.maimages(targets$FileName, source="genepix", >> wt.fun=wtflags(cutoff=-50 weight=0)) >> #read .gal file >> #remove extra tab in file >> >> a <- readGAL() > > It is highly unlikely that you need to read a GAL file. ?The limma User's > Guide tells you that you only need to do this with SPOT input, not with > GenePix. > > It is obvious from the information you give that whatever GAL file you are > reading, it doesn't match your GenePix files, because it has twice as many > rows. > >> b <- a[,-6] >> RG$genes<-b >> #spot types file >> spottypes <- readSpotTypes() >> RG$genes$Status <- controlStatus(spottypes, RG$genes) >> >> ##################CHANGE weighting for spot types##################### >> ###################################################################### >> multiply <- c(1,0,2,0,1,0,1,1,1) >> ###################################################################### >> ###################################################################### >> >> a <- unique(RG$genes$ID) >> status=RG$genes$Status >> w <- modifyWeights(RG$weights, RG$genes$Status, a, c(0, 1)) > > Have you looked at the help page for modifyWeights? ?I'd think a quick read > would tell you that your input arguments aren't the right dimensions, so > there's no chance of this call working correctly. > > I also wonder what you're trying to achieve with modifyWeights, and whether > you need it at all? ?This function is only needed for special situations. > > Best wishes > Gordon > >> -- >> Stephen Sefick > > ______________________________________________________________________ > The information in this email is confidential and inte...{{dropped:19}}
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Dear Stephen, The normalization process that you outline doesn't make sense, as least to me. In my opinion, you cannot sensibly combine two-dimensional loess (which is what maNorm is doing) with one-dimensional loess (which is what normalizeWithinArrays is doing). You say that this is your first microarray analysis, so I wonder what causes you to want to do it this way. There is no documentation I know of that recommends it. Similarly, no published papers that recommend it. I can't help thinking you're making it unnecessarily hard for yourself. Why not follow the documentation, and do something simple and easy that works? I might also add that two-dimensional loess is a marray package function, not a limma function. And your desired normalization process seems to have nothing to do with modifyWeights. So it's not really my problem! Best wishes Gordon On Thu, 4 Feb 2010, stephen sefick wrote: > There are housekeeping genes that should not be differentially > expressed. I was trying to up weight these in the normalization > process. Also, I am sorry if I am a bother, but what I am trying to > recreate in the normalization process is this: > > background normalization > two dimensional normalization for spatial and then print tip loess > scale normalization between arrays > > #MA <- maNormMain(as(RG, "marrayRaw"), f.loc = list(maNorm2D(weights=w))) > MA <- maNorm(as(RG, "marrayRaw"), norm="twoD") > MA <- normalizeWithinArrays(as(MA, "MAList")) > ################################################################## > > #MA <- normalizeWithinArrays(RG) > > #scale normalization between arrays > WA <- normalizeBetweenArrays(as(MA, "MAList"), method="scale") > > I appreciate everyone's help. I will work on this tomorrow, and try > to form my questions more coherently. > > > thanks, > > Stephen > > On Thu, Feb 4, 2010 at 4:51 PM, Gordon K Smyth <smyth at="" wehi.edu.au=""> wrote: >> >> >>> Date: Wed, 3 Feb 2010 23:31:40 -0600 >>> From: stephen sefick <ssefick at="" gmail.com=""> >>> To: bioc-devel at stat.math.ethz.ch >>> Subject: [Bioc-devel] modifyWeights Problem >>> Content-Type: text/plain; charset=UTF-8 >>> >>> I am using the limma packages for the first time, and I need help with >>> the modifyWeights function. ?I have about three years of experience >>> with R programing, but this is the first time that I have run an >>> analysis with a bioconductor package. ?I have included the code below. >>> I know that this is not a reproducible example and I would gladly >>> give any more information requested. ?I am trying to modify the >>> weights of genes that I know are housekeeping genes (upweight). ?I can >>> not get the modifyWeights function to work to save my life. ?The >>> weights array is 6400, 6. ?The control status vector is 12800- that >>> seems like only two of the arrays are being represented??????? ?I >>> don't know what is wrong. ?Any help would be greatly appreciated >>> thanks, >>> >>> Stephen Sefick >>> >>> library(limma) >>> library(marray) >>> library(convert) >>> library(statmod) >>> #read in targets file >>> targets <- readTargets("targets.txt", row.names="Name") >>> #weight everything with flags !cutoff=0! >>> RG <- read.maimages(targets$FileName, source="genepix", >>> wt.fun=wtflags(cutoff=-50 weight=0)) >>> #read .gal file >>> #remove extra tab in file >>> >>> a <- readGAL() >> >> It is highly unlikely that you need to read a GAL file. ?The limma User's >> Guide tells you that you only need to do this with SPOT input, not with >> GenePix. >> >> It is obvious from the information you give that whatever GAL file you are >> reading, it doesn't match your GenePix files, because it has twice as many >> rows. >> >>> b <- a[,-6] >>> RG$genes<-b >>> #spot types file >>> spottypes <- readSpotTypes() >>> RG$genes$Status <- controlStatus(spottypes, RG$genes) >>> >>> ##################CHANGE weighting for spot types##################### >>> ###################################################################### >>> multiply <- c(1,0,2,0,1,0,1,1,1) >>> ###################################################################### >>> ###################################################################### >>> >>> a <- unique(RG$genes$ID) >>> status=RG$genes$Status >>> w <- modifyWeights(RG$weights, RG$genes$Status, a, c(0, 1)) >> >> Have you looked at the help page for modifyWeights? ?I'd think a quick read >> would tell you that your input arguments aren't the right dimensions, so >> there's no chance of this call working correctly. >> >> I also wonder what you're trying to achieve with modifyWeights, and whether >> you need it at all? ?This function is only needed for special situations. >> >> Best wishes >> Gordon >> >>> -- >>> Stephen Sefick >> >> ______________________________________________________________________ >> The information in this email is confidential and intended solely for the >> addressee. >> You must not disclose, forward, print or use it without the permission of >> the sender. >> ______________________________________________________________________ >> > > > > -- > Stephen Sefick > > Let's not spend our time and resources thinking about things that are > so little or so large that all they really do for us is puff us up and > make us feel like gods. We are mammals, and have not exhausted the > annoying little problems of being mammals. > > -K. Mullis > ______________________________________________________________________ The information in this email is confidential and intend...{{dropped:5}}
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