RNA degradation (Chris Paulse)
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@vawter-marquis-23
Last seen 10.3 years ago
Hi Chris, we have seen the same phenomenon with affyRNA degradation plots. There is definitely a smooth trend, until the last point. It is very reproducible, in fact this position should show the highest intensity overall, but shows about 50% of what would be expected. Best, Mark -----Original Message----- From: bioconductor-request@stat.math.ethz.ch [mailto:bioconductor-request@stat.math.ethz.ch] Sent: Sunday, August 03, 2003 4:36 PM To: bioconductor@stat.math.ethz.ch Subject: Bioconductor Digest, Vol 6, Issue 1 Send Bioconductor mailing list submissions to bioconductor@stat.math.ethz.ch To subscribe or unsubscribe via the World Wide Web, visit https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor or, via email, send a message with subject or body 'help' to bioconductor-request@stat.math.ethz.ch You can reach the person managing the list at bioconductor-owner@stat.math.ethz.ch When replying, please edit your Subject line so it is more specific than "Re: Contents of Bioconductor digest..." Today's Topics: 1. marrayNorm - Getting Data Out (michael watson (IAH-C)) 2. RNA degradation (Chris Paulse) 3. Repost: marrayNorm 1.1.3 gets stuck (Rob Dunne) 4. Re: Spelling mistakes and some questions re limma (Gordon Smyth) 5. Re: RMA t-test (Rafael A. Irizarry) 6. Re: Repost: marrayNorm 1.1.3 gets stuck (Gordon Smyth) ---------------------------------------------------------------------- Message: 1 Date: Thu, 31 Jul 2003 11:16:02 +0100 From: "michael watson (IAH-C)" <michael.watson@bbsrc.ac.uk> Subject: [BioC] marrayNorm - Getting Data Out To: Bioconductor mailing list <bioconductor@stat.math.ethz.ch> Message-ID: <20B7EB075F2D4542AFFAF813E98ACD9301C0099D@cl-exsrv1.irad.bbsrc.ac.uk> Content-Type: text/plain; charset="iso-8859-1" Hi This sounds kind of stupid, but if I have my data in an marrayNorm object, can anyone give any pointers on how to get it out into, say, a tab- delimited text file? Are there any special functions or is it simply write.table() ..?? Thanks Mick ------------------------------ Message: 2 Date: Thu, 31 Jul 2003 15:18:25 -0700 From: "Chris Paulse" <chrispaulse@hotmail.com> Subject: [BioC] RNA degradation To: bioconductor@stat.math.ethz.ch Message-ID: <bay8-f114y0om3g80ce00005707@hotmail.com> Content-Type: text/plain; format=flowed Hi, How much faith should I place in the p-values reported by summaryAffyRNAdeg? The plots of average probe intensity vs probe number (5'<-->3') for some chips I have show a definite positive trend, but usually the last one or two data points drive the curve negative. Does this correspond to any known phenomenon? Thanks, Chris Paulse ------------------------------ Message: 3 Date: Fri, 1 Aug 2003 08:24:07 +1000 (EST) From: Rob Dunne <rob.dunne@csiro.au> Subject: [BioC] Repost: marrayNorm 1.1.3 gets stuck To: bioconductor@stat.math.ethz.ch Message-ID: <16169.38663.319920.3044@pride.nsw.cmis.CSIRO.AU> Content-Type: text/plain; charset=us-ascii Hi List, Please excuse the repost. No one responded to my previous post -- and it seems to me to be quite important. The problem is the new marrayNorm 1.1.3 (installed with bioconductor 1.2) -- which seems to get stuck in an endless loop marrayNorm 1.1.3 (installed with bioconductor 1.2) > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) Timing stopped at: 8874.73 19.65 10289.06 0 0 ie I interrupted the process - but with marrayNorm 1.1.1 reinstalled marrayNorm 1.1.1 > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) [1] 803.99 29.73 843.40 0.00 0.00 is there a known problem with this package? bye rob -- Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 CSIRO Mathematical and Information Sciences +61 2 9325 3100 Locked Bag 17, North Ryde, New South Wales, Australia, 1670 http://matilda.vu.edu.au/~dunne Email: Rob.Dunne@csiro.au Java has certainly revolutionized marketing and litigation. ------------------------------ Message: 4 Date: Fri, 01 Aug 2003 12:09:54 +1000 From: Gordon Smyth <smyth@wehi.edu.au> Subject: [BioC] Re: Spelling mistakes and some questions re limma To: "Dave Waddell" <dwaddell@nutecsciences.com> Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> Message-ID: <5.2.0.9.1.20030801111855.00aed328@imaphost.wehi.edu.au> Content-Type: text/plain; charset="us-ascii"; format=flowed Dear Dave, At 10:45 PM 31/07/2003, Dave Waddell wrote: >You have a couple of spelling mistakes in the page: > ><http: bioinf.wehi.edu.au="" limma="" library="" limma="" html="" 5linearmodels.htm="" l="">http ://bioinf.wehi.edu.au/limma/library/limma/html/5linearmodels.html > >estime and explanded Thanks for letting me know. These typos have been corrected in later versions of limma. >Can you point me to a place that would more fully explain the design >matrix and contrasts with respect to 2-colour dye experiments? My best suggestion at this time is: Yang, Y. H., and Speed, T. P. (2003). Design and analysis of comparative microarray experiments. In T. P. Speed (ed.), Statistical Analysis of Gene Expression Microarray Data. Chapman & Hall/CRC Press, pages 35-91. But basically limma is breaking new ground here so there are no good references for this stuff apart from the User's Guide itself. I am working on providing more user friendly interfaces to create design and contrast matrices and more documentation, but obviously these things take time. In the meantime, a local statistician would be able to give you some help. Or you could ask for help on bioconductor about specific designs. > In some Bioconductor packages, the design matrix appears to be > applicable to the Cy3/Cy5 experiment as a whole and in others to the > individual Cy3 and Cy5 experiments. I am not clear what you mean here. As far as I know, limma is the only package to have the concept of a design matrix and limma is designed to analyze the whole experiment at once. Other packages basically assume you are making only one comparison usually with replicate arrays. > It is very confusing. In addition, the meaning of a contrasts matrix and > how to put one together is not very clear. Both of these values, if > applied incorrectly, would appear to me (as a non-statistician assigned > to put together a package) to completely change the results. Yes, this is true. > Finally, can you tell me how limma handles control spots? The only explicit handling of control spots in limma is in the plotMA function. I assume that you will leave the control spots in during the normalization (perhaps using weights to downweight ratio controls spots or to upweight MSP titration spots) and you will remove them before doing inference about differential expression. There are subsetting commands to make removing control spots easy. >Thanks for a great package, Dave. Thanks for your comments. Gordon ------------------------------ Message: 5 Date: Thu, 31 Jul 2003 22:31:13 -0400 (EDT) From: "Rafael A. Irizarry" <ririzarr@jhsph.edu> Subject: Re: [BioC] RMA t-test To: James MacDonald <jmacdon@med.umich.edu> Cc: bioconductor@stat.math.ethz.ch, dgrigor1@jhmi.edu Message-ID: <pine.gso.4.10.10307312222420.8322-100000@athena.biostat.jhsph.edu> Content-Type: TEXT/PLAIN; charset=US-ASCII hi! fyi, all the ROC curves in the NAR paper comparing expression measures was done on 1-1 comps (i.e. 2 chips). rma seems to perform weel according to these curves. notice that if you only have one chip median polish turns into a median which in my opinion is not a terrible thing to use. as for t-tests with two arrays all you could use for estimating variability (denominator in the t-test) are the residuals from the median polish fit. these have (at least) two problemsB 1) as james points out they have no information about biological variation 2) its not clear what the statistical properites of these residuals are. the se estimate one gets with expresso-rma are given only as an ad-hoc estimate of uncertainty of the expression estimates due to technology. hope this helps, rafael On Mon, 28 Jul 2003, James MacDonald wrote: > I would be cautious about using RMA with only two chips. You will be > estimating the probe-specific intensity with only two observations, so > it is doubtful that the estimate will be very accurate. I recall reading > somewhere that a good minimum number of chips is around 5-6 for RMA. > > As for a t-test with only one observation per group, this is not > possible. How are you going to estimate the variance for each group? > Without replication all you can do is ratios, and you are then stuck > with the assumption that large ratios equal significant differences. > > Jim > > > > > James W. MacDonald > Affymetrix and cDNA Microarray Core > University of Michigan Cancer Center > 1500 E. Medical Center Drive > 7410 CCGC > Ann Arbor MI 48109 > 734-647-5623 > > >>> DMITRY GRIGORYEV <dgrigor1@jhmi.edu> 07/28/03 12:08PM >>> > Hi everyone. > > One quick question. > When I run RMA on just two chips, how could I conduct pairwise t-test > for each probe set between these chips? > > Thank you > > Dima > > _______________________________________________ > Bioconductor mailing list > Bioconductor@stat.math.ethz.ch > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > _______________________________________________ > Bioconductor mailing list > Bioconductor@stat.math.ethz.ch > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > ------------------------------ Message: 6 Date: Fri, 01 Aug 2003 15:30:19 +1000 From: Gordon Smyth <smyth@wehi.edu.au> Subject: Re: [BioC] Repost: marrayNorm 1.1.3 gets stuck To: Rob.Dunne@csiro.au Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> Message-ID: <5.2.1.1.1.20030801151709.00b1ee48@imaphost.wehi.edu.au> Content-Type: text/plain; charset="us-ascii"; format=flowed >Hi List, > >Please excuse the repost. No one responded to my >previous post -- and it seems to me to be quite >important. > >The problem is the new marrayNorm 1.1.3 >(installed with bioconductor 1.2) -- which seems to get >stuck in an endless loop It isn't in an endless loop, it's just very slow. The problem is the loess function. If you use family="symmetric" and iterations=4 to get a robust loess curve rather than just least squares, then the function is quite slow with lots of data and you get heaps of warnings associated with memory limits and the use of a k-d tree. If you use surface="direct" to avoid the k-d tree and stop the warnings, then the function is very slow indeed with lots of points. You see the result below when you try to run it on 30,000 data points. Versions of marrayNorm prior to 1.1.3 used least squares for the loess curves - much quicker but not ideal as a normalization tool. I have used some tricks to avoid this sort of speed degradation in the limma package. I believe that Jean is in the process of implementing to same sort of thing in the marrayNorm package. Regards Gordon >marrayNorm 1.1.3 (installed with bioconductor 1.2) > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) >Timing stopped at: 8874.73 19.65 10289.06 0 0 > >ie I interrupted the process - >but with marrayNorm 1.1.1 reinstalled > > marrayNorm 1.1.1 > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) >[1] 803.99 29.73 843.40 0.00 0.00 > > > >is there a known problem with this package? > > bye > rob > >-- >Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 >CSIRO Mathematical and Information Sciences +61 2 9325 3100 >Locked Bag 17, North Ryde, New South Wales, Australia, 1670 ><http: matilda.vu.edu.au="" ~dunne="">http://matilda.vu.edu.au/~dunne Email: ><https: www.stat.math.ethz.ch="" mailman="" listinfo="" bioconductor="">Rob.Dunn e at >csiro.au ------------------------------ _______________________________________________ Bioconductor mailing list Bioconductor@stat.math.ethz.ch https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor End of Bioconductor Digest, Vol 6, Issue 1
Microarray Normalization Cancer probe ROC limma PROcess Microarray Normalization Cancer • 1.6k views
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Chris Paulse ▴ 90
@chris-paulse-155
Last seen 10.3 years ago
Thanks. We see this behaviour in almost every array (RGU34a layout). The test slides do not show any noticable signs of degradation (test3 layout). I notice in a set of slides for the recent Milan short course that RNA degradation is discussed as an effect that could be detected and corrected for once the G-C sequence effect is corrected for. Can anyone (Rafael?) provide some indication of progress with this? Does the additive model in RMA do anything to reduce the variance caused by RNA degradation? Thanks, Chris >From: "Vawter, Marquis" <mvawter@uci.edu> >To: "'bioconductor@stat.math.ethz.ch'" <bioconductor@stat.math.ethz.ch> >Subject: [BioC] RNA degradation (Chris Paulse) >Date: Mon, 4 Aug 2003 10:03:15 -0700 > >Hi Chris, we have seen the same phenomenon with affyRNA degradation plots. >There is definitely a smooth trend, until the last point. It is very >reproducible, in fact this position should show the highest intensity >overall, but shows about 50% of what would be expected. >Best, Mark > > >-----Original Message----- >From: bioconductor-request@stat.math.ethz.ch >[mailto:bioconductor-request@stat.math.ethz.ch] >Sent: Sunday, August 03, 2003 4:36 PM >To: bioconductor@stat.math.ethz.ch >Subject: Bioconductor Digest, Vol 6, Issue 1 > > >Send Bioconductor mailing list submissions to > bioconductor@stat.math.ethz.ch > >To subscribe or unsubscribe via the World Wide Web, visit > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor >or, via email, send a message with subject or body 'help' to > bioconductor-request@stat.math.ethz.ch > >You can reach the person managing the list at > bioconductor-owner@stat.math.ethz.ch > >When replying, please edit your Subject line so it is more specific >than "Re: Contents of Bioconductor digest..." > > >Today's Topics: > > 1. marrayNorm - Getting Data Out (michael watson (IAH-C)) > 2. RNA degradation (Chris Paulse) > 3. Repost: marrayNorm 1.1.3 gets stuck (Rob Dunne) > 4. Re: Spelling mistakes and some questions re limma (Gordon Smyth) > 5. Re: RMA t-test (Rafael A. Irizarry) > 6. Re: Repost: marrayNorm 1.1.3 gets stuck (Gordon Smyth) > > >--------------------------------------------------------------------- - > >Message: 1 >Date: Thu, 31 Jul 2003 11:16:02 +0100 >From: "michael watson (IAH-C)" <michael.watson@bbsrc.ac.uk> >Subject: [BioC] marrayNorm - Getting Data Out >To: Bioconductor mailing list <bioconductor@stat.math.ethz.ch> >Message-ID: > ><20B7EB075F2D4542AFFAF813E98ACD9301C0099D@cl-exsrv1.irad.bbsrc.ac.uk> >Content-Type: text/plain; charset="iso-8859-1" > >Hi > >This sounds kind of stupid, but if I have my data in an marrayNorm object, >can anyone give any pointers on how to get it out into, say, a >tab-delimited >text file? > >Are there any special functions or is it simply write.table() ..?? > >Thanks >Mick > > >------------------------------ > >Message: 2 >Date: Thu, 31 Jul 2003 15:18:25 -0700 >From: "Chris Paulse" <chrispaulse@hotmail.com> >Subject: [BioC] RNA degradation >To: bioconductor@stat.math.ethz.ch >Message-ID: <bay8-f114y0om3g80ce00005707@hotmail.com> >Content-Type: text/plain; format=flowed > >Hi, >How much faith should I place in the p-values reported by >summaryAffyRNAdeg? > > The plots of average probe intensity vs probe number (5'<-->3') for some >chips I have show a definite positive trend, but usually the last one or >two > >data points drive the curve negative. Does this correspond to any known >phenomenon? > >Thanks, >Chris Paulse > > >------------------------------ > >Message: 3 >Date: Fri, 1 Aug 2003 08:24:07 +1000 (EST) >From: Rob Dunne <rob.dunne@csiro.au> >Subject: [BioC] Repost: marrayNorm 1.1.3 gets stuck >To: bioconductor@stat.math.ethz.ch >Message-ID: <16169.38663.319920.3044@pride.nsw.cmis.CSIRO.AU> >Content-Type: text/plain; charset=us-ascii > >Hi List, > >Please excuse the repost. No one responded to my >previous post -- and it seems to me to be quite >important. > >The problem is the new marrayNorm 1.1.3 >(installed with bioconductor 1.2) -- which seems to get >stuck in an endless loop > > >marrayNorm 1.1.3 (installed with bioconductor 1.2) > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) >Timing stopped at: 8874.73 19.65 10289.06 0 0 > >ie I interrupted the process - >but with marrayNorm 1.1.1 reinstalled > > marrayNorm 1.1.1 > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) >[1] 803.99 29.73 843.40 0.00 0.00 > > > >is there a known problem with this package? > > bye > rob > >-- >Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 >CSIRO Mathematical and Information Sciences +61 2 9325 3100 >Locked Bag 17, North Ryde, New South Wales, Australia, 1670 >http://matilda.vu.edu.au/~dunne Email: Rob.Dunne@csiro.au > > Java has certainly revolutionized marketing and litigation. > > >------------------------------ > >Message: 4 >Date: Fri, 01 Aug 2003 12:09:54 +1000 >From: Gordon Smyth <smyth@wehi.edu.au> >Subject: [BioC] Re: Spelling mistakes and some questions re limma >To: "Dave Waddell" <dwaddell@nutecsciences.com> >Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> >Message-ID: <5.2.0.9.1.20030801111855.00aed328@imaphost.wehi.edu.au> >Content-Type: text/plain; charset="us-ascii"; format=flowed > >Dear Dave, > >At 10:45 PM 31/07/2003, Dave Waddell wrote: > >You have a couple of spelling mistakes in the page: > > > ><http: bioinf.wehi.edu.au="" limma="" library="" limma="" html="" 5linearmodels.h="" tml="">http >://bioinf.wehi.edu.au/limma/library/limma/html/5linearmodels.html > > > >estime and explanded > >Thanks for letting me know. These typos have been corrected in later >versions of limma. > > >Can you point me to a place that would more fully explain the design > >matrix and contrasts with respect to 2-colour dye experiments? > >My best suggestion at this time is: > >Yang, Y. H., and Speed, T. P. (2003). Design and analysis of comparative >microarray experiments. In T. P. Speed (ed.), Statistical Analysis of Gene >Expression Microarray Data. Chapman & Hall/CRC Press, pages 35-91. > >But basically limma is breaking new ground here so there are no good >references for this stuff apart from the User's Guide itself. I am working >on providing more user friendly interfaces to create design and contrast >matrices and more documentation, but obviously these things take time. In >the meantime, a local statistician would be able to give you some help. Or >you could ask for help on bioconductor about specific designs. > > > In some Bioconductor packages, the design matrix appears to be > > applicable to the Cy3/Cy5 experiment as a whole and in others to the > > individual Cy3 and Cy5 experiments. > >I am not clear what you mean here. As far as I know, limma is the only >package to have the concept of a design matrix and limma is designed to >analyze the whole experiment at once. Other packages basically assume you >are making only one comparison usually with replicate arrays. > > > It is very confusing. In addition, the meaning of a contrasts matrix >and > > how to put one together is not very clear. Both of these values, if > > applied incorrectly, would appear to me (as a non-statistician assigned > > to put together a package) to completely change the results. > >Yes, this is true. > > > Finally, can you tell me how limma handles control spots? > >The only explicit handling of control spots in limma is in the plotMA >function. I assume that you will leave the control spots in during the >normalization (perhaps using weights to downweight ratio controls spots or >to upweight MSP titration spots) and you will remove them before doing >inference about differential expression. There are subsetting commands to >make removing control spots easy. > > >Thanks for a great package, Dave. > >Thanks for your comments. > >Gordon > > >------------------------------ > >Message: 5 >Date: Thu, 31 Jul 2003 22:31:13 -0400 (EDT) >From: "Rafael A. Irizarry" <ririzarr@jhsph.edu> >Subject: Re: [BioC] RMA t-test >To: James MacDonald <jmacdon@med.umich.edu> >Cc: bioconductor@stat.math.ethz.ch, dgrigor1@jhmi.edu >Message-ID: > <pine.gso.4.10.10307312222420.8322-100000@athena.biostat.jhsph.edu> >Content-Type: TEXT/PLAIN; charset=US-ASCII > >hi! fyi, all the ROC curves in the NAR paper comparing expression measures >was done on 1-1 comps (i.e. 2 chips). rma seems to perform weel >according to these curves. notice that if you only have one >chip median polish turns into a median which in my opinion is not a >terrible thing to use. > >as for t-tests with two arrays all you could use for estimating >variability (denominator in the t-test) are the residuals from the median >polish fit. these have (at least) two problemsB >1) as james points out they have no information about biological >variation >2) its not clear what the statistical properites of these residuals are. >the se estimate one gets with expresso-rma are given only as an ad- hoc >estimate of uncertainty of the expression estimates due to technology. > >hope this helps, >rafael >On Mon, 28 Jul 2003, James MacDonald wrote: > > > I would be cautious about using RMA with only two chips. You will be > > estimating the probe-specific intensity with only two observations, so > > it is doubtful that the estimate will be very accurate. I recall reading > > somewhere that a good minimum number of chips is around 5-6 for RMA. > > > > As for a t-test with only one observation per group, this is not > > possible. How are you going to estimate the variance for each group? > > Without replication all you can do is ratios, and you are then stuck > > with the assumption that large ratios equal significant differences. > > > > Jim > > > > > > > > > > James W. MacDonald > > Affymetrix and cDNA Microarray Core > > University of Michigan Cancer Center > > 1500 E. Medical Center Drive > > 7410 CCGC > > Ann Arbor MI 48109 > > 734-647-5623 > > > > >>> DMITRY GRIGORYEV <dgrigor1@jhmi.edu> 07/28/03 12:08PM >>> > > Hi everyone. > > > > One quick question. > > When I run RMA on just two chips, how could I conduct pairwise t-test > > for each probe set between these chips? > > > > Thank you > > > > Dima > > > > _______________________________________________ > > Bioconductor mailing list > > Bioconductor@stat.math.ethz.ch > > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > > > _______________________________________________ > > Bioconductor mailing list > > Bioconductor@stat.math.ethz.ch > > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > > > >------------------------------ > >Message: 6 >Date: Fri, 01 Aug 2003 15:30:19 +1000 >From: Gordon Smyth <smyth@wehi.edu.au> >Subject: Re: [BioC] Repost: marrayNorm 1.1.3 gets stuck >To: Rob.Dunne@csiro.au >Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> >Message-ID: <5.2.1.1.1.20030801151709.00b1ee48@imaphost.wehi.edu.au> >Content-Type: text/plain; charset="us-ascii"; format=flowed > > > >Hi List, > > > >Please excuse the repost. No one responded to my > >previous post -- and it seems to me to be quite > >important. > > > >The problem is the new marrayNorm 1.1.3 > >(installed with bioconductor 1.2) -- which seems to get > >stuck in an endless loop > >It isn't in an endless loop, it's just very slow. > >The problem is the loess function. If you use family="symmetric" and >iterations=4 to get a robust loess curve rather than just least squares, >then the function is quite slow with lots of data and you get heaps of >warnings associated with memory limits and the use of a k-d tree. If you >use surface="direct" to avoid the k-d tree and stop the warnings, then the >function is very slow indeed with lots of points. You see the result below >when you try to run it on 30,000 data points. > >Versions of marrayNorm prior to 1.1.3 used least squares for the loess >curves - much quicker but not ideal as a normalization tool. > >I have used some tricks to avoid this sort of speed degradation in the >limma package. I believe that Jean is in the process of implementing to >same sort of thing in the marrayNorm package. > >Regards >Gordon > > >marrayNorm 1.1.3 (installed with bioconductor 1.2) > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > >Timing stopped at: 8874.73 19.65 10289.06 0 0 > > > >ie I interrupted the process - > >but with marrayNorm 1.1.1 reinstalled > > > > marrayNorm 1.1.1 > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > >[1] 803.99 29.73 843.40 0.00 0.00 > > > > > > > >is there a known problem with this package? > > > > bye > > rob > > > >-- > >Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 > >CSIRO Mathematical and Information Sciences +61 2 9325 3100 > >Locked Bag 17, North Ryde, New South Wales, Australia, 1670 > ><http: matilda.vu.edu.au="" ~dunne="">http://matilda.vu.edu.au/~dunne Email: > ><https: www.stat.math.ethz.ch="" mailman="" listinfo="" bioconductor="">Rob.Du nne at > >csiro.au > > >------------------------------ > >_______________________________________________ >Bioconductor mailing list >Bioconductor@stat.math.ethz.ch >https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > >End of Bioconductor Digest, Vol 6, Issue 1 > >_______________________________________________ >Bioconductor mailing list >Bioconductor@stat.math.ethz.ch >https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor
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i have to take a second look athos milan slides but its possible you misinterpreted them. we dont expect gc content and location to be confounded so i dont see how correcting for gc-content could help here. the robust fitting of the linear model may help, as probes with more variance usually result in more "outliers" and thus are counted less. On Mon, 4 Aug 2003, Chris Paulse wrote: > Thanks. We see this behaviour in almost every array (RGU34a layout). The > test slides do not show any noticable signs of degradation (test3 layout). > I notice in a set of slides for the recent Milan short course that RNA > degradation is discussed as an effect that could be detected and corrected > for once the G-C sequence effect is corrected for. Can anyone (Rafael?) > provide some indication of progress with this? Does the additive model in > RMA do anything to reduce the variance caused by RNA degradation? > > Thanks, > Chris > > > >From: "Vawter, Marquis" <mvawter@uci.edu> > >To: "'bioconductor@stat.math.ethz.ch'" <bioconductor@stat.math.ethz.ch> > >Subject: [BioC] RNA degradation (Chris Paulse) > >Date: Mon, 4 Aug 2003 10:03:15 -0700 > > > >Hi Chris, we have seen the same phenomenon with affyRNA degradation plots. > >There is definitely a smooth trend, until the last point. It is very > >reproducible, in fact this position should show the highest intensity > >overall, but shows about 50% of what would be expected. > >Best, Mark > > > > > >-----Original Message----- > >From: bioconductor-request@stat.math.ethz.ch > >[mailto:bioconductor-request@stat.math.ethz.ch] > >Sent: Sunday, August 03, 2003 4:36 PM > >To: bioconductor@stat.math.ethz.ch > >Subject: Bioconductor Digest, Vol 6, Issue 1 > > > > > >Send Bioconductor mailing list submissions to > > bioconductor@stat.math.ethz.ch > > > >To subscribe or unsubscribe via the World Wide Web, visit > > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > >or, via email, send a message with subject or body 'help' to > > bioconductor-request@stat.math.ethz.ch > > > >You can reach the person managing the list at > > bioconductor-owner@stat.math.ethz.ch > > > >When replying, please edit your Subject line so it is more specific > >than "Re: Contents of Bioconductor digest..." > > > > > >Today's Topics: > > > > 1. marrayNorm - Getting Data Out (michael watson (IAH-C)) > > 2. RNA degradation (Chris Paulse) > > 3. Repost: marrayNorm 1.1.3 gets stuck (Rob Dunne) > > 4. Re: Spelling mistakes and some questions re limma (Gordon Smyth) > > 5. Re: RMA t-test (Rafael A. Irizarry) > > 6. Re: Repost: marrayNorm 1.1.3 gets stuck (Gordon Smyth) > > > > > >------------------------------------------------------------------- --- > > > >Message: 1 > >Date: Thu, 31 Jul 2003 11:16:02 +0100 > >From: "michael watson (IAH-C)" <michael.watson@bbsrc.ac.uk> > >Subject: [BioC] marrayNorm - Getting Data Out > >To: Bioconductor mailing list <bioconductor@stat.math.ethz.ch> > >Message-ID: > > > ><20B7EB075F2D4542AFFAF813E98ACD9301C0099D@cl- exsrv1.irad.bbsrc.ac.uk> > >Content-Type: text/plain; charset="iso-8859-1" > > > >Hi > > > >This sounds kind of stupid, but if I have my data in an marrayNorm object, > >can anyone give any pointers on how to get it out into, say, a > >tab-delimited > >text file? > > > >Are there any special functions or is it simply write.table() ..?? > > > >Thanks > >Mick > > > > > >------------------------------ > > > >Message: 2 > >Date: Thu, 31 Jul 2003 15:18:25 -0700 > >From: "Chris Paulse" <chrispaulse@hotmail.com> > >Subject: [BioC] RNA degradation > >To: bioconductor@stat.math.ethz.ch > >Message-ID: <bay8-f114y0om3g80ce00005707@hotmail.com> > >Content-Type: text/plain; format=flowed > > > >Hi, > >How much faith should I place in the p-values reported by > >summaryAffyRNAdeg? > > > > The plots of average probe intensity vs probe number (5'<-->3') for some > >chips I have show a definite positive trend, but usually the last one or > >two > > > >data points drive the curve negative. Does this correspond to any known > >phenomenon? > > > >Thanks, > >Chris Paulse > > > > > >------------------------------ > > > >Message: 3 > >Date: Fri, 1 Aug 2003 08:24:07 +1000 (EST) > >From: Rob Dunne <rob.dunne@csiro.au> > >Subject: [BioC] Repost: marrayNorm 1.1.3 gets stuck > >To: bioconductor@stat.math.ethz.ch > >Message-ID: <16169.38663.319920.3044@pride.nsw.cmis.CSIRO.AU> > >Content-Type: text/plain; charset=us-ascii > > > >Hi List, > > > >Please excuse the repost. No one responded to my > >previous post -- and it seems to me to be quite > >important. > > > >The problem is the new marrayNorm 1.1.3 > >(installed with bioconductor 1.2) -- which seems to get > >stuck in an endless loop > > > > > >marrayNorm 1.1.3 (installed with bioconductor 1.2) > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > >Timing stopped at: 8874.73 19.65 10289.06 0 0 > > > >ie I interrupted the process - > >but with marrayNorm 1.1.1 reinstalled > > > > marrayNorm 1.1.1 > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > >[1] 803.99 29.73 843.40 0.00 0.00 > > > > > > > >is there a known problem with this package? > > > > bye > > rob > > > >-- > >Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 > >CSIRO Mathematical and Information Sciences +61 2 9325 3100 > >Locked Bag 17, North Ryde, New South Wales, Australia, 1670 > >http://matilda.vu.edu.au/~dunne Email: Rob.Dunne@csiro.au > > > > Java has certainly revolutionized marketing and litigation. > > > > > >------------------------------ > > > >Message: 4 > >Date: Fri, 01 Aug 2003 12:09:54 +1000 > >From: Gordon Smyth <smyth@wehi.edu.au> > >Subject: [BioC] Re: Spelling mistakes and some questions re limma > >To: "Dave Waddell" <dwaddell@nutecsciences.com> > >Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> > >Message-ID: <5.2.0.9.1.20030801111855.00aed328@imaphost.wehi.edu.au> > >Content-Type: text/plain; charset="us-ascii"; format=flowed > > > >Dear Dave, > > > >At 10:45 PM 31/07/2003, Dave Waddell wrote: > > >You have a couple of spelling mistakes in the page: > > > > > ><http: bioinf.wehi.edu.au="" limma="" library="" limma="" html="" 5linearmodels="" .html="">http > >://bioinf.wehi.edu.au/limma/library/limma/html/5linearmodels.html > > > > > >estime and explanded > > > >Thanks for letting me know. These typos have been corrected in later > >versions of limma. > > > > >Can you point me to a place that would more fully explain the design > > >matrix and contrasts with respect to 2-colour dye experiments? > > > >My best suggestion at this time is: > > > >Yang, Y. H., and Speed, T. P. (2003). Design and analysis of comparative > >microarray experiments. In T. P. Speed (ed.), Statistical Analysis of Gene > >Expression Microarray Data. Chapman & Hall/CRC Press, pages 35-91. > > > >But basically limma is breaking new ground here so there are no good > >references for this stuff apart from the User's Guide itself. I am working > >on providing more user friendly interfaces to create design and contrast > >matrices and more documentation, but obviously these things take time. In > >the meantime, a local statistician would be able to give you some help. Or > >you could ask for help on bioconductor about specific designs. > > > > > In some Bioconductor packages, the design matrix appears to be > > > applicable to the Cy3/Cy5 experiment as a whole and in others to the > > > individual Cy3 and Cy5 experiments. > > > >I am not clear what you mean here. As far as I know, limma is the only > >package to have the concept of a design matrix and limma is designed to > >analyze the whole experiment at once. Other packages basically assume you > >are making only one comparison usually with replicate arrays. > > > > > It is very confusing. In addition, the meaning of a contrasts matrix > >and > > > how to put one together is not very clear. Both of these values, if > > > applied incorrectly, would appear to me (as a non-statistician assigned > > > to put together a package) to completely change the results. > > > >Yes, this is true. > > > > > Finally, can you tell me how limma handles control spots? > > > >The only explicit handling of control spots in limma is in the plotMA > >function. I assume that you will leave the control spots in during the > >normalization (perhaps using weights to downweight ratio controls spots or > >to upweight MSP titration spots) and you will remove them before doing > >inference about differential expression. There are subsetting commands to > >make removing control spots easy. > > > > >Thanks for a great package, Dave. > > > >Thanks for your comments. > > > >Gordon > > > > > >------------------------------ > > > >Message: 5 > >Date: Thu, 31 Jul 2003 22:31:13 -0400 (EDT) > >From: "Rafael A. Irizarry" <ririzarr@jhsph.edu> > >Subject: Re: [BioC] RMA t-test > >To: James MacDonald <jmacdon@med.umich.edu> > >Cc: bioconductor@stat.math.ethz.ch, dgrigor1@jhmi.edu > >Message-ID: > > <pine.gso.4.10.10307312222420.8322-100000@athena.biostat.jhsph.edu> > >Content-Type: TEXT/PLAIN; charset=US-ASCII > > > >hi! fyi, all the ROC curves in the NAR paper comparing expression measures > >was done on 1-1 comps (i.e. 2 chips). rma seems to perform weel > >according to these curves. notice that if you only have one > >chip median polish turns into a median which in my opinion is not a > >terrible thing to use. > > > >as for t-tests with two arrays all you could use for estimating > >variability (denominator in the t-test) are the residuals from the median > >polish fit. these have (at least) two problemsB > >1) as james points out they have no information about biological > >variation > >2) its not clear what the statistical properites of these residuals are. > >the se estimate one gets with expresso-rma are given only as an ad- hoc > >estimate of uncertainty of the expression estimates due to technology. > > > >hope this helps, > >rafael > >On Mon, 28 Jul 2003, James MacDonald wrote: > > > > > I would be cautious about using RMA with only two chips. You will be > > > estimating the probe-specific intensity with only two observations, so > > > it is doubtful that the estimate will be very accurate. I recall reading > > > somewhere that a good minimum number of chips is around 5-6 for RMA. > > > > > > As for a t-test with only one observation per group, this is not > > > possible. How are you going to estimate the variance for each group? > > > Without replication all you can do is ratios, and you are then stuck > > > with the assumption that large ratios equal significant differences. > > > > > > Jim > > > > > > > > > > > > > > > James W. MacDonald > > > Affymetrix and cDNA Microarray Core > > > University of Michigan Cancer Center > > > 1500 E. Medical Center Drive > > > 7410 CCGC > > > Ann Arbor MI 48109 > > > 734-647-5623 > > > > > > >>> DMITRY GRIGORYEV <dgrigor1@jhmi.edu> 07/28/03 12:08PM >>> > > > Hi everyone. > > > > > > One quick question. > > > When I run RMA on just two chips, how could I conduct pairwise t-test > > > for each probe set between these chips? > > > > > > Thank you > > > > > > Dima > > > > > > _______________________________________________ > > > Bioconductor mailing list > > > Bioconductor@stat.math.ethz.ch > > > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > > > > > _______________________________________________ > > > Bioconductor mailing list > > > Bioconductor@stat.math.ethz.ch > > > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > > > > > > > >------------------------------ > > > >Message: 6 > >Date: Fri, 01 Aug 2003 15:30:19 +1000 > >From: Gordon Smyth <smyth@wehi.edu.au> > >Subject: Re: [BioC] Repost: marrayNorm 1.1.3 gets stuck > >To: Rob.Dunne@csiro.au > >Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> > >Message-ID: <5.2.1.1.1.20030801151709.00b1ee48@imaphost.wehi.edu.au> > >Content-Type: text/plain; charset="us-ascii"; format=flowed > > > > > > >Hi List, > > > > > >Please excuse the repost. No one responded to my > > >previous post -- and it seems to me to be quite > > >important. > > > > > >The problem is the new marrayNorm 1.1.3 > > >(installed with bioconductor 1.2) -- which seems to get > > >stuck in an endless loop > > > >It isn't in an endless loop, it's just very slow. > > > >The problem is the loess function. If you use family="symmetric" and > >iterations=4 to get a robust loess curve rather than just least squares, > >then the function is quite slow with lots of data and you get heaps of > >warnings associated with memory limits and the use of a k-d tree. If you > >use surface="direct" to avoid the k-d tree and stop the warnings, then the > >function is very slow indeed with lots of points. You see the result below > >when you try to run it on 30,000 data points. > > > >Versions of marrayNorm prior to 1.1.3 used least squares for the loess > >curves - much quicker but not ideal as a normalization tool. > > > >I have used some tricks to avoid this sort of speed degradation in the > >limma package. I believe that Jean is in the process of implementing to > >same sort of thing in the marrayNorm package. > > > >Regards > >Gordon > > > > >marrayNorm 1.1.3 (installed with bioconductor 1.2) > > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > > >Timing stopped at: 8874.73 19.65 10289.06 0 0 > > > > > >ie I interrupted the process - > > >but with marrayNorm 1.1.1 reinstalled > > > > > > marrayNorm 1.1.1 > > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > > >[1] 803.99 29.73 843.40 0.00 0.00 > > > > > > > > > > > >is there a known problem with this package? > > > > > > bye > > > rob > > > > > >-- > > >Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 > > >CSIRO Mathematical and Information Sciences +61 2 9325 3100 > > >Locked Bag 17, North Ryde, New South Wales, Australia, 1670 > > ><http: matilda.vu.edu.au="" ~dunne="">http://matilda.vu.edu.au/~dunne Email: > > ><https: www.stat.math.ethz.ch="" mailman="" listinfo="" bioconductor="">Rob. Dunne at > > >csiro.au > > > > > >------------------------------ > > > >_______________________________________________ > >Bioconductor mailing list > >Bioconductor@stat.math.ethz.ch > >https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > > > > >End of Bioconductor Digest, Vol 6, Issue 1 > > > >_______________________________________________ > >Bioconductor mailing list > >Bioconductor@stat.math.ethz.ch > >https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > _______________________________________________ > Bioconductor mailing list > Bioconductor@stat.math.ethz.ch > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor >
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Rafael should correct me on this if I am wrong, but I think the critical thing for a RNA degradation plot is that the slopes for all the chips should be as similar as possible. Not to say that horizontal isn't ideal, but I have never seen any plots that *were* horizontal (correction; the slopes for the affy spike-in data set are pretty close to horizontal, except for the inevitable drop off at the 3' end). Note too that these plots show more than simple degradation. There is also the second strand synthesis that proceeds from 3' to 5'. If this doesn't go to completion, you will also see a slope to the plots. Also, the G-C sequence code has been released in the gcrma library, so you can play around with it to see if it helps with the RNA degradation plots. Jim James W. MacDonald Affymetrix and cDNA Microarray Core University of Michigan Cancer Center 1500 E. Medical Center Drive 7410 CCGC Ann Arbor MI 48109 734-647-5623 >>> "Chris Paulse" <chrispaulse@hotmail.com> 08/04/03 01:55PM >>> Thanks. We see this behaviour in almost every array (RGU34a layout). The test slides do not show any noticable signs of degradation (test3 layout). I notice in a set of slides for the recent Milan short course that RNA degradation is discussed as an effect that could be detected and corrected for once the G-C sequence effect is corrected for. Can anyone (Rafael?) provide some indication of progress with this? Does the additive model in RMA do anything to reduce the variance caused by RNA degradation? Thanks, Chris >From: "Vawter, Marquis" <mvawter@uci.edu> >To: "'bioconductor@stat.math.ethz.ch'" <bioconductor@stat.math.ethz.ch> >Subject: [BioC] RNA degradation (Chris Paulse) >Date: Mon, 4 Aug 2003 10:03:15 -0700 > >Hi Chris, we have seen the same phenomenon with affyRNA degradation plots. >There is definitely a smooth trend, until the last point. It is very >reproducible, in fact this position should show the highest intensity >overall, but shows about 50% of what would be expected. >Best, Mark > > >-----Original Message----- >From: bioconductor-request@stat.math.ethz.ch >[mailto:bioconductor-request@stat.math.ethz.ch] >Sent: Sunday, August 03, 2003 4:36 PM >To: bioconductor@stat.math.ethz.ch >Subject: Bioconductor Digest, Vol 6, Issue 1 > > >Send Bioconductor mailing list submissions to > bioconductor@stat.math.ethz.ch > >To subscribe or unsubscribe via the World Wide Web, visit > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor >or, via email, send a message with subject or body 'help' to > bioconductor-request@stat.math.ethz.ch > >You can reach the person managing the list at > bioconductor-owner@stat.math.ethz.ch > >When replying, please edit your Subject line so it is more specific >than "Re: Contents of Bioconductor digest..." > > >Today's Topics: > > 1. marrayNorm - Getting Data Out (michael watson (IAH-C)) > 2. RNA degradation (Chris Paulse) > 3. Repost: marrayNorm 1.1.3 gets stuck (Rob Dunne) > 4. Re: Spelling mistakes and some questions re limma (Gordon Smyth) > 5. Re: RMA t-test (Rafael A. Irizarry) > 6. Re: Repost: marrayNorm 1.1.3 gets stuck (Gordon Smyth) > > >--------------------------------------------------------------------- - > >Message: 1 >Date: Thu, 31 Jul 2003 11:16:02 +0100 >From: "michael watson (IAH-C)" <michael.watson@bbsrc.ac.uk> >Subject: [BioC] marrayNorm - Getting Data Out >To: Bioconductor mailing list <bioconductor@stat.math.ethz.ch> >Message-ID: > ><20B7EB075F2D4542AFFAF813E98ACD9301C0099D@cl-exsrv1.irad.bbsrc.ac.uk> >Content-Type: text/plain; charset="iso-8859-1" > >Hi > >This sounds kind of stupid, but if I have my data in an marrayNorm object, >can anyone give any pointers on how to get it out into, say, a >tab-delimited >text file? > >Are there any special functions or is it simply write.table() ..?? > >Thanks >Mick > > >------------------------------ > >Message: 2 >Date: Thu, 31 Jul 2003 15:18:25 -0700 >From: "Chris Paulse" <chrispaulse@hotmail.com> >Subject: [BioC] RNA degradation >To: bioconductor@stat.math.ethz.ch >Message-ID: <bay8-f114y0om3g80ce00005707@hotmail.com> >Content-Type: text/plain; format=flowed > >Hi, >How much faith should I place in the p-values reported by >summaryAffyRNAdeg? > > The plots of average probe intensity vs probe number (5'<-->3') for some >chips I have show a definite positive trend, but usually the last one or >two > >data points drive the curve negative. Does this correspond to any known >phenomenon? > >Thanks, >Chris Paulse > > >------------------------------ > >Message: 3 >Date: Fri, 1 Aug 2003 08:24:07 +1000 (EST) >From: Rob Dunne <rob.dunne@csiro.au> >Subject: [BioC] Repost: marrayNorm 1.1.3 gets stuck >To: bioconductor@stat.math.ethz.ch >Message-ID: <16169.38663.319920.3044@pride.nsw.cmis.CSIRO.AU> >Content-Type: text/plain; charset=us-ascii > >Hi List, > >Please excuse the repost. No one responded to my >previous post -- and it seems to me to be quite >important. > >The problem is the new marrayNorm 1.1.3 >(installed with bioconductor 1.2) -- which seems to get >stuck in an endless loop > > >marrayNorm 1.1.3 (installed with bioconductor 1.2) > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) >Timing stopped at: 8874.73 19.65 10289.06 0 0 > >ie I interrupted the process - >but with marrayNorm 1.1.1 reinstalled > > marrayNorm 1.1.1 > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) >[1] 803.99 29.73 843.40 0.00 0.00 > > > >is there a known problem with this package? > > bye > rob > >-- >Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 >CSIRO Mathematical and Information Sciences +61 2 9325 3100 >Locked Bag 17, North Ryde, New South Wales, Australia, 1670 >http://matilda.vu.edu.au/~dunne Email: Rob.Dunne@csiro.au > > Java has certainly revolutionized marketing and litigation. > > >------------------------------ > >Message: 4 >Date: Fri, 01 Aug 2003 12:09:54 +1000 >From: Gordon Smyth <smyth@wehi.edu.au> >Subject: [BioC] Re: Spelling mistakes and some questions re limma >To: "Dave Waddell" <dwaddell@nutecsciences.com> >Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> >Message-ID: <5.2.0.9.1.20030801111855.00aed328@imaphost.wehi.edu.au> >Content-Type: text/plain; charset="us-ascii"; format=flowed > >Dear Dave, > >At 10:45 PM 31/07/2003, Dave Waddell wrote: > >You have a couple of spelling mistakes in the page: > > > ><http: bioinf.wehi.edu.au="" limma="" library="" limma="" html="" 5linearmodels.htm="" l="">http >://bioinf.wehi.edu.au/limma/library/limma/html/5linearmodels.html > > > >estime and explanded > >Thanks for letting me know. These typos have been corrected in later >versions of limma. > > >Can you point me to a place that would more fully explain the design > >matrix and contrasts with respect to 2-colour dye experiments? > >My best suggestion at this time is: > >Yang, Y. H., and Speed, T. P. (2003). Design and analysis of comparative >microarray experiments. In T. P. Speed (ed.), Statistical Analysis of Gene >Expression Microarray Data. Chapman & Hall/CRC Press, pages 35-91. > >But basically limma is breaking new ground here so there are no good >references for this stuff apart from the User's Guide itself. I am working >on providing more user friendly interfaces to create design and contrast >matrices and more documentation, but obviously these things take time. In >the meantime, a local statistician would be able to give you some help. Or >you could ask for help on bioconductor about specific designs. > > > In some Bioconductor packages, the design matrix appears to be > > applicable to the Cy3/Cy5 experiment as a whole and in others to the > > individual Cy3 and Cy5 experiments. > >I am not clear what you mean here. As far as I know, limma is the only >package to have the concept of a design matrix and limma is designed to >analyze the whole experiment at once. Other packages basically assume you >are making only one comparison usually with replicate arrays. > > > It is very confusing. In addition, the meaning of a contrasts matrix >and > > how to put one together is not very clear. Both of these values, if > > applied incorrectly, would appear to me (as a non-statistician assigned > > to put together a package) to completely change the results. > >Yes, this is true. > > > Finally, can you tell me how limma handles control spots? > >The only explicit handling of control spots in limma is in the plotMA >function. I assume that you will leave the control spots in during the >normalization (perhaps using weights to downweight ratio controls spots or >to upweight MSP titration spots) and you will remove them before doing >inference about differential expression. There are subsetting commands to >make removing control spots easy. > > >Thanks for a great package, Dave. > >Thanks for your comments. > >Gordon > > >------------------------------ > >Message: 5 >Date: Thu, 31 Jul 2003 22:31:13 -0400 (EDT) >From: "Rafael A. Irizarry" <ririzarr@jhsph.edu> >Subject: Re: [BioC] RMA t-test >To: James MacDonald <jmacdon@med.umich.edu> >Cc: bioconductor@stat.math.ethz.ch, dgrigor1@jhmi.edu >Message-ID: > <pine.gso.4.10.10307312222420.8322-100000@athena.biostat.jhsph.edu> >Content-Type: TEXT/PLAIN; charset=US-ASCII > >hi! fyi, all the ROC curves in the NAR paper comparing expression measures >was done on 1-1 comps (i.e. 2 chips). rma seems to perform weel >according to these curves. notice that if you only have one >chip median polish turns into a median which in my opinion is not a >terrible thing to use. > >as for t-tests with two arrays all you could use for estimating >variability (denominator in the t-test) are the residuals from the median >polish fit. these have (at least) two problemsB >1) as james points out they have no information about biological >variation >2) its not clear what the statistical properites of these residuals are. >the se estimate one gets with expresso-rma are given only as an ad-hoc >estimate of uncertainty of the expression estimates due to technology. > >hope this helps, >rafael >On Mon, 28 Jul 2003, James MacDonald wrote: > > > I would be cautious about using RMA with only two chips. You will be > > estimating the probe-specific intensity with only two observations, so > > it is doubtful that the estimate will be very accurate. I recall reading > > somewhere that a good minimum number of chips is around 5-6 for RMA. > > > > As for a t-test with only one observation per group, this is not > > possible. How are you going to estimate the variance for each group? > > Without replication all you can do is ratios, and you are then stuck > > with the assumption that large ratios equal significant differences. > > > > Jim > > > > > > > > > > James W. MacDonald > > Affymetrix and cDNA Microarray Core > > University of Michigan Cancer Center > > 1500 E. Medical Center Drive > > 7410 CCGC > > Ann Arbor MI 48109 > > 734-647-5623 > > > > >>> DMITRY GRIGORYEV <dgrigor1@jhmi.edu> 07/28/03 12:08PM >>> > > Hi everyone. > > > > One quick question. > > When I run RMA on just two chips, how could I conduct pairwise t-test > > for each probe set between these chips? > > > > Thank you > > > > Dima > > > > _______________________________________________ > > Bioconductor mailing list > > Bioconductor@stat.math.ethz.ch > > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > > > _______________________________________________ > > Bioconductor mailing list > > Bioconductor@stat.math.ethz.ch > > https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > > > >------------------------------ > >Message: 6 >Date: Fri, 01 Aug 2003 15:30:19 +1000 >From: Gordon Smyth <smyth@wehi.edu.au> >Subject: Re: [BioC] Repost: marrayNorm 1.1.3 gets stuck >To: Rob.Dunne@csiro.au >Cc: BioC Mailing List <bioconductor@stat.math.ethz.ch> >Message-ID: <5.2.1.1.1.20030801151709.00b1ee48@imaphost.wehi.edu.au> >Content-Type: text/plain; charset="us-ascii"; format=flowed > > > >Hi List, > > > >Please excuse the repost. No one responded to my > >previous post -- and it seems to me to be quite > >important. > > > >The problem is the new marrayNorm 1.1.3 > >(installed with bioconductor 1.2) -- which seems to get > >stuck in an endless loop > >It isn't in an endless loop, it's just very slow. > >The problem is the loess function. If you use family="symmetric" and >iterations=4 to get a robust loess curve rather than just least squares, >then the function is quite slow with lots of data and you get heaps of >warnings associated with memory limits and the use of a k-d tree. If you >use surface="direct" to avoid the k-d tree and stop the warnings, then the >function is very slow indeed with lots of points. You see the result below >when you try to run it on 30,000 data points. > >Versions of marrayNorm prior to 1.1.3 used least squares for the loess >curves - much quicker but not ideal as a normalization tool. > >I have used some tricks to avoid this sort of speed degradation in the >limma package. I believe that Jean is in the process of implementing to >same sort of thing in the marrayNorm package. > >Regards >Gordon > > >marrayNorm 1.1.3 (installed with bioconductor 1.2) > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > >Timing stopped at: 8874.73 19.65 10289.06 0 0 > > > >ie I interrupted the process - > >but with marrayNorm 1.1.1 reinstalled > > > > marrayNorm 1.1.1 > > > unix.time(experiment1.norm<-maNorm(experiment1, norm="loess")) > >[1] 803.99 29.73 843.40 0.00 0.00 > > > > > > > >is there a known problem with this package? > > > > bye > > rob > > > >-- > >Rob Dunne Fax: +61 2 9325 3200 Tel: +61 2 9325 3263 > >CSIRO Mathematical and Information Sciences +61 2 9325 3100 > >Locked Bag 17, North Ryde, New South Wales, Australia, 1670 > ><http: matilda.vu.edu.au="" ~dunne="">http://matilda.vu.edu.au/~dunne Email: > ><https: www.stat.math.ethz.ch="" mailman="" listinfo="" bioconductor="">Rob.Dunn e at > >csiro.au > > >------------------------------ > >_______________________________________________ >Bioconductor mailing list >Bioconductor@stat.math.ethz.ch >https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor > > >End of Bioconductor Digest, Vol 6, Issue 1 > >_______________________________________________ >Bioconductor mailing list >Bioconductor@stat.math.ethz.ch >https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor _______________________________________________ Bioconductor mailing list Bioconductor@stat.math.ethz.ch https://www.stat.math.ethz.ch/mailman/listinfo/bioconductor
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