[BioC] limma and single-dye (R) gpr
Paul Geeleher
paulgeeleher at gmail.com
Tue Jun 3 13:06:06 CEST 2008
Check out this previous thread from the mailing list:
http://article.gmane.org/gmane.science.biology.informatics.conductor/18032
/match=read+single+channel+genepix+limma+analyze+miRNA+experiment
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-Paul
On Mon, Jun 2, 2008 at 11:25 AM, Ng Stanley <stanleyngkl at gmail.com> wrote:
> Hi,
>
> I have inherited a set of single-dye (R) gpr, and need to process them via
> limma. After several tries, managed to load via read.maimages and
> backgroundCorrect using dummies values for G and Gb from R and Rb,
> respectively. Two questions:
>
> A) Am I right to say that normalizeWithinArrays for single-dye gpr ?
> B) How to normalize between arrays in the right way ? Should it
> be normalizeBetweenArrays(RG, method="quantile") or
> normalizeBetweenArrays(RG$R, method="quantile") or something else ?
>
> [[alternative HTML version deleted]]
>
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