[BioC] doing some math on an array of PM probes
James W. MacDonald
jmacdon at med.umich.edu
Wed Jan 5 18:55:24 CET 2005
Stuart Brown wrote:
>
> I would like to normalize probe signals per gene on a single Affy array
> by dividing
> each pm probe by the mean of all pm probes on that array. Never mind
> that this is a
> stupid thing to do, I have an idea...
>
> The command pm(affybatch)
> gives a single probe value in each row and adds a numerical suffix to
> the gene name so
> that each probe has a unique gene name.
>
> Instead, I'd like to extract the pm probes into a matrix that has a
> single Affy gene name for a row header and the signal values for all of
> the pm probes for that gene in the following columns of that row. Some
> genes will have different numbers of columns since they have different
> numbers of
> pm probes. [If I could just get a table in this shape, I could actually
> do all the rest of the work
> in Excel.]
You will have a hard time making a matrix in R that has different column
lengths (recycling rules will make the matrix rectangular). You will be
much better off using a list and the lapply() function.
mn <- mean(pm(abatch)) ## where abatch is the name of your AffyBatch
norm.pm <- lapply(pm(abatch, LISTRUE=TRUE), function(x) x / mn)
This will give you a list of all PM probes normalized by the overall mean.
HTH,
Jim
>
> Then I'd like to take the mean of all the probe signal values for each
> gene and write that into a new array that has just 2 rows - genename
> (which serves as the index) and mean-pm for that gene.
>
> Finally, I'd like to replace the values of each pm probe signal with the
> ratio of that probe signal divided by the mean of all pm probes for
> that gene.
>
> There must be an easy way to do this, but I'm new to Bioconductor.
>
> Thanks for any and all helpful suggestions
> -Stuart Brown
>
>
--
James W. MacDonald
Affymetrix and cDNA Microarray Core
University of Michigan Cancer Center
1500 E. Medical Center Drive
7410 CCGC
Ann Arbor MI 48109
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