[BioC] LIMMA - fold change direction?
J.delasHeras at ed.ac.uk
J.delasHeras at ed.ac.uk
Fri Jul 18 12:31:31 CEST 2008
Quoting Glyn Bradley <glyn.bradley at googlemail.com>:
> Hi all
>
> 3 bio replicate and dye swap cDNA array experiment comparing 17day and
> 27day samples being analyzed with limma
> targets file:
> "Name" "FileNameCy3" "FileNameCy5" "Cy3" "Cy5"
> "1-Cy3-Ac-17d.txt" "1-Cy5-Ac-27d.txt" "17day" "27day"
> "2-Cy3-Ac-27d.txt" "2-Cy5-Ac-17d.txt" "27day" "17day"
> "3-Cy3-Ac-17d.txt" "3-Cy5-Ac-27d.txt" "17day" "27day"
> "4-Cy3-Ac27d.txt" "4-Cy5-Ac17d.txt" "27day" "17day"
> "5-Cy3-Ac17d.txt" "5-Cy5-Ac27d.txt" "17day" "27day"
> "6-Cy3-Ac27d.txt" "6-Cy5-Ac17d.txt" "27day" "17day"
>
> so after
> ...
> RG <- read.maimages(files, source="imagene")
> MA <- normalizeWithinArrays(RG)
> design=c(1,-1,1,-1,1,-1)
> fit <- lmFit(MA, design)
> .
> what direct are the fold changes I get out in
> does a positive FC mean up regulated in the 27day sample?
>
> Thanks
If in doubt, and you don't understand the design matrix, you can
simply find a probe with a large positive M value, and then look at
the raw intensities for that one. Then it will be obvious.
Jose
--
Dr. Jose I. de las Heras Email: J.delasHeras at ed.ac.uk
The Wellcome Trust Centre for Cell Biology Phone: +44 (0)131 6513374
Institute for Cell & Molecular Biology Fax: +44 (0)131 6507360
Swann Building, Mayfield Road
University of Edinburgh
Edinburgh EH9 3JR
UK
--
The University of Edinburgh is a charitable body, registered in
Scotland, with registration number SC005336.
More information about the Bioconductor
mailing list