Problem with Beadarray package for beadchipHT-12
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Leo Nitsche ▴ 20
@leo-nitsche-3551
Last seen 10.2 years ago
Hi all, I have already obtained a data set from Illumina Beadchip-HT12 experience and I would like to analyse them in R with Beadarray package. I have files with the following extensions (.txt, .csv, .idat, .xml, .locs, .tiff) with a text file called Metrics. I guess that only two files are required (.txt and .tiff), right ? Now, I try to use the following script, wrote by Mark Dunning (thanks for him!) but I don't get what I should to get! Surely because the formats are not the same between the new HumanV3 beadchip I use and the previous one (HumanV2 for which the script was written) ! Here is the program and I will be grateful if somebody could tell me where in the script and what I have to change to adapt it my HumanHT12 beadchip? targets = read.table("targets.txt", sep = "\t", header = TRUE, as.is = TRUE) dir() targets = read.table("targets.txt", sep = "\t", header = TRUE, as.is = TRUE) Metrics = read.table("targets.txt", sep = "\t", header = TRUE, as.is=TRUE) Metrics = read.table("Metrics.txt", sep = "\t", header = TRUE, as.is=TRUE) Metrics BLData <- readIllumina(textType = ".csv", backgroundMethod = "none", targets = targets, arrayNames = targets$ArrayName, metrics = TRUE) BLData <- readIllumina(textType = ".csv", backgroundMethod = "none", Matrics = Matrics, arrayNames = Metrics$ArrayName, metrics = TRUE) is(BLData) class(BLData) slotNames(BLData) an = arrayNames(BLData) an names(BLData@beadData[[an[1]]]) BLData[[an[1]]]$G[1:10] BLData[[an[2]]]$Gb[1:10] pData(BLData) getArrayData(BLData, array = 1, what = "G", log = FALSE)[1:10] getArrayData(BLData, array = 2, what = "Gb", log = FALSE)[1:10] par(mfrow = c(1, 3)) boxplotBeads(BLData, las = 2, outline = FALSE, ylim = c(4, 12), main = "Foreground") boxplotBeads(BLData, las = 2, whatToPlot = "Gb", outline = FALSE, ylim = c(4, 12), main = "Background") BLData.bc = backgroundCorrect(BLData, method = "subtract") boxplotBeads(BLData.bc, las = 2, outline = FALSE, ylim = c(4, 12), main = "Background Corrected") ids = unique(BLData[[an[1]]]$ProbeID)[1:10] ids ProbeCols = rainbow(10) plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15)) ProbeCols = rainbow(10) > plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, + ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15))ProbeCols = rainbow(10) plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15)) o = findAllOutliers(BLData, array = 1) o[1:10] length(o)/numBeads(BLData)[1] par(mfrow = c(2, 1)) par(mar = c(1, 1, 3, 1)) for (i in 1:2) { o = findAllOutliers(BLData, array = i) plotBeadLocations(BLData, BeadIDs = o[1:1000], array = i, SAM = FALSE, cex = 0.5, col = "red", pch = 16) } par(mfrow = c(2, 1)) for (i in 1:2) { imageplot(BLData, array = i, nrow = 20, ncol = 200, zlim = range(9, 10), low = "yellow", high = "red", what = "G") } Thank you very much Leon [[alternative HTML version deleted]]
beadarray beadarray • 1.1k views
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@perry-moerland-1109
Last seen 2.7 years ago
Bioinformatics Laboratory, Academic Med…
Hi Leon, Could you tell us where your code stops working, include the error message, and also include a sessionInfo(), otherwise it will be hard to give you any input. best Perry Leo Nitsche wrote: > Hi all, > > > I have already obtained a data set from Illumina Beadchip-HT12 experience > and I would like to analyse them in R with Beadarray package. I have files > with the following extensions (.txt, .csv, .idat, .xml, .locs, .tiff) with a > text file called Metrics. I guess that only two files are required (.txt and > .tiff), right ? > Now, I try to use the following script, wrote by Mark Dunning (thanks for > him!) but I don't get what I should to get! Surely because the formats are > not the same between the new HumanV3 beadchip I use and the previous one > (HumanV2 for which the script was written) ! > Here is the program and I will be grateful if somebody could tell me where > in the script and what I have to change to adapt it my HumanHT12 beadchip? > > targets = read.table("targets.txt", sep = "\t", header = TRUE, > as.is = TRUE) > dir() > targets = read.table("targets.txt", sep = "\t", header = TRUE, > as.is = TRUE) > Metrics = read.table("targets.txt", sep = "\t", header = TRUE, > as.is=TRUE) > Metrics = read.table("Metrics.txt", sep = "\t", header = TRUE, > as.is=TRUE) > Metrics > BLData <- readIllumina(textType = ".csv", backgroundMethod = "none", > targets = targets, arrayNames = targets$ArrayName, metrics = TRUE) > BLData <- readIllumina(textType = ".csv", backgroundMethod = "none", > Matrics = Matrics, arrayNames = Metrics$ArrayName, metrics = TRUE) > is(BLData) > class(BLData) > slotNames(BLData) > an = arrayNames(BLData) > an > names(BLData at beadData[[an[1]]]) > BLData[[an[1]]]$G[1:10] > BLData[[an[2]]]$Gb[1:10] > pData(BLData) > getArrayData(BLData, array = 1, what = "G", log = FALSE)[1:10] > getArrayData(BLData, array = 2, what = "Gb", log = FALSE)[1:10] > par(mfrow = c(1, 3)) > boxplotBeads(BLData, las = 2, outline = FALSE, ylim = c(4, 12), > main = "Foreground") > boxplotBeads(BLData, las = 2, whatToPlot = "Gb", outline = FALSE, > ylim = c(4, 12), main = "Background") > BLData.bc = backgroundCorrect(BLData, method = "subtract") > boxplotBeads(BLData.bc, las = 2, outline = FALSE, ylim = c(4, > 12), main = "Background Corrected") > ids = unique(BLData[[an[1]]]$ProbeID)[1:10] > ids > ProbeCols = rainbow(10) > plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, > ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15)) > ProbeCols = rainbow(10) >> plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, > + ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15))ProbeCols = rainbow(10) > plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, > ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15)) > o = findAllOutliers(BLData, array = 1) > o[1:10] > length(o)/numBeads(BLData)[1] > par(mfrow = c(2, 1)) > par(mar = c(1, 1, 3, 1)) > for (i in 1:2) { > o = findAllOutliers(BLData, array = i) > plotBeadLocations(BLData, BeadIDs = o[1:1000], array = i, > SAM = FALSE, cex = 0.5, col = "red", pch = 16) > } > par(mfrow = c(2, 1)) > for (i in 1:2) { > imageplot(BLData, array = i, nrow = 20, ncol = 200, zlim = range(9, > 10), low = "yellow", high = "red", what = "G") > } > > > Thank you very much > > Leon > > [[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 > -- Perry Moerland, PhD Room J1B-206, Bioinformatics Laboratory Department of Clinical Epidemiology, Biostatistics and Bioinformatics Academic Medical Centre, University of Amsterdam Postbus 22660, 1100 DD Amsterdam, The Netherlands tel: +31 20 5664660 p.d.moerland at amc.uva.nl, http://www.amc.uva.nl/
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Hi Leon, What error message are you getting? The HumanHT-12 data should be in the exact same format as for earlier arrays. However, the bead-level intensities are probably found in the .txt files in your directory, unlike the example script where the bead-level intensities were in .csv files. Try the following. BLData <- readIllumina(backgroundMethod = "none", targets = targets, arrayNames = targets$ArrayName, metrics = TRUE, annoPkg="Humanv3") Best, Mark On Fri, Jul 3, 2009 at 1:08 PM, Perry Moerland<p.d.moerland at="" amc.uva.nl=""> wrote: > Hi Leon, > Could you tell us where your code stops working, include the error message, > and also include a sessionInfo(), otherwise it will be hard to give you any > input. > best > Perry > > Leo Nitsche wrote: >> >> Hi all, >> >> >> I have already obtained a data set from Illumina Beadchip-HT12 experience >> and I would like to analyse them in R with Beadarray package. I have files >> with the following extensions (.txt, .csv, .idat, .xml, .locs, .tiff) with >> a >> text file called Metrics. I guess that only two files are required (.txt >> and >> .tiff), right ? >> Now, I try to use the following script, wrote by Mark Dunning (thanks for >> him!) but I don't get what I should to get! Surely because the formats are >> not the same between the new HumanV3 beadchip I use and the previous one >> (HumanV2 for which the script was written) ! >> Here is the program and I will be grateful if somebody could tell me where >> in the script and what I have to change to adapt it my HumanHT12 beadchip? >> >> targets = read.table("targets.txt", sep = "\t", header = TRUE, >> as.is = TRUE) >> dir() >> targets = read.table("targets.txt", sep = "\t", header = TRUE, >> as.is = TRUE) >> Metrics = read.table("targets.txt", sep = "\t", header = TRUE, >> as.is=TRUE) >> Metrics = read.table("Metrics.txt", sep = "\t", header = TRUE, >> as.is=TRUE) >> Metrics >> BLData <- readIllumina(textType = ".csv", backgroundMethod = "none", >> targets = targets, arrayNames = targets$ArrayName, metrics = TRUE) >> ?BLData <- readIllumina(textType = ".csv", backgroundMethod = "none", >> Matrics = Matrics, arrayNames = Metrics$ArrayName, metrics = TRUE) >> is(BLData) >> class(BLData) >> slotNames(BLData) >> an = arrayNames(BLData) >> an >> names(BLData at beadData[[an[1]]]) >> BLData[[an[1]]]$G[1:10] >> BLData[[an[2]]]$Gb[1:10] >> pData(BLData) >> getArrayData(BLData, array = 1, what = "G", log = FALSE)[1:10] >> getArrayData(BLData, array = 2, what = "Gb", log = FALSE)[1:10] >> par(mfrow = c(1, 3)) >> boxplotBeads(BLData, las = 2, outline = FALSE, ylim = c(4, 12), >> main = "Foreground") >> boxplotBeads(BLData, las = 2, whatToPlot = "Gb", outline = FALSE, >> ylim = c(4, 12), main = "Background") >> BLData.bc = backgroundCorrect(BLData, method = "subtract") >> boxplotBeads(BLData.bc, las = 2, outline = FALSE, ylim = c(4, >> 12), main = "Background Corrected") >> ids = unique(BLData[[an[1]]]$ProbeID)[1:10] >> ids >> ProbeCols = rainbow(10) >> plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, >> ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15)) >> ProbeCols = rainbow(10) >>> >>> plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, >> >> + ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15))ProbeCols = >> rainbow(10) >> plotBeadIntensities(BLData, arrays = c(1, 3), ProbeIDs = ids, >> ProbeCols = ProbeCols, log = TRUE, ylim = c(8, 15)) >> o = findAllOutliers(BLData, array = 1) >> o[1:10] >> length(o)/numBeads(BLData)[1] >> par(mfrow = c(2, 1)) >> par(mar = c(1, 1, 3, 1)) >> for (i in 1:2) { >> o = findAllOutliers(BLData, array = i) >> plotBeadLocations(BLData, BeadIDs = o[1:1000], array = i, >> SAM = FALSE, cex = 0.5, col = "red", pch = 16) >> } >> par(mfrow = c(2, 1)) >> for (i in 1:2) { >> imageplot(BLData, array = i, nrow = 20, ncol = 200, zlim = range(9, >> 10), low = "yellow", high = "red", what = "G") >> } >> >> >> Thank you very much >> >> Leon >> >> ? ? ? ?[[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 >> > > > -- > Perry Moerland, PhD > Room J1B-206, Bioinformatics Laboratory > Department of Clinical Epidemiology, Biostatistics and Bioinformatics > Academic Medical Centre, University of Amsterdam > Postbus 22660, 1100 DD Amsterdam, The Netherlands > tel: +31 20 5664660 > p.d.moerland at amc.uva.nl, http://www.amc.uva.nl/ > > _______________________________________________ > 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 >
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