oneChannelGUI and Affymetrix 1.0 ST arrays
1
0
Entering edit mode
Steve Taylor ▴ 280
@steve-taylor-2838
Last seen 10.3 years ago
Hi, I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST arrays but I can't read in the data. I have two questions: 1) Why is this not working in OneChannelGUI? 2) If I can't get this to work, what are the best alternatives to read and normalise this data (to be subsequently analysed by LIMMA)? I have 12 CEL files: 1A.CEL 1B.CEL 2A.CEL 2B.CEL T10.CEL T11.CEL T12.CEL T3.CEL T4.CEL T5.CEL T6.CEL T7.CEL T8.CEL T9.CEL Using OneChannelGUI, when I try and read in the CEL files using rma- sketch or iter-plier I get Error in read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: no lines available in input and then various other errors in the Tk window. In my terminal window I get: Gene level probe sets summary started Read 12 cel files from: target327b23c6 Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 FATAL ERROR: Can't read file: 3.CEL Gene level probe sets summary ended Error in as.matrix(my.exons) : no function to return from, jumping to top level > sessionInfo() R version 2.10.1 (2009-12-14) x86_64-unknown-linux-gnu locale: [1] LC_CTYPE=en_GB.ISO-8859-1 LC_NUMERIC=C [3] LC_TIME=en_GB.ISO-8859-1 LC_COLLATE=en_GB.ISO-8859-1 [5] LC_MONETARY=C LC_MESSAGES=en_GB.ISO-8859-1 [7] LC_PAPER=en_GB.ISO-8859-1 LC_NAME=C [9] LC_ADDRESS=C LC_TELEPHONE=C [11] LC_MEASUREMENT=en_GB.ISO-8859-1 LC_IDENTIFICATION=C attached base packages: [1] tools tcltk stats graphics grDevices utils datasets [8] methods base other attached packages: [1] oneChannelGUI_1.12.5 preprocessCore_1.8.0 GOstats_2.12.0 [4] RSQLite_0.8-4 DBI_0.2-5 graph_1.24.4 [7] Category_2.12.0 AnnotationDbi_1.8.1 tkWidgets_1.24.0 [10] DynDoc_1.24.0 widgetTools_1.24.0 affylmGUI_1.20.0 [13] affyio_1.14.0 affy_1.24.2 limma_3.2.2 [16] Biobase_2.6.1 loaded via a namespace (and not attached): [1] annotate_1.24.1 genefilter_1.28.2 GO.db_2.3.5 GSEABase_1.8.0 [5] RBGL_1.22.0 splines_2.10.1 survival_2.35-8 XML_2.6-0 [9] xtable_1.5-6 Thanks very much for any help, Steve
GO probe oneChannelGUI GO probe oneChannelGUI • 1.9k views
ADD COMMENT
0
Entering edit mode
rcaloger ▴ 500
@rcaloger-1888
Last seen 9.9 years ago
European Union
Il 09/06/2010 12:00, bioconductor-request at stat.math.ethz.ch ha scritto: > Steve Taylor<stephen.taylor at="" imm.ox.ac.uk=""> > Dear Steve, there is some problem with the cel files you are using as indicated by the error: Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 This is an error from APT tools which are unable to read some of your CEL file. Furthermore, you must have an error in the target file used to load the data set, since the software try to read CEL file 3.CEL FATAL ERROR: Can't read file: 3.CEL but this is not present in the list of arrays you have indicated in the mail. To help you in solving your problem I need to know which are the arrays under analysis: human, mouse, rat gene, exon arrays To have an idea of the installation please write in the main R window: sessionInfo() affylmGUIenvironment$libDirLocation affylmGUIenvironment$aptDir and send the output to me. Cheers Raffaele >Hi, >I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST arrays but I can't read in the data. I have two questions: >1) Why is this not working in OneChannelGUI? >2) If I can't get this to work, what are the best alternatives to read and normalise this data (to be> >subsequently analysed by LIMMA)? >1A.CEL >1B.CEL >2A.CEL >2B.CEL >T10.CEL >T11.CEL >T12.CEL >T3.CEL >T4.CEL >T5.CEL >T6.CEL >T7.CEL >T8.CEL >T9.CEL >Using OneChannelGUI, when I try and read in the CEL files using>rma- sketch or iter-plier I get >Error in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >no lines available in input >and then various other errors in the Tk window. In my terminal window>I get: >Gene level probe sets summary started >Read 12 cel files from: target327b23c6 >Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >FATAL ERROR: Can't read file: 3.CEL -- ---------------------------------------- Prof. Raffaele A. Calogero Bioinformatics and Genomics Unit Dipartimento di Scienze Cliniche e Biologiche c/o Az. Ospedaliera S. Luigi Regione Gonzole 10, Orbassano 10043 Torino tel. ++39 0116705417 Lab. ++39 0116705408 Fax ++39 0119038639 Mobile ++39 3333827080 email: raffaele.calogero at unito.it raffaele[dot]calogero[at]gmail[dot]com www: http://www.bioinformatica.unito.it Info: http://publicationslist.org/raffaele.calogero
ADD COMMENT
0
Entering edit mode
DearRaffaele, >> > Dear Steve, > there is some problem with the cel files you are using as indicated by > the error: > > Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 > Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 > > This is an error from APT tools which are unable to read some of your > CEL file. > Furthermore, you must have an error in the target file used to load the > data set, since > the software try to read CEL file 3.CEL > > FATAL ERROR: Can't read file: 3.CEL This file definitely exists and is defined in the targets file... > > but this is not present in the list of arrays you have indicated in the > mail. > > To help you in solving your problem I need to know which are the arrays > under analysis: > human, mouse, rat > gene, exon arrays > Human Affymetrix Gene 1.0 ST array > sessionInfo() R version 2.10.1 (2009-12-14) x86_64-unknown-linux-gnu locale: [1] LC_CTYPE=en_GB.ISO-8859-1 LC_NUMERIC=C [3] LC_TIME=en_GB.ISO-8859-1 LC_COLLATE=en_GB.ISO-8859-1 [5] LC_MONETARY=C LC_MESSAGES=en_GB.ISO-8859-1 [7] LC_PAPER=en_GB.ISO-8859-1 LC_NAME=C [9] LC_ADDRESS=C LC_TELEPHONE=C [11] LC_MEASUREMENT=en_GB.ISO-8859-1 LC_IDENTIFICATION=C attached base packages: [1] tools tcltk stats graphics grDevices utils datasets [8] methods base other attached packages: [1] oneChannelGUI_1.12.5 preprocessCore_1.8.0 GOstats_2.12.0 [4] RSQLite_0.8-4 DBI_0.2-5 graph_1.24.4 [7] Category_2.12.0 AnnotationDbi_1.8.1 tkWidgets_1.24.0 [10] DynDoc_1.24.0 widgetTools_1.24.0 affylmGUI_1.20.0 [13] affyio_1.14.0 affy_1.24.2 limma_3.2.2 [16] Biobase_2.6.1 loaded via a namespace (and not attached): [1] annotate_1.24.1 genefilter_1.28.2 GO.db_2.3.5 GSEABase_1.8.0 [5] RBGL_1.22.0 splines_2.10.1 survival_2.35-8 XML_2.6-0 [9] xtable_1.5-6 > affylmGUIenvironment$libDirLocation [1] "/package/R/2.10.1/lib64/R/library/oneChannelGUI/affylibs" > affylmGUIenvironment$aptDir [1] "/package/apt/1.10.0-20080710" Thanks, Steve > To have an idea of the installation please write in the main R window: > sessionInfo() > affylmGUIenvironment$libDirLocation > affylmGUIenvironment$aptDir > > and send the output to me. > Cheers > Raffaele > > > >> Hi, > >> I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST arrays but I can't read in the data. I have two questions: > >> 1) Why is this not working in OneChannelGUI? >> 2) If I can't get this to work, what are the best alternatives to read and normalise this data (to be> >> subsequently analysed by LIMMA)? > >> 1A.CEL >> 1B.CEL >> 2A.CEL >> 2B.CEL >> T10.CEL >> T11.CEL >> T12.CEL >> T3.CEL >> T4.CEL >> T5.CEL >> T6.CEL >> T7.CEL >> T8.CEL >> T9.CEL >> Using OneChannelGUI, when I try and read in the CEL files using >rma-sketch or iter-plier I get > >> Error in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >> no lines available in input > >> and then various other errors in the Tk window. In my terminal window>I get: > >> Gene level probe sets summary started >> Read 12 cel files from: target327b23c6 >> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 > >> FATAL ERROR: Can't read file: 3.CEL
ADD REPLY
0
Entering edit mode
Hi Steve, thanks for the prompt answer. Actually you are using R 2.10.1 and the lastest oneChannelGUI is running on R 2.11 You need to update R and oneChannelGUi using the code at: http://www.bioinformatica.unito.it/oneChannelGUI/ <http: www.bioinformatica.unito.it="" onechannelgui=""/> The error you get is due to the fact that in the new release of oneChannelGUI, gene array in the 96 plate format can be also run and those arrays use a different set of library files, which are now embedded in the library files you are downloading from my web site when you run the first time an analysis with APT tools. In the previous version of oneChannelGUI this was not present and this produces the error you have found. Please let me know if everything is working after the new installation of R and bioconductor. Cheers Raffaele Il 09/06/2010 15:06, Steve Taylor ha scritto: > DearRaffaele, > >>> >> Dear Steve, >> there is some problem with the cel files you are using as indicated by >> the error: >> >> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >> >> This is an error from APT tools which are unable to read some of your >> CEL file. >> Furthermore, you must have an error in the target file used to load the >> data set, since >> the software try to read CEL file 3.CEL >> >> FATAL ERROR: Can't read file: 3.CEL > > This file definitely exists and is defined in the targets file... > >> >> but this is not present in the list of arrays you have indicated in the >> mail. >> >> To help you in solving your problem I need to know which are the arrays >> under analysis: >> human, mouse, rat >> gene, exon arrays >> > > Human Affymetrix Gene 1.0 ST array > >> sessionInfo() > R version 2.10.1 (2009-12-14) > x86_64-unknown-linux-gnu > > locale: > [1] LC_CTYPE=en_GB.ISO-8859-1 LC_NUMERIC=C > [3] LC_TIME=en_GB.ISO-8859-1 LC_COLLATE=en_GB.ISO-8859-1 > [5] LC_MONETARY=C LC_MESSAGES=en_GB.ISO-8859-1 > [7] LC_PAPER=en_GB.ISO-8859-1 LC_NAME=C > [9] LC_ADDRESS=C LC_TELEPHONE=C > [11] LC_MEASUREMENT=en_GB.ISO-8859-1 LC_IDENTIFICATION=C > > attached base packages: > [1] tools tcltk stats graphics grDevices utils datasets > [8] methods base > > other attached packages: > [1] oneChannelGUI_1.12.5 preprocessCore_1.8.0 GOstats_2.12.0 > [4] RSQLite_0.8-4 DBI_0.2-5 graph_1.24.4 > [7] Category_2.12.0 AnnotationDbi_1.8.1 tkWidgets_1.24.0 > [10] DynDoc_1.24.0 widgetTools_1.24.0 affylmGUI_1.20.0 > [13] affyio_1.14.0 affy_1.24.2 limma_3.2.2 > [16] Biobase_2.6.1 > > loaded via a namespace (and not attached): > [1] annotate_1.24.1 genefilter_1.28.2 GO.db_2.3.5 GSEABase_1.8.0 > [5] RBGL_1.22.0 splines_2.10.1 survival_2.35-8 XML_2.6-0 > [9] xtable_1.5-6 >> affylmGUIenvironment$libDirLocation > [1] "/package/R/2.10.1/lib64/R/library/oneChannelGUI/affylibs" >> affylmGUIenvironment$aptDir > [1] "/package/apt/1.10.0-20080710" > > Thanks, > > Steve > > > >> To have an idea of the installation please write in the main R window: >> sessionInfo() >> affylmGUIenvironment$libDirLocation >> affylmGUIenvironment$aptDir >> >> and send the output to me. >> Cheers >> Raffaele >> >> >> >>> Hi, >> >>> I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST >>> arrays but I can't read in the data. I have two questions: >> >>> 1) Why is this not working in OneChannelGUI? >>> 2) If I can't get this to work, what are the best alternatives to >>> read and normalise this data (to be> >>> subsequently analysed by LIMMA)? >> >>> 1A.CEL >>> 1B.CEL >>> 2A.CEL >>> 2B.CEL >>> T10.CEL >>> T11.CEL >>> T12.CEL >>> T3.CEL >>> T4.CEL >>> T5.CEL >>> T6.CEL >>> T7.CEL >>> T8.CEL >>> T9.CEL >>> Using OneChannelGUI, when I try and read in the CEL files >>> using>rma-sketch or iter-plier I get >> >>> Error >>> in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >>> no lines available in input >> >>> and then various other errors in the Tk window. In my terminal >>> window>I get: >> >>> Gene level probe sets summary started >>> Read 12 cel files from: target327b23c6 >>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >> >>> FATAL ERROR: Can't read file: 3.CEL > -- ---------------------------------------- Prof. Raffaele A. Calogero Bioinformatics and Genomics Unit Dipartimento di Scienze Cliniche e Biologiche c/o Az. Ospedaliera S. Luigi Regione Gonzole 10, Orbassano 10043 Torino tel. ++39 0116705417 Lab. ++39 0116705408 Fax ++39 0119038639 Mobile ++39 3333827080 email: raffaele.calogero@unito.it raffaele[dot]calogero[at]gmail[dot]com www: http://www.bioinformatica.unito.it Info: http://publicationslist.org/raffaele.calogero [[alternative HTML version deleted]]
ADD REPLY
0
Entering edit mode
Dear Raffaele, I do not think that this is an error from APT tools unable to read some of the CEL files. The output: Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 suggests that the PGF-file for HuGene-1_1-st-v1 was used and not the PGF-file for HuGene-1_0-st-v1: HuGene-1_0-st-v1 has a size of 1050 x 1050 = 1102500 HuGene-1_1-st-v1 has a size of 1190 x 990 = 1178100 Thus for 2A.CEL APT seems to require the PGF-file for HuGene- 1_0-st-v1. Best regards Christian _._._._._._._._._._._._._._._._._._ C.h.r.i.s.t.i.a.n S.t.r.a.t.o.w.a V.i.e.n.n.a A.u.s.t.r.i.a e.m.a.i.l: cstrato at aon.at _._._._._._._._._._._._._._._._._._ On 6/9/10 2:54 PM, rcaloger wrote: > Il 09/06/2010 12:00, bioconductor-request at stat.math.ethz.ch ha scritto: >> Steve Taylor<stephen.taylor at="" imm.ox.ac.uk=""> > Dear Steve, > there is some problem with the cel files you are using as indicated by > the error: > > Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 > Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 > > This is an error from APT tools which are unable to read some of your > CEL file. > Furthermore, you must have an error in the target file used to load the > data set, since > the software try to read CEL file 3.CEL > > FATAL ERROR: Can't read file: 3.CEL > > but this is not present in the list of arrays you have indicated in the > mail. > > To help you in solving your problem I need to know which are the arrays > under analysis: > human, mouse, rat > gene, exon arrays > > To have an idea of the installation please write in the main R window: > sessionInfo() > affylmGUIenvironment$libDirLocation > affylmGUIenvironment$aptDir > > and send the output to me. > Cheers > Raffaele > > > >> Hi, > >> I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST arrays >> but I can't read in the data. I have two questions: > >> 1) Why is this not working in OneChannelGUI? >> 2) If I can't get this to work, what are the best alternatives to read >> and normalise this data (to be> >> subsequently analysed by LIMMA)? > >> 1A.CEL >> 1B.CEL >> 2A.CEL >> 2B.CEL >> T10.CEL >> T11.CEL >> T12.CEL >> T3.CEL >> T4.CEL >> T5.CEL >> T6.CEL >> T7.CEL >> T8.CEL >> T9.CEL >> Using OneChannelGUI, when I try and read in the CEL files >> using>rma-sketch or iter-plier I get > >> Error in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >> no lines available in input > >> and then various other errors in the Tk window. In my terminal >> window>I get: > >> Gene level probe sets summary started >> Read 12 cel files from: target327b23c6 >> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 > >> FATAL ERROR: Can't read file: 3.CEL
ADD REPLY
0
Entering edit mode
Hi Christian, after Steve, sent me the sessionInfo() results, it came out that he was using onechannelGUI from Bioconductor release 2.5. oneChannelGUI released with Bioconductor 2.6 now allows to handle both normal gene arrays and 96 format gene arrays. For this reason in the library files that are associated to oneChannelGUI there are two different types of Gene array library files: HuGene-1_0-st-v1 and HuGene-1_1-st-v1 So I told Steve to upgrade the oneChannelGUI installation and the problem will be solved. Cheers Raffaele Il 09/06/2010 21:23, cstrato ha scritto: > Dear Raffaele, > > I do not think that this is an error from APT tools unable to read > some of the CEL files. > > The output: > Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 > suggests that the PGF-file for HuGene-1_1-st-v1 was used and not the > PGF-file for HuGene-1_0-st-v1: > > HuGene-1_0-st-v1 has a size of 1050 x 1050 = 1102500 > HuGene-1_1-st-v1 has a size of 1190 x 990 = 1178100 > > Thus for 2A.CEL APT seems to require the PGF-file for HuGene- 1_0-st-v1. > > Best regards > Christian > _._._._._._._._._._._._._._._._._._ > C.h.r.i.s.t.i.a.n S.t.r.a.t.o.w.a > V.i.e.n.n.a A.u.s.t.r.i.a > e.m.a.i.l: cstrato at aon.at > _._._._._._._._._._._._._._._._._._ > > > On 6/9/10 2:54 PM, rcaloger wrote: >> Il 09/06/2010 12:00, bioconductor-request at stat.math.ethz.ch ha scritto: >>> Steve Taylor<stephen.taylor at="" imm.ox.ac.uk=""> >> Dear Steve, >> there is some problem with the cel files you are using as indicated by >> the error: >> >> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >> >> This is an error from APT tools which are unable to read some of your >> CEL file. >> Furthermore, you must have an error in the target file used to load the >> data set, since >> the software try to read CEL file 3.CEL >> >> FATAL ERROR: Can't read file: 3.CEL >> >> but this is not present in the list of arrays you have indicated in the >> mail. >> >> To help you in solving your problem I need to know which are the arrays >> under analysis: >> human, mouse, rat >> gene, exon arrays >> >> To have an idea of the installation please write in the main R window: >> sessionInfo() >> affylmGUIenvironment$libDirLocation >> affylmGUIenvironment$aptDir >> >> and send the output to me. >> Cheers >> Raffaele >> >> >> >>> Hi, >> >>> I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST arrays >>> but I can't read in the data. I have two questions: >> >>> 1) Why is this not working in OneChannelGUI? >>> 2) If I can't get this to work, what are the best alternatives to read >>> and normalise this data (to be> >>> subsequently analysed by LIMMA)? >> >>> 1A.CEL >>> 1B.CEL >>> 2A.CEL >>> 2B.CEL >>> T10.CEL >>> T11.CEL >>> T12.CEL >>> T3.CEL >>> T4.CEL >>> T5.CEL >>> T6.CEL >>> T7.CEL >>> T8.CEL >>> T9.CEL >>> Using OneChannelGUI, when I try and read in the CEL files >>> using>rma-sketch or iter-plier I get >> >>> Error >>> in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >>> no lines available in input >> >>> and then various other errors in the Tk window. In my terminal >>> window>I get: >> >>> Gene level probe sets summary started >>> Read 12 cel files from: target327b23c6 >>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >> >>> FATAL ERROR: Can't read file: 3.CEL > -- ---------------------------------------- Prof. Raffaele A. Calogero Bioinformatics and Genomics Unit Dipartimento di Scienze Cliniche e Biologiche c/o Az. Ospedaliera S. Luigi Regione Gonzole 10, Orbassano 10043 Torino tel. ++39 0116705417 Lab. ++39 0116705408 Fax ++39 0119038639 Mobile ++39 3333827080 email: raffaele.calogero at unito.it raffaele[dot]calogero[at]gmail[dot]com www: http://www.bioinformatica.unito.it Info: http://publicationslist.org/raffaele.calogero
ADD REPLY
0
Entering edit mode
Hi, > after Steve, sent me the sessionInfo() results, it came out that he was > using onechannelGUI from Bioconductor release 2.5. oneChannelGUI > released with Bioconductor 2.6 now allows to handle both normal gene > arrays and 96 format gene arrays. For this reason in the library files > that are associated to oneChannelGUI there are two different types of > Gene array library files: > HuGene-1_0-st-v1 and HuGene-1_1-st-v1 > So I told Steve to upgrade the oneChannelGUI installation and the > problem will be solved. Thanks for your advice. I upgraded to the latest version of R/OneChannelGUI and it is basically working, though there seem to be a bug using Iter-plier. Here is the output when loading in the data using RMA-Sketch > Gene level probe sets summary started Read 12 cel files from: target79e2a9e3 Opening clf file: HuGene-1_0-st-v1.r4.clf Opening pgf file: HuGene-1_0-st-v1.r4.pgf Expecting 1 iteration. Doing iteration: 1 Opening clf file: HuGene-1_0-st-v1.r4.clf Opening pgf file: HuGene-1_0-st-v1.r4.pgf Loading 33297 probesets and 804955 probes. Reading 12 cel files............Done. Processing Probesets......................Done. Flushing output reporters. Finalizing output. Done. Cleaning up. Done. Run took approximately: 0.96 minute. But if I use Iter-plier Gene level probe sets summary started Read 12 cel files from: target1d4ed43b Opening bgp file: terminate called after throwing an instance of 'std::ios_base::failure' what(): basic_filebuf::underflow error reading the file Gene level probe sets summary ended Error in as.matrix(my.exons) : no function to return from, jumping to top level In addition: Warning messages: 1: In file(file, "rt") : only first element of 'description' argument used 2: In file(file, "rt") : only first element of 'description' argument used Also, is there anyway to change the font size in the QC steps (e.g. PCA plot/Dendrogram display)? Thanks again, Steve > Cheers > Raffaele > > > > Il 09/06/2010 21:23, cstrato ha scritto: >> Dear Raffaele, >> >> I do not think that this is an error from APT tools unable to read >> some of the CEL files. >> >> The output: >> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >> suggests that the PGF-file for HuGene-1_1-st-v1 was used and not the >> PGF-file for HuGene-1_0-st-v1: >> >> HuGene-1_0-st-v1 has a size of 1050 x 1050 = 1102500 >> HuGene-1_1-st-v1 has a size of 1190 x 990 = 1178100 >> >> Thus for 2A.CEL APT seems to require the PGF-file for HuGene- 1_0-st-v1. >> >> Best regards >> Christian >> _._._._._._._._._._._._._._._._._._ >> C.h.r.i.s.t.i.a.n S.t.r.a.t.o.w.a >> V.i.e.n.n.a A.u.s.t.r.i.a >> e.m.a.i.l: cstrato at aon.at >> _._._._._._._._._._._._._._._._._._ >> >> >> On 6/9/10 2:54 PM, rcaloger wrote: >>> Il 09/06/2010 12:00, bioconductor-request at stat.math.ethz.ch ha scritto: >>>> Steve Taylor<stephen.taylor at="" imm.ox.ac.uk=""> >>> Dear Steve, >>> there is some problem with the cel files you are using as indicated by >>> the error: >>> >>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>> >>> This is an error from APT tools which are unable to read some of your >>> CEL file. >>> Furthermore, you must have an error in the target file used to load the >>> data set, since >>> the software try to read CEL file 3.CEL >>> >>> FATAL ERROR: Can't read file: 3.CEL >>> >>> but this is not present in the list of arrays you have indicated in the >>> mail. >>> >>> To help you in solving your problem I need to know which are the arrays >>> under analysis: >>> human, mouse, rat >>> gene, exon arrays >>> >>> To have an idea of the installation please write in the main R window: >>> sessionInfo() >>> affylmGUIenvironment$libDirLocation >>> affylmGUIenvironment$aptDir >>> >>> and send the output to me. >>> Cheers >>> Raffaele >>> >>> >>> >>>> Hi, >>> >>>> I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST arrays >>>> but I can't read in the data. I have two questions: >>> >>>> 1) Why is this not working in OneChannelGUI? >>>> 2) If I can't get this to work, what are the best alternatives to read >>>> and normalise this data (to be> >>>> subsequently analysed by LIMMA)? >>> >>>> 1A.CEL >>>> 1B.CEL >>>> 2A.CEL >>>> 2B.CEL >>>> T10.CEL >>>> T11.CEL >>>> T12.CEL >>>> T3.CEL >>>> T4.CEL >>>> T5.CEL >>>> T6.CEL >>>> T7.CEL >>>> T8.CEL >>>> T9.CEL >>>> Using OneChannelGUI, when I try and read in the CEL files >>>> using>rma-sketch or iter-plier I get >>> >>>> Error >>>> in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >>>> no lines available in input >>> >>>> and then various other errors in the Tk window. In my terminal >>>> window>I get: >>> >>>> Gene level probe sets summary started >>>> Read 12 cel files from: target327b23c6 >>>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>> >>>> FATAL ERROR: Can't read file: 3.CEL >> > >
ADD REPLY
0
Entering edit mode
Glad to hear it working. I will investigate the problem related to the iter-plier usage. Cheers Raffaele Il 14/06/2010 14:52, Steve Taylor ha scritto: > Hi, > >> after Steve, sent me the sessionInfo() results, it came out that he was >> using onechannelGUI from Bioconductor release 2.5. oneChannelGUI >> released with Bioconductor 2.6 now allows to handle both normal gene >> arrays and 96 format gene arrays. For this reason in the library files >> that are associated to oneChannelGUI there are two different types of >> Gene array library files: >> HuGene-1_0-st-v1 and HuGene-1_1-st-v1 >> So I told Steve to upgrade the oneChannelGUI installation and the >> problem will be solved. > > Thanks for your advice. > > I upgraded to the latest version of R/OneChannelGUI and it is > basically working, though there seem to be a bug using Iter-plier. > > Here is the output when loading in the data using RMA-Sketch >> > Gene level probe sets summary started > Read 12 cel files from: target79e2a9e3 > Opening clf file: HuGene-1_0-st-v1.r4.clf > Opening pgf file: HuGene-1_0-st-v1.r4.pgf > Expecting 1 iteration. > Doing iteration: 1 > Opening clf file: HuGene-1_0-st-v1.r4.clf > Opening pgf file: HuGene-1_0-st-v1.r4.pgf > Loading 33297 probesets and 804955 probes. > Reading 12 cel files............Done. > Processing Probesets......................Done. > Flushing output reporters. Finalizing output. > Done. > Cleaning up. > Done. > Run took approximately: 0.96 minute. > > But if I use Iter-plier > > Gene level probe sets summary started > Read 12 cel files from: target1d4ed43b > Opening bgp file: > terminate called after throwing an instance of 'std::ios_base::failure' > what(): basic_filebuf::underflow error reading the file > > Gene level probe sets summary ended > Error in as.matrix(my.exons) : > no function to return from, jumping to top level > In addition: Warning messages: > 1: In file(file, "rt") : only first element of 'description' argument > used > 2: In file(file, "rt") : only first element of 'description' argument > used > > Also, is there anyway to change the font size in the QC steps (e.g. > PCA plot/Dendrogram display)? > > Thanks again, > > Steve > > >> Cheers >> Raffaele >> >> >> >> Il 09/06/2010 21:23, cstrato ha scritto: >>> Dear Raffaele, >>> >>> I do not think that this is an error from APT tools unable to read >>> some of the CEL files. >>> >>> The output: >>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>> suggests that the PGF-file for HuGene-1_1-st-v1 was used and not the >>> PGF-file for HuGene-1_0-st-v1: >>> >>> HuGene-1_0-st-v1 has a size of 1050 x 1050 = 1102500 >>> HuGene-1_1-st-v1 has a size of 1190 x 990 = 1178100 >>> >>> Thus for 2A.CEL APT seems to require the PGF-file for HuGene- 1_0-st-v1. >>> >>> Best regards >>> Christian >>> _._._._._._._._._._._._._._._._._._ >>> C.h.r.i.s.t.i.a.n S.t.r.a.t.o.w.a >>> V.i.e.n.n.a A.u.s.t.r.i.a >>> e.m.a.i.l: cstrato at aon.at >>> _._._._._._._._._._._._._._._._._._ >>> >>> >>> On 6/9/10 2:54 PM, rcaloger wrote: >>>> Il 09/06/2010 12:00, bioconductor-request at stat.math.ethz.ch ha >>>> scritto: >>>>> Steve Taylor<stephen.taylor at="" imm.ox.ac.uk=""> >>>> Dear Steve, >>>> there is some problem with the cel files you are using as indicated by >>>> the error: >>>> >>>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>>> >>>> This is an error from APT tools which are unable to read some of your >>>> CEL file. >>>> Furthermore, you must have an error in the target file used to load >>>> the >>>> data set, since >>>> the software try to read CEL file 3.CEL >>>> >>>> FATAL ERROR: Can't read file: 3.CEL >>>> >>>> but this is not present in the list of arrays you have indicated in >>>> the >>>> mail. >>>> >>>> To help you in solving your problem I need to know which are the >>>> arrays >>>> under analysis: >>>> human, mouse, rat >>>> gene, exon arrays >>>> >>>> To have an idea of the installation please write in the main R window: >>>> sessionInfo() >>>> affylmGUIenvironment$libDirLocation >>>> affylmGUIenvironment$aptDir >>>> >>>> and send the output to me. >>>> Cheers >>>> Raffaele >>>> >>>> >>>> >>>>> Hi, >>>> >>>>> I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST >>>>> arrays >>>>> but I can't read in the data. I have two questions: >>>> >>>>> 1) Why is this not working in OneChannelGUI? >>>>> 2) If I can't get this to work, what are the best alternatives to >>>>> read >>>>> and normalise this data (to be> >>>>> subsequently analysed by LIMMA)? >>>> >>>>> 1A.CEL >>>>> 1B.CEL >>>>> 2A.CEL >>>>> 2B.CEL >>>>> T10.CEL >>>>> T11.CEL >>>>> T12.CEL >>>>> T3.CEL >>>>> T4.CEL >>>>> T5.CEL >>>>> T6.CEL >>>>> T7.CEL >>>>> T8.CEL >>>>> T9.CEL >>>>> Using OneChannelGUI, when I try and read in the CEL files >>>>> using>rma-sketch or iter-plier I get >>>> >>>>> Error >>>>> in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >>>>> no lines available in input >>>> >>>>> and then various other errors in the Tk window. In my terminal >>>>> window>I get: >>>> >>>>> Gene level probe sets summary started >>>>> Read 12 cel files from: target327b23c6 >>>>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>>>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>>> >>>>> FATAL ERROR: Can't read file: 3.CEL >>> >> >> > -- ---------------------------------------- Prof. Raffaele A. Calogero Bioinformatics and Genomics Unit Dipartimento di Scienze Cliniche e Biologiche c/o Az. Ospedaliera S. Luigi Regione Gonzole 10, Orbassano 10043 Torino tel. ++39 0116705417 Lab. ++39 0116705408 Fax ++39 0119038639 Mobile ++39 3333827080 email: raffaele.calogero at unito.it raffaele[dot]calogero[at]gmail[dot]com www: http://www.bioinformatica.unito.it Info: http://publicationslist.org/raffaele.calogero
ADD REPLY
0
Entering edit mode
Hi Steve, many thanks for the bug report. The bug in the usage of iter-plier summarization for gene arrays is fixed in oneChannelGUI 1.14.4, which should be available in a 24 hours on the bioconductor web Cheer Raffaele Il 14/06/2010 14:52, Steve Taylor ha scritto: > Hi, > >> after Steve, sent me the sessionInfo() results, it came out that he was >> using onechannelGUI from Bioconductor release 2.5. oneChannelGUI >> released with Bioconductor 2.6 now allows to handle both normal gene >> arrays and 96 format gene arrays. For this reason in the library files >> that are associated to oneChannelGUI there are two different types of >> Gene array library files: >> HuGene-1_0-st-v1 and HuGene-1_1-st-v1 >> So I told Steve to upgrade the oneChannelGUI installation and the >> problem will be solved. > > Thanks for your advice. > > I upgraded to the latest version of R/OneChannelGUI and it is > basically working, though there seem to be a bug using Iter-plier. > > Here is the output when loading in the data using RMA-Sketch >> > Gene level probe sets summary started > Read 12 cel files from: target79e2a9e3 > Opening clf file: HuGene-1_0-st-v1.r4.clf > Opening pgf file: HuGene-1_0-st-v1.r4.pgf > Expecting 1 iteration. > Doing iteration: 1 > Opening clf file: HuGene-1_0-st-v1.r4.clf > Opening pgf file: HuGene-1_0-st-v1.r4.pgf > Loading 33297 probesets and 804955 probes. > Reading 12 cel files............Done. > Processing Probesets......................Done. > Flushing output reporters. Finalizing output. > Done. > Cleaning up. > Done. > Run took approximately: 0.96 minute. > > But if I use Iter-plier > > Gene level probe sets summary started > Read 12 cel files from: target1d4ed43b > Opening bgp file: > terminate called after throwing an instance of 'std::ios_base::failure' > what(): basic_filebuf::underflow error reading the file > > Gene level probe sets summary ended > Error in as.matrix(my.exons) : > no function to return from, jumping to top level > In addition: Warning messages: > 1: In file(file, "rt") : only first element of 'description' argument > used > 2: In file(file, "rt") : only first element of 'description' argument > used > > Also, is there anyway to change the font size in the QC steps (e.g. > PCA plot/Dendrogram display)? > > Thanks again, > > Steve > > >> Cheers >> Raffaele >> >> >> >> Il 09/06/2010 21:23, cstrato ha scritto: >>> Dear Raffaele, >>> >>> I do not think that this is an error from APT tools unable to read >>> some of the CEL files. >>> >>> The output: >>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>> suggests that the PGF-file for HuGene-1_1-st-v1 was used and not the >>> PGF-file for HuGene-1_0-st-v1: >>> >>> HuGene-1_0-st-v1 has a size of 1050 x 1050 = 1102500 >>> HuGene-1_1-st-v1 has a size of 1190 x 990 = 1178100 >>> >>> Thus for 2A.CEL APT seems to require the PGF-file for HuGene- 1_0-st-v1. >>> >>> Best regards >>> Christian >>> _._._._._._._._._._._._._._._._._._ >>> C.h.r.i.s.t.i.a.n S.t.r.a.t.o.w.a >>> V.i.e.n.n.a A.u.s.t.r.i.a >>> e.m.a.i.l: cstrato at aon.at >>> _._._._._._._._._._._._._._._._._._ >>> >>> >>> On 6/9/10 2:54 PM, rcaloger wrote: >>>> Il 09/06/2010 12:00, bioconductor-request at stat.math.ethz.ch ha >>>> scritto: >>>>> Steve Taylor<stephen.taylor at="" imm.ox.ac.uk=""> >>>> Dear Steve, >>>> there is some problem with the cel files you are using as indicated by >>>> the error: >>>> >>>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>>> >>>> This is an error from APT tools which are unable to read some of your >>>> CEL file. >>>> Furthermore, you must have an error in the target file used to load >>>> the >>>> data set, since >>>> the software try to read CEL file 3.CEL >>>> >>>> FATAL ERROR: Can't read file: 3.CEL >>>> >>>> but this is not present in the list of arrays you have indicated in >>>> the >>>> mail. >>>> >>>> To help you in solving your problem I need to know which are the >>>> arrays >>>> under analysis: >>>> human, mouse, rat >>>> gene, exon arrays >>>> >>>> To have an idea of the installation please write in the main R window: >>>> sessionInfo() >>>> affylmGUIenvironment$libDirLocation >>>> affylmGUIenvironment$aptDir >>>> >>>> and send the output to me. >>>> Cheers >>>> Raffaele >>>> >>>> >>>> >>>>> Hi, >>>> >>>>> I am trying use oneChannelGUI to analyse some Affymetrix 1.0 ST >>>>> arrays >>>>> but I can't read in the data. I have two questions: >>>> >>>>> 1) Why is this not working in OneChannelGUI? >>>>> 2) If I can't get this to work, what are the best alternatives to >>>>> read >>>>> and normalise this data (to be> >>>>> subsequently analysed by LIMMA)? >>>> >>>>> 1A.CEL >>>>> 1B.CEL >>>>> 2A.CEL >>>>> 2B.CEL >>>>> T10.CEL >>>>> T11.CEL >>>>> T12.CEL >>>>> T3.CEL >>>>> T4.CEL >>>>> T5.CEL >>>>> T6.CEL >>>>> T7.CEL >>>>> T8.CEL >>>>> T9.CEL >>>>> Using OneChannelGUI, when I try and read in the CEL files >>>>> using>rma-sketch or iter-plier I get >>>> >>>>> Error >>>>> in>read.table(paste(tempOut,"/",content.outDir[tempOut1],sep=""),: >>>>> no lines available in input >>>> >>>>> and then various other errors in the Tk window. In my terminal >>>>> window>I get: >>>> >>>>> Gene level probe sets summary started >>>>> Read 12 cel files from: target327b23c6 >>>>> Wrong number of cells: Expecting: 1178100 and 1A.CEL has: 1102500 >>>>> Wrong number of cells: Expecting: 1178100 and 2A.CEL has: 1102500 >>>> >>>>> FATAL ERROR: Can't read file: 3.CEL >>> >> >> > -- ---------------------------------------- Prof. Raffaele A. Calogero Bioinformatics and Genomics Unit Dipartimento di Scienze Cliniche e Biologiche c/o Az. Ospedaliera S. Luigi Regione Gonzole 10, Orbassano 10043 Torino tel. ++39 0116705417 Lab. ++39 0116705408 Fax ++39 0119038639 Mobile ++39 3333827080 email: raffaele.calogero at unito.it raffaele[dot]calogero[at]gmail[dot]com www: http://www.bioinformatica.unito.it Info: http://publicationslist.org/raffaele.calogero
ADD REPLY

Login before adding your answer.

Traffic: 322 users visited in the last hour
Help About
FAQ
Access RSS
API
Stats

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by the version 2.3.6