Loop design -> inferring
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@gordon-smyth
Last seen 8 hours ago
WEHI, Melbourne, Australia
Dear Yannick, Most clustering algorithms are invariant relative to linear transformations, so you can cluster with your individual array data without any transformation. It doesn't matter than you don't have a common reference, except from the point of view of interpretting the clustered patterns that you end up with. (Personally I usually prefer to cluster on fitted coefficients, but that's another matter.) To visualize variability, you have 10 reps of T0-T1, 10 of T1-T2, 10 of T2-T10. Why not just do boxplots for each group. Again no need to transform. Best wishes Gordon >Date: Thu, 9 Aug 2007 18:58:46 +0200 >From: Yannick Wurm <yannick.wurm at="" unil.ch=""> >Subject: [BioC] Loop design -> inferring >To: bioconductor at stat.math.ethz.ch > >Hello list, > >I am a graduate student doing some micorarray experiments on social >behavior in ants. I've recently started using limma, and have been >pleasantly surprised by the elegance of its implementation. This is >my first question to the list. > >My experiment is a 3 point time-course that I set up as a loop design >on our two-color cDNA arrays: > T0 -> T1 -> T2 ---> (back to T0) >My 10 replicates of this are dye-balanced. > >My favorite contrasts are T1-T0 and T2-T0. I can get my genes >estimated relative expression levels through either topTable or by fit >$coefficients. >However, I would like to visuallze relative expression levels, at the >level of individual replicates. That way I can get visual feeling of >how much variability there is between my replicates. And do >clustering as if I had used a reference design. >So for each gene I want 10 values for T1-T0, and 10 values for T2-T0. >I could get these by simply taking the numbers from my direct >comparisons. But it feels wrong ignoring the information provided >indirectly about T1-T0 through (T1-T2)+(T2-T0). > >How would you go about this? > >Thanks for any tips, > >Yannick
GO Clustering limma GO Clustering limma • 954 views
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Yannick Wurm ▴ 220
@yannick-wurm-2314
Last seen 10.2 years ago
Hello Gordon & list, thanks for your help. Clustering on the fitted coefficients make sense to see a gene's general profile. But once again, getting a feeling for a gene's variability is important because it gives information about both the gene's robustness, as well as the sample's. And if I'm looking at a large number of genes, it doesn't make sense to do boxplots for each. What I did for now is just directly use my individual array data. But I think I'd get a better estimation if I used the information provided by the loop. So for each comparison, I think I'll use a weigted average of the 2 loop directions. Eg if I want to estimate differences between T0 and T1, I could do: ratio = 2/3 * (T1vsT0) + 1/3 * (T1vsT2 - T2vsT0) Kind regards, yannick On Aug 12, 2007, at 11:41 PM, Gordon Smyth wrote: > Dear Yannick, > > Most clustering algorithms are invariant relative to linear > transformations, so you can cluster with your individual array data > without any transformation. It doesn't matter than you don't have a > common reference, except from the point of view of interpretting the > clustered patterns that you end up with. > > (Personally I usually prefer to cluster on fitted coefficients, but > that's another matter.) > > To visualize variability, you have 10 reps of T0-T1, 10 of T1-T2, 10 > of T2-T10. Why not just do boxplots for each group. Again no need > to transform. > > Best wishes > Gordon > >> Date: Thu, 9 Aug 2007 18:58:46 +0200 >> From: Yannick Wurm <yannick.wurm at="" unil.ch=""> >> Subject: [BioC] Loop design -> inferring >> To: bioconductor at stat.math.ethz.ch >> >> Hello list, >> >> I am a graduate student doing some micorarray experiments on social >> behavior in ants. I've recently started using limma, and have been >> pleasantly surprised by the elegance of its implementation. This is >> my first question to the list. >> >> My experiment is a 3 point time-course that I set up as a loop design >> on our two-color cDNA arrays: >> T0 -> T1 -> T2 ---> (back to T0) >> My 10 replicates of this are dye-balanced. >> >> My favorite contrasts are T1-T0 and T2-T0. I can get my genes >> estimated relative expression levels through either topTable or by >> fit >> $coefficients. >> However, I would like to visuallze relative expression levels, at the >> level of individual replicates. That way I can get visual feeling of >> how much variability there is between my replicates. And do >> clustering as if I had used a reference design. >> So for each gene I want 10 values for T1-T0, and 10 values for T2-T0. >> I could get these by simply taking the numbers from my direct >> comparisons. But it feels wrong ignoring the information provided >> indirectly about T1-T0 through (T1-T2)+(T2-T0). >> >> How would you go about this? >> >> Thanks for any tips, >> >> Yannick > > _______________________________________________ > Bioconductor mailing list > Bioconductor at stat.math.ethz.ch > https://stat.ethz.ch/mailman/listinfo/bioconductor > Search the archives: http://news.gmane.org/ > gmane.science.biology.informatics.conductor
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