different normalized results using oneChannelGUI, and oligo packages
1
0
Entering edit mode
rcaloger ▴ 500
@rcaloger-1888
Last seen 9.9 years ago
European Union
Hi, dear Benilton, you are right oneChannelGUI uses sketch-quantile. APT-tools are used by oneChannelGUI to calculate intensities. Actually oneChannelGUI uses a graphical interface to execute apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m MPSFILE.mps -out rmasketch *.cel cheers Raffaele >Javier, >my knowledge on the oneChannelGUI is pretty limited, but it seems to >me that it does either rma-sketch or iter-plier. >oligo will do the "regular" rma, ie. no sketch normalization. Now, if >you could download APT and run it yourself (I'm not sure how it is >packaged in oneChannel), you could try the following: >apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m MPSFILE.mps -out rmasketch *.cel >And you may get more similar results... I'm not saying they'll be >identical, but when I implemented this for oligo the mean relative >difference between oligo and APT was something like 0.001. b On Nov 10, 2009, at 3:30 PM, Javier P?rez Florido wrote: > > Dear all, > > I have normalized a GeneChip Human Gene ST 1.0 dataset using oligo > > package and oneChannelGUI. I've checked that the log2 normalized > > values > > are different (not so different, but different). When applying limma > > on > > them, the statistic values (p-value, M, B and statistic t) are also > > different. > > > > I've read that oneChannelGUI uses APT tools to summarize data and, > > maybe, that is the point: they produce similar but different > > normalized > > values that have an effect in the final list of differentially > > expressed > > genes. > > > > For oligo, I've normalized using rma method and core as a target: > > OligoEset<-rma(OligoRaw,target="core") > > For oneChannelGUI, I've used the option "Load gene 1.0 ST arrays from > > .CEL files." > > > > In both cases, the limma parameters are the same. > > So, I suspect the APT tools used by oneChannelGUI has influence on the > > data. Is there a way to normalize the raw data in OneChannelGUI to > > select the subgroup (core) instead of using APT tools? I think this is > > only available in Exon Arrays. > > > > Or may be I am wrong with these conclusions. > > Any tips? > > Thanks, > > Javier > > > -- ---------------------------------------- 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
Normalization limma oligo oneChannelGUI Normalization limma oligo oneChannelGUI • 1.4k views
ADD COMMENT
0
Entering edit mode
@benilton-carvalho-1375
Last seen 4.7 years ago
Brazil/Campinas/UNICAMP
Thanks for the heads up, Raffaele. My suggestion was Javier to try "-a rma" manually, instead of "-a rma- sketch" (which appears to be what oneChannelGUI uses - at least that's what I saw when skimmed the source ). cheers, b On Nov 12, 2009, at 6:32 AM, rcaloger wrote: > Hi, > dear Benilton, > you are right oneChannelGUI uses sketch-quantile. APT-tools are used > by oneChannelGUI to calculate intensities. > Actually oneChannelGUI uses a graphical interface to execute > apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m > MPSFILE.mps -out rmasketch *.cel > cheers > Raffaele > > >> Javier, > >> my knowledge on the oneChannelGUI is pretty limited, but it seems to >> me that it does either rma-sketch or iter-plier. > >> oligo will do the "regular" rma, ie. no sketch normalization. Now, if >> you could download APT and run it yourself (I'm not sure how it is >> packaged in oneChannel), you could try the following: > >> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m > MPSFILE.mps -out rmasketch *.cel > >> And you may get more similar results... I'm not saying they'll be >> identical, but when I implemented this for oligo the mean relative >> difference between oligo and APT was something like 0.001. > > b > > On Nov 10, 2009, at 3:30 PM, Javier P?rez Florido wrote: > > >>> Dear all, >>> I have normalized a GeneChip Human Gene ST 1.0 dataset using oligo >>> package and oneChannelGUI. I've checked that the log2 normalized >>> values >>> are different (not so different, but different). When applying limma >>> on >>> them, the statistic values (p-value, M, B and statistic t) are also >>> different. >>> >>> I've read that oneChannelGUI uses APT tools to summarize data and, >>> maybe, that is the point: they produce similar but different >>> normalized >>> values that have an effect in the final list of differentially >>> expressed >>> genes. >>> >>> For oligo, I've normalized using rma method and core as a target: >>> OligoEset<-rma(OligoRaw,target="core") >>> For oneChannelGUI, I've used the option "Load gene 1.0 ST arrays >>> from >>> .CEL files." >>> >>> In both cases, the limma parameters are the same. >>> So, I suspect the APT tools used by oneChannelGUI has influence on >>> the >>> data. Is there a way to normalize the raw data in OneChannelGUI to >>> select the subgroup (core) instead of using APT tools? I think >>> this is >>> only available in Exon Arrays. >>> >>> Or may be I am wrong with these conclusions. >>> Any tips? >>> Thanks, >>> Javier >>> >> > -- > > ---------------------------------------- > 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
Dear Benilton and Raffaele, I've tried what you suggested and I got the following results: * Comparison between rma and rma-sketch using APT tools: o apt-probeset-summarize -a rma -p Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma --cel-files cel_list.txt o apt-probeset-summarize -a rma-sketch -p Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma-sketch --cel-files cel_list.txt The error given by abs(exprs(rma)-exprs(rma-sketch)) / num_points is 1.4147e-004 * Comparison between rma using APT tools and rma using oligo: o apt-probeset-summarize -a rma -p Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma --cel-files cel_list.txt o OligoEset<-rma(OligoRaw,target="core") The error given by abs(exprs(rma)-exprs(OligoEset)) / num_points is 1.8915 * Comparison between rma-sketch using APT tools and rma using oligo: o apt-probeset-summarize -a rma-sketch -p Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma --cel-files cel_list.txt o OligoEset<-rma(OligoRaw,target="core") The mean error given by abs(exprs(rma-sketch)-exprs(OligoEset)) / num_points is 1.8915 Surprisingly, the difference between APT tools and oligo are quite high (you can notice it when having a look at the normalized data). Is there anything wrong above? Thanks, Javier Benilton Carvalho escribió: > Thanks for the heads up, Raffaele. > > My suggestion was Javier to try "-a rma" manually, instead of "-a > rma-sketch" (which appears to be what oneChannelGUI uses - at least > that's what I saw when skimmed the source ). > > cheers, > > b > > On Nov 12, 2009, at 6:32 AM, rcaloger wrote: > >> Hi, >> dear Benilton, >> you are right oneChannelGUI uses sketch-quantile. APT-tools are used >> by oneChannelGUI to calculate intensities. >> Actually oneChannelGUI uses a graphical interface to execute >> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m >> MPSFILE.mps -out rmasketch *.cel >> cheers >> Raffaele >> >> >>> Javier, >> >>> my knowledge on the oneChannelGUI is pretty limited, but it seems to >>> me that it does either rma-sketch or iter-plier. >> >>> oligo will do the "regular" rma, ie. no sketch normalization. Now, if >>> you could download APT and run it yourself (I'm not sure how it is >>> packaged in oneChannel), you could try the following: >> >>> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m >> MPSFILE.mps -out rmasketch *.cel >> >>> And you may get more similar results... I'm not saying they'll be >>> identical, but when I implemented this for oligo the mean relative >>> difference between oligo and APT was something like 0.001. >> >> b >> >> On Nov 10, 2009, at 3:30 PM, Javier P?rez Florido wrote: >> >> >>>> Dear all, >>>> I have normalized a GeneChip Human Gene ST 1.0 dataset using oligo >>>> package and oneChannelGUI. I've checked that the log2 normalized >>>> values >>>> are different (not so different, but different). When applying limma >>>> on >>>> them, the statistic values (p-value, M, B and statistic t) are also >>>> different. >>>> >>>> I've read that oneChannelGUI uses APT tools to summarize data and, >>>> maybe, that is the point: they produce similar but different >>>> normalized >>>> values that have an effect in the final list of differentially >>>> expressed >>>> genes. >>>> >>>> For oligo, I've normalized using rma method and core as a target: >>>> OligoEset<-rma(OligoRaw,target="core") >>>> For oneChannelGUI, I've used the option "Load gene 1.0 ST arrays from >>>> .CEL files." >>>> >>>> In both cases, the limma parameters are the same. >>>> So, I suspect the APT tools used by oneChannelGUI has influence on the >>>> data. Is there a way to normalize the raw data in OneChannelGUI to >>>> select the subgroup (core) instead of using APT tools? I think this is >>>> only available in Exon Arrays. >>>> >>>> Or may be I am wrong with these conclusions. >>>> Any tips? >>>> Thanks, >>>> Javier >>>> >>> >> -- >> >> ---------------------------------------- >> 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
Are you sure the probesets are in the same order? Instead of (A-B)/N, you could use all.equal(A,B), which will also assess dimnames, especially important in this case (because you'll be able to notice if the probesets are alligned). When I first wrote the code I did this comparison myself and the relative difference was something like 1e-4. So, my guess: probesets are misaligned. Best, b On Nov 16, 2009, at 8:00 AM, Javier Pérez Florido wrote: > Dear Benilton and Raffaele, > I've tried what you suggested and I got the following results: > Comparison between rma and rma-sketch using APT tools: > apt-probeset-summarize -a rma -p Hugene-1_0-st-v1.r3.pgf -c > Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma --cel- > files cel_list.txt > apt-probeset-summarize -a rma-sketch -p Hugene-1_0-st-v1.r3.pgf -c > Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma-sketch -- > cel-files cel_list.txt > The error given by abs(exprs(rma)-exprs(rma-sketch)) / num_points is > 1.4147e-004 > Comparison between rma using APT tools and rma using oligo: > apt-probeset-summarize -a rma -p Hugene-1_0-st-v1.r3.pgf -c > Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma --cel- > files cel_list.txt > OligoEset<-rma(OligoRaw,target="core") > The error given by abs(exprs(rma)-exprs(OligoEset)) / num_points is > 1.8915 > Comparison between rma-sketch using APT tools and rma using oligo: > apt-probeset-summarize -a rma-sketch -p Hugene-1_0-st-v1.r3.pgf -c > Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma --cel- > files cel_list.txt > OligoEset<-rma(OligoRaw,target="core") > The mean error given by abs(exprs(rma-sketch)-exprs(OligoEset)) / > num_points is 1.8915 > Surprisingly, the difference between APT tools and oligo are quite > high (you can notice it when having a look at the normalized data). > Is there anything wrong above? > Thanks, > Javier > > > > Benilton Carvalho escribió: >> >> Thanks for the heads up, Raffaele. >> >> My suggestion was Javier to try "-a rma" manually, instead of "-a >> rma-sketch" (which appears to be what oneChannelGUI uses - at least >> that's what I saw when skimmed the source ). >> >> cheers, >> >> b >> >> On Nov 12, 2009, at 6:32 AM, rcaloger wrote: >> >>> Hi, >>> dear Benilton, >>> you are right oneChannelGUI uses sketch-quantile. APT-tools are >>> used by oneChannelGUI to calculate intensities. >>> Actually oneChannelGUI uses a graphical interface to execute >>> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m >>> MPSFILE.mps -out rmasketch *.cel >>> cheers >>> Raffaele >>> >>> >>>> Javier, >>> >>>> my knowledge on the oneChannelGUI is pretty limited, but it seems >>>> to >>>> me that it does either rma-sketch or iter-plier. >>> >>>> oligo will do the "regular" rma, ie. no sketch normalization. >>>> Now, if >>>> you could download APT and run it yourself (I'm not sure how it is >>>> packaged in oneChannel), you could try the following: >>> >>>> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m >>> MPSFILE.mps -out rmasketch *.cel >>> >>>> And you may get more similar results... I'm not saying they'll be >>>> identical, but when I implemented this for oligo the mean relative >>>> difference between oligo and APT was something like 0.001. >>> >>> b >>> >>> On Nov 10, 2009, at 3:30 PM, Javier P?rez Florido wrote: >>> >>> >>>>> Dear all, >>>>> I have normalized a GeneChip Human Gene ST 1.0 dataset using oligo >>>>> package and oneChannelGUI. I've checked that the log2 normalized >>>>> values >>>>> are different (not so different, but different). When applying >>>>> limma >>>>> on >>>>> them, the statistic values (p-value, M, B and statistic t) are >>>>> also >>>>> different. >>>>> >>>>> I've read that oneChannelGUI uses APT tools to summarize data and, >>>>> maybe, that is the point: they produce similar but different >>>>> normalized >>>>> values that have an effect in the final list of differentially >>>>> expressed >>>>> genes. >>>>> >>>>> For oligo, I've normalized using rma method and core as a target: >>>>> OligoEset<-rma(OligoRaw,target="core") >>>>> For oneChannelGUI, I've used the option "Load gene 1.0 ST arrays >>>>> from >>>>> .CEL files." >>>>> >>>>> In both cases, the limma parameters are the same. >>>>> So, I suspect the APT tools used by oneChannelGUI has influence >>>>> on the >>>>> data. Is there a way to normalize the raw data in OneChannelGUI to >>>>> select the subgroup (core) instead of using APT tools? I think >>>>> this is >>>>> only available in Exon Arrays. >>>>> >>>>> Or may be I am wrong with these conclusions. >>>>> Any tips? >>>>> Thanks, >>>>> Javier >>>>> >>>> >>> -- >>> >>> ---------------------------------------- >>> 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 Benilton, Sorry, you were right. I was too confident (I had a look at the first hundred of rows and the probesets were the same BUT they were misaligned around the probeset number 4000 towards). I aligned the rows manually and the mean relative error using all.equal() was 0.001885846. Therefore, APT tools and oligo produce the expression set in different order regarding the probesets. Apologise again for this and thanks again for your kindly help. Kind regards, Javier Benilton Carvalho escribi?: > Are you sure the probesets are in the same order? > > Instead of (A-B)/N, you could use all.equal(A,B), which will also > assess dimnames, especially important in this case (because you'll be > able to notice if the probesets are alligned). > > When I first wrote the code I did this comparison myself and the > relative difference was something like 1e-4. > > So, my guess: probesets are misaligned. > > Best, > b > > On Nov 16, 2009, at 8:00 AM, Javier P?rez Florido wrote: > >> Dear Benilton and Raffaele, >> I've tried what you suggested and I got the following results: >> >> * Comparison between rma and rma-sketch using APT tools: >> o apt-probeset-summarize -a rma -p Hugene- 1_0-st-v1.r3.pgf >> -c Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o >> rma --cel-files cel_list.txt >> o apt-probeset-summarize -a rma-sketch -p >> Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m >> Hugene-1_0-st-v1.r3.mps -o rma-sketch --cel-files >> cel_list.txt >> >> The error given by abs(exprs(rma)-exprs(rma-sketch)) / num_points >> is 1.4147e-004 >> >> * Comparison between rma using APT tools and rma using oligo: >> o apt-probeset-summarize -a rma -p Hugene- 1_0-st-v1.r3.pgf >> -c Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o >> rma --cel-files cel_list.txt >> o OligoEset<-rma(OligoRaw,target="core") >> >> The error given by abs(exprs(rma)-exprs(OligoEset)) / num_points >> is 1.8915 >> >> * Comparison between rma-sketch using APT tools and rma using oligo: >> o apt-probeset-summarize -a rma-sketch -p >> Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m >> Hugene-1_0-st-v1.r3.mps -o rma --cel-files cel_list.txt >> o OligoEset<-rma(OligoRaw,target="core") >> >> The mean error given by abs(exprs(rma-sketch)-exprs(OligoEset)) / >> num_points is 1.8915 >> >> Surprisingly, the difference between APT tools and oligo are quite >> high (you can notice it when having a look at the normalized data). >> Is there anything wrong above? >> Thanks, >> Javier >> >> >> >> Benilton Carvalho escribi?: >>> Thanks for the heads up, Raffaele. >>> >>> My suggestion was Javier to try "-a rma" manually, instead of "-a >>> rma-sketch" (which appears to be what oneChannelGUI uses - at least >>> that's what I saw when skimmed the source ). >>> >>> cheers, >>> >>> b >>> >>> On Nov 12, 2009, at 6:32 AM, rcaloger wrote: >>> >>>> Hi, >>>> dear Benilton, >>>> you are right oneChannelGUI uses sketch-quantile. APT-tools are >>>> used by oneChannelGUI to calculate intensities. >>>> Actually oneChannelGUI uses a graphical interface to execute >>>> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m >>>> MPSFILE.mps -out rmasketch *.cel >>>> cheers >>>> Raffaele >>>> >>>> >>>>> Javier, >>>> >>>>> my knowledge on the oneChannelGUI is pretty limited, but it seems to >>>>> me that it does either rma-sketch or iter-plier. >>>> >>>>> oligo will do the "regular" rma, ie. no sketch normalization. Now, if >>>>> you could download APT and run it yourself (I'm not sure how it is >>>>> packaged in oneChannel), you could try the following: >>>> >>>>> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf -m >>>> MPSFILE.mps -out rmasketch *.cel >>>> >>>>> And you may get more similar results... I'm not saying they'll be >>>>> identical, but when I implemented this for oligo the mean relative >>>>> difference between oligo and APT was something like 0.001. >>>> >>>> b >>>> >>>> On Nov 10, 2009, at 3:30 PM, Javier P?rez Florido wrote: >>>> >>>> >>>>>> Dear all, >>>>>> I have normalized a GeneChip Human Gene ST 1.0 dataset using oligo >>>>>> package and oneChannelGUI. I've checked that the log2 normalized >>>>>> values >>>>>> are different (not so different, but different). When applying limma >>>>>> on >>>>>> them, the statistic values (p-value, M, B and statistic t) are also >>>>>> different. >>>>>> >>>>>> I've read that oneChannelGUI uses APT tools to summarize data and, >>>>>> maybe, that is the point: they produce similar but different >>>>>> normalized >>>>>> values that have an effect in the final list of differentially >>>>>> expressed >>>>>> genes. >>>>>> >>>>>> For oligo, I've normalized using rma method and core as a target: >>>>>> OligoEset<-rma(OligoRaw,target="core") >>>>>> For oneChannelGUI, I've used the option "Load gene 1.0 ST arrays >>>>>> from >>>>>> .CEL files." >>>>>> >>>>>> In both cases, the limma parameters are the same. >>>>>> So, I suspect the APT tools used by oneChannelGUI has influence >>>>>> on the >>>>>> data. Is there a way to normalize the raw data in OneChannelGUI to >>>>>> select the subgroup (core) instead of using APT tools? I think >>>>>> this is >>>>>> only available in Exon Arrays. >>>>>> >>>>>> Or may be I am wrong with these conclusions. >>>>>> Any tips? >>>>>> Thanks, >>>>>> Javier >>>>>> >>>>> >>>> -- >>>> >>>> ---------------------------------------- >>>> 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
A pairwise plot reveals difference too: x <- exprs(OligoEset); y <- exprs(rma-sketch); x <- as.vector(x); y <- as.vector(y); plot(x,y, pch='."); abline(a=0, b=1); /Henrik 2009/11/16 Javier P?rez Florido <jpflorido at="" gmail.com="">: > Dear Benilton and Raffaele, > I've tried what you suggested and I got the following results: > > ? ?* Comparison between rma and rma-sketch using APT tools: > ? ? ? ? ?o apt-probeset-summarize -a rma -p Hugene-1_0-st-v1.r3.pgf -c > ? ? ? ? ? ?Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma > ? ? ? ? ? ?--cel-files cel_list.txt > ? ? ? ? ?o apt-probeset-summarize -a rma-sketch -p > ? ? ? ? ? ?Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m > ? ? ? ? ? ?Hugene-1_0-st-v1.r3.mps -o rma-sketch --cel-files cel_list.txt > > ? ?The error given by abs(exprs(rma)-exprs(rma-sketch)) / num_points is > ? ?1.4147e-004 > > ? ?* Comparison between rma using APT tools and rma using oligo: > ? ? ? ? ?o apt-probeset-summarize -a rma -p Hugene-1_0-st-v1.r3.pgf -c > ? ? ? ? ? ?Hugene-1_0-st-v1.r3.clf -m Hugene-1_0-st-v1.r3.mps -o rma > ? ? ? ? ? ?--cel-files cel_list.txt > ? ? ? ? ?o OligoEset<-rma(OligoRaw,target="core") > > ? ?The error given by abs(exprs(rma)-exprs(OligoEset)) / num_points is > ? ?1.8915 > > ? ?* Comparison between rma-sketch using APT tools and rma using oligo: > ? ? ? ? ?o apt-probeset-summarize -a rma-sketch -p > ? ? ? ? ? ?Hugene-1_0-st-v1.r3.pgf -c Hugene-1_0-st-v1.r3.clf -m > ? ? ? ? ? ?Hugene-1_0-st-v1.r3.mps -o rma --cel-files cel_list.txt > ? ? ? ? ?o OligoEset<-rma(OligoRaw,target="core") > > ? ?The mean error given by abs(exprs(rma-sketch)-exprs(OligoEset)) / > ? ?num_points is 1.8915 > > Surprisingly, the difference between APT tools and oligo are quite high > (you can notice it when having a look at the normalized data). > Is there anything wrong above? > Thanks, > Javier > > > > Benilton Carvalho escribi?: >> Thanks for the heads up, Raffaele. >> >> My suggestion was Javier to try "-a rma" manually, instead of "-a >> rma-sketch" (which appears to be what oneChannelGUI uses - at least >> that's what I saw when skimmed the source ). >> >> cheers, >> >> b >> >> On Nov 12, 2009, at 6:32 AM, rcaloger wrote: >> >>> Hi, >>> dear Benilton, >>> you are right oneChannelGUI uses sketch-quantile. APT-tools are used >>> by oneChannelGUI to calculate intensities. >>> Actually oneChannelGUI uses a graphical interface to execute >>> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf ?-m >>> MPSFILE.mps -out rmasketch *.cel >>> cheers >>> Raffaele >>> >>> >>>> Javier, >>> >>>> my knowledge on the oneChannelGUI is pretty limited, but it seems to >>>> me that it does either rma-sketch or iter-plier. >>> >>>> oligo will do the "regular" rma, ie. no sketch normalization. Now, if >>>> you could download APT and run it yourself (I'm not sure how it is >>>> packaged in oneChannel), you could try the following: >>> >>>> apt-probeset-summarize -a rma -p PGFFILE.pgf -c CLFFILE.clf ?-m >>> MPSFILE.mps -out rmasketch *.cel >>> >>>> And you may get more similar results... I'm not saying they'll be >>>> identical, but when I implemented this for oligo the mean relative >>>> difference between oligo and APT was something like 0.001. >>> >>> b >>> >>> On Nov 10, 2009, at 3:30 PM, Javier P?rez Florido wrote: >>> >>> >>>>> Dear all, >>>>> I have normalized a GeneChip Human Gene ST 1.0 dataset using oligo >>>>> package and oneChannelGUI. I've checked that the log2 normalized >>>>> values >>>>> are different (not so different, but different). When applying limma >>>>> on >>>>> them, the statistic values (p-value, M, B and statistic t) are also >>>>> different. >>>>> >>>>> I've read that oneChannelGUI uses APT tools to summarize data and, >>>>> maybe, that is the point: they produce similar but different >>>>> normalized >>>>> values that have an effect in the final list of differentially >>>>> expressed >>>>> genes. >>>>> >>>>> For oligo, I've normalized using rma method and core as a target: >>>>> OligoEset<-rma(OligoRaw,target="core") >>>>> For oneChannelGUI, I've used the option "Load gene 1.0 ST arrays from >>>>> .CEL files." >>>>> >>>>> In both cases, the limma parameters are the same. >>>>> So, I suspect the APT tools used by oneChannelGUI has influence on the >>>>> data. Is there a way to normalize the raw data in OneChannelGUI to >>>>> select the subgroup (core) instead of using APT tools? I think this is >>>>> only available in Exon Arrays. >>>>> >>>>> Or may be I am wrong with these conclusions. >>>>> Any tips? >>>>> Thanks, >>>>> Javier >>>>> >>>> >>> -- >>> >>> ---------------------------------------- >>> 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 >>> >> >> > > > ? ? ? ?[[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 >
ADD REPLY

Login before adding your answer.

Traffic: 526 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