Entering edit mode
arnaud Le Cavorzin
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110
@arnaud-le-cavorzin-3364
Last seen 10.2 years ago
Hi.
Thank you for your anwser.
I have downloaded the last version of xps and performed the
metaProbesets with success.
So if I understand, xps use the same background correction algorithm
than Partek or APT. But the difference between these softwares seems
to be caused by the probes used for the background correction.
Moreover it seems to get a difference not only for the background
correction, but for the quantile normalization too, again due to the
different probes.
In fact I can't get the same results on my samples with xps package
and with Partek.
With Partek we found no expression differences for all of the genes
(after fdr correction), while xps found a little more than 1100 genes
who are differentially expressed (after using prefilter() and
unifilter() function, with the same options than in Partek).
And I don't know why.
Thank you for your help and your answer,
Best regards
Arnaud
> Date: Tue, 31 Mar 2009 22:04:42 +0200
> From: cstrato@aon.at
> To: arnaudlc@msn.com
> CC: bioconductor@stat.math.ethz.ch; delphine.rossille@chu-rennes.fr
> Subject: Re: [BioC] Xps package : errors and RMA difference with
Partek GS
>
> Dear Arnaud,
>
> Let me first answer your question how to export the background data
> (although an example is shown in vignette xps.pdf p.15):
>
> # 1. compute background (or rma)
> data.bg <- bgcorrect(data.exon, "ExonRMABgrdCore", filedir=datdir,
> method="rma", select="antigenomic",
option="pmonly:epanechnikov",
> params=c(16384), exonlevel="core")
>
> # 2. find background treenames for data.bg
> getTreeNames(rootFiledata.bg))
>
> # 3. get background for all trees
> export.root(rootFiledata.bg), schemeFiledata.bg),
setNamedata.bg),
> "*", "rbg", "fBg", "BgrdAll.txt")
> # or get background intensity for e.g. tree "BreastA.rbg"
> export.root(rootFiledata.bg), schemeFiledata.bg),
setNamedata.bg),
> "BreastA", "rbg", "fBg", "BgrdBreastA.txt")
>
> In addition you can also export the background subtracted
intensities:
> # 4. get background corrected intensities for all trees
> export.root(rootFiledata.bg), schemeFiledata.bg),
setNamedata.bg),
> "*", "int", "fInten", "IntenAll.txt")
>
> However, please note that only the "core" probes are corrected, so I
am
> not sure if you can use these data in another program.
>
>
> Some notes on background correction:
>
> Please note that the above background correction does NOT use
> "antigenomic" probes for background correction. The parameter
> select="antigenomic" does only define the kind of MM probes
(although
> they are not used in this case). Which probes are used as PM probes
is
> defined by exonlevel="core", which means that only "core" probes are
> used for background correction.
>
> As you know, in the RMA background algorithm observed PM probes are
> modeled as the sum of a normal noise component and an exponential
signal
> component. Since in above case only "core" probes are selected as PM
> probes, only these probes are used for background correction. This
may
> be the reason why the background data differ from the background
data
> computed by APT, as explained in vignette APTvsXPS.pdf.
>
> If you want to compute the background using "genomic" or
"antigenomic"
> probes and the APT algorithm based on GC content of these probes
then
> you need to use:
> data.bg <- bgcorrect(data.exon, "ExonGCBgrdCore", filedir=datdir,
> method="gccontent", select="antigenomic",
option="attenuatebg",
> params=c(0.4, 0.005, -1.0), exonlevel="core")
> or the dedicated function:
> data.bg <- bgcorrect.gc(data.exon, "ExonGCBgrdCore", filedir=datdir,
> select="antigenomic", exonlevel="core")
>
>
> Maybe one note on processing time:
> My main goal was to allow processing of exon arrays on computers
with
> 1GB RAM only, and to allow access to all interim data such as
background
> intensities and background-corrected probe intensities. Thus, all
these
> data are stored as root trees, which means that saving all these
interim
> data on HD is probably the time-consuming step.
>
> I hope that I could answer your questions.
>
> Best regards
> Christian
>
>
> arnaud Le Cavorzin wrote:
> > Hi
> >
> > Thank you for your answer, I will download your last version when
it
> > will be available.
> >
> > We found that the difference between Partek GS and xps package is
the
> > background correction.
> > And Partek's support confirmed that Partek GS doesn't use genomic
or
> > antigenomic background correction but correction like described by
> > Professor Bolstad.
> >
> > But I have an other problem : I would like to perform background
> > correction with xps, using the function bgcorrect(), and after to
> > export the data.bg.rma for performing the normalization and
> > summarization with Partek GS (that take less time than xps)
> > I have tried with function export.expr(), export.data and export()
> > without success.
> >
> > How can I do to extract the data.bg.rma into a .txt file, if it
was
> > possible of course?
> >
> > Thanks
> > Best regards
> >
> > Arnaud
> >
> >
> > > Date: Mon, 30 Mar 2009 22:33:48 +0200
> > > From: cstrato@aon.at
> > > To: arnaudlc@msn.com
> > > CC: bioconductor@stat.math.ethz.ch; delphine.rossille@chu-
rennes.fr
> > > Subject: Re: [BioC] Xps package : errors and RMA difference with
> > Partek GS
> > >
> > > Dear Arnaud,
> > >
> > > The error you get does only appear on Windows, since MS VC++
requires
> > > every C function used to be listed in an Export Definition File
> > > "xps.def". Since I have added this function later and do use
WinXP only
> > > for testing purposes, I have forgotten to add function
"MetaProbesets".
> > >
> > > I have just uploaded a new version xps_1.2.8 to BioC which adds
this
> > > function to xps.def.
> > > You should be able to download the new version in the next one
or
> > two days.
> > >
> > > Thank you for reporting this error. I am sorry for the
inconvenience.
> > >
> > > Best regards
> > > Christian
> > >
> > >
> > > arnaud Le Cavorzin wrote:
> > > > Hi
> > > >
> > > > I have tried to create a .mps file with xps. But I have got an
error,
> > > > in french
> > > > "Erreur dans .C("MetaProbesets", as.character(schemefile),
> > > > as.character(infile), :
> > > > le nom C de symbole "MetaProbesets" est introuvable dans la
DLL pour
> > > > le package "xps" "
> > > > That means that there is an error with the name C of symbol
> > > > MetaProbesets is missing into the ddl for the package xps.
> > > >
> > > > I don't understand what it mean, can you help me about this?
> > > >
> > > > The script used :
> > > >
> > > > /> xps.rma=validData(data.rma)
> > > > > writeLines(rownames(xps.rma),"core.txt")
> > > > > metaProbesets(scheme.huex10stv2r2,"core.txt","coreList.mps",
> > > > + exonlevel="core")/
> > > >
> > > > (I have performed a RMA with
> > > > background="antigenomic",option="transcript" and
exonlevel="core"
> > > > before this, for the comparison with APT and Partek GS)
> > > >
> > > > Thank you
> > > > Best regards
> > > >
> > > > Arnaud
> > > >
> > > >
> > > > > Date: Sat, 28 Mar 2009 23:03:21 +0100
> > > > > From: cstrato@aon.at
> > > > > To: arnaudlc@msn.com
> > > > > CC: bioconductor@stat.math.ethz.ch; delphine.rossille@chu-
rennes.fr
> > > > > Subject: Re: [BioC] Xps package : errors and RMA difference
with
> > > > Partek GS
> > > > >
> > > > > Dear Arnaud,
> > > > >
> > > > > Regarding the problem with "bgcorrect.rma()":
> > > > > Currently function "bgcorrect.rma()" works only with
expression
> > arrays,
> > > > > I will update it in the next version.
> > > > > At the moment you need to use the general function
"bgcorrect()"
> > with
> > > > > the correct settings.
> > > > >
> > > > > Thus if you want to compute RMA stepwise you need to do:
> > > > > ## 1.step: background - rma
> > > > > data.bg.rma <- bgcorrect(data.exon, "ExonRMABgrd",
filedir=datdir,
> > > > > method="rma", select="antigenomic",
option="pmonly:epanechnikov",
> > > > > params=c(16384), exonlevel="core")
> > > > >
> > > > > ## 2.step: normalization - quantile
> > > > > data.qu.rma <- normalize.quantiles(data.bg.rma,
"ExonRMANorm",
> > > > > filedir=datdir , exonlevel="core")
> > > > >
> > > > > ## 3.step: summarization - medpol
> > > > > data.mp.rma <- summarize.rma(data.qu.rma, "ExonRMASum",
> > filedir=datdir,
> > > > > exonlevel="core")
> > > > >
> > > > >
> > > > > This will give the same expression levels as using function
"rma()"
> > > > > directly:
> > > > > ## compute rma:
> > > > > data.rma <- rma(data.exon, "ExonRMAcore", filedir=datdir,
> > > > > background="antigenomic",
> > > > > normalize=T, option="transcript", exonlevel="core")
> > > > >
> > > > >
> > > > > Alternatively you can use function "express()" to compute
RMA:
> > > > > a, stepwise:
> > > > > ## 1.step: background - rma
> > > > > expr.bg.rma <- express(data.exon, "ExonExprsBgrd",
filedir=datdir,
> > > > > tmpdir="",
> > > > > bgcorrect.method="rma", bgcorrect.select="antigenomic",
> > > > > bgcorrect.option="pmonly:epanechnikov",
bgcorrect.params=c(16384),
> > > > > exonlevel="core")
> > > > >
> > > > > ## 2.step: normalization - quantile
> > > > > expr.qu.rma <- express(expr.bg.rma, "ExonExprsNorm",
filedir=datdir,
> > > > > tmpdir="",
> > > > > normalize.method="quantile", normalize.select="pmonly",
> > > > > normalize.option="transcript:together:none",
normalize.logbase="0",
> > > > > normalize.params=c(0.0), exonlevel="core")
> > > > >
> > > > > ## 3.step: summarization - medpol
> > > > > expr.mp.rma <- express(expr.qu.rma, "ExonExprsSum",
filedir=datdir,
> > > > > tmpdir="",
> > > > > summarize.method="medianpolish", summarize.select="pmonly",
> > > > > summarize.option="transcript", summarize.logbase="log2",
> > > > > summarize.params=c(10, 0.01, 1.0), exonlevel="core")
> > > > >
> > > > >
> > > > > b, with a single call to express()
> > > > > expr.rma <- express(data.exon, "ExonExprs", filedir=datdir,
> > tmpdir="",
> > > > > bgcorrect.method="rma", bgcorrect.select="antigenomic",
> > > > > bgcorrect.option="pmonly:epanechnikov",
bgcorrect.params=c(16384),
> > > > > normalize.method="quantile", normalize.select="pmonly",
> > > > > normalize.option="transcript:together:none",
normalize.logbase="0",
> > > > > normalize.params=c(0.0), summarize.method="medianpolish",
> > > > > summarize.select="pmonly", summarize.option="transcript",
> > > > > summarize.logbase="log2", summarize.params=c(10, 0.01, 1.0),
> > > > > exonlevel="core")
> > > > >
> > > > >
> > > > > I hope that these examples help you to use functions
bgcorrect(),
> > > > > normalize.quantiles(), summarize.rma() and express().
> > > > >
> > > > > Best regards
> > > > > Christian
> > > > >
> > > > >
> > > > > arnaud Le Cavorzin wrote:
> > > > > > Hi all.
> > > > > >
> > > > > > I'm a new user of the xps package and I have some
questions about
> > > > it and some problems.
> > > > > >
> > > > > > I use xps package for analysing exon arrays (using
Affymetrix
> > > > Human Exon 1.0 ST Arrays), and I try to compare the results
with the
> > > > results obtained with Partek GS.
> > > > > >
> > > > > > So for that in R I import .CEL files and perform a RMA
(using
> > > > function rma with xps). I have no problem with this step, it
works
> > but
> > > > I don't obtain the same results with Partek.
> > > > > > I have tried different options for rma (xps package) and
for
> > > > Partek (changing option=transcript or probeset, exonlevel=core
or
> > > > metacore in xps for example, and do the same thing in Partek)
but the
> > > > results are always differents.
> > > > > >
> > > > > > When I import the data from the .CEL files, all is ok, I
have the
> > > > same results with xps and Partek. But whenever I try a
normalization
> > > > (RMA) the results are different from the two softwares.
> > > > > > I have done for example :
> > > > > >
> > > > > >
> > > > > >>
> > > >
> > data.probesetnoback.rma=rma(data.huextest,"tmpdt_Huextestprobesetn
obackRMA",background="none",
> > > > > >>
> > > > > > +
normalize=TRUE,option="probeset",exonlevel="core",verbose=FALSE)
> > > > > >
> > > > > >>
> > > >
> > data.rma=rma(data.huextest,"tmpdt_HuextestRMA",background="antigen
omic",
> > > > > >>
> > > > > > +
normalize=TRUE,option="probeset",exonlevel="core",verbose=FALSE)
> > > > > >
> > > > > >>
> > > >
> > data.metacore.rma=rma(data.huextest,"tmpdt_HuextestprobesetnobackR
MA",background="antigenomic",
> > > > > >>
> > > > > > +
> >
normalize=TRUE,option="probeset",exonlevel="metacore",verbose=FALSE)
> > > > > >
> > > > > >
> > > > > > I have also tried with the xps package to perform a
background
> > > > correction first, after a quantile normalization and finally a
> > > > summarization for compare step by step with Partek but it
doesn't
> > work.
> > > > > >
> > > > > > I can't perform bgcorrect without error, like for example
:
> > > > > >
> > > > > >
> > > > > >>
> > > >
> > data.qu.rma=bgcorrect.rma(data.huextest,"tmpdt_HuextestbgqumpRMA",
filedir=getwd(),
> > > > > >>
> > > > > > + tmpdir="",exonlevel="core",verbose=FALSE)
> > > > > > Erreur dans .local(object, ...) : error in function
BgCorrect
> > > > > >
> > > > > >> traceback()
> > > > > >>
> > > > > > 6: stop(paste("error in function", sQuote("BgCorrect")))
> > > > > > 5: .local(object, ...)
> > > > > > 4: xpsBgCorrect(xps.data, filename = filename, filedir =
filedir,
> > > > > > tmpdir = tmpdir, update = update, select = select, method
=
> > method,
> > > > > > option = option, exonlevel = exonlevel, params = params,
> > > > > > verbose = verbose)
> > > > > > 3: xpsBgCorrect(xps.data, filename = filename, filedir =
filedir,
> > > > > > tmpdir = tmpdir, update = update, select = select, method
=
> > method,
> > > > > > option = option, exonlevel = exonlevel, params = params,
> > > > > > verbose = verbose)
> > > > > > 2: bgcorrect(xps.data, filename = filename, filedir =
filedir,
> > > > tmpdir = tmpdir,
> > > > > > update = update, select = "none", method = "rma", option =
> > > > "pmonly:epanechnikov",
> > > > > > exonlevel = exonlevel, params = c(16384), verbose =
verbose)
> > > > > > 1: bgcorrect.rma(data.huextest, "tmpdt_HuextestbgqumpRMA",
> > filedir
> > > > = getwd(),
> > > > > > tmpdir = "", exonlevel = "core", verbose = FALSE)
> > > > > >
> > > > > >>
data.bg.rma=bgcorrect(data.huextest,"tmpdt_HuextestbgqumpRMA",
> > > > filedir = getwd(), tmpdir = "",
> > > > select="none",method="rma",option="none",exonlevel = "core",
> > verbose =
> > > > FALSE)
> > > > > >>
> > > > > > Erreur dans .local(object, ...) : empty parameter list
params
> > > > > > De plus : Warning message:
> > > > > > In .local(object, ...) :
> > > > > > option is different from <pmonly:epanechnikov> for rma
> > > > > >
> > > > > >
> > > > > > If I perform a normalization.quantiles without performing
a
> > > > bgcorrect it doesn't work, I obtain 0 for all of the values.
> > > > > > And summarization give the same kind of error than
bgcorrect.
> > > > > >
> > > > > > Therefore my questions :
> > > > > >
> > > > > > Why xps pakage and R don't give the same results using the
same
> > > > setup options?
> > > > > > What does exactly xps when performing a RMA? A bgcorrect?
A
> > > > normalization?
> > > > > >
> > > > > > Thanks for your answer
> > > > > > Best regards
> > > > > >
> > > > > > Arnaud
> > > > > >
> > > > > >
> > > > > >
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