[BioC] Mapping Image ID's and Affy probesets
Robert Gentleman
rgentlem at fhcrc.org
Thu May 26 02:32:07 CEST 2005
Hi Aedin,
Aedin wrote:
> Thanks for the info on my last question. Can I please ask another ;-))
>
> What do you recommend to use when mapping IMAGE ID's and Affy ID's.
> UniGene and locus link are returning some very strange results (not a
> surprise really :-)).
>
It depends a lot on what you are trying to do. If you are trying to
combine different data sets, then you probably want to match on sequence
- which sounds like what you are suggesting below.
You might also want to look at MergeMaid, and accompanying papers, as
they have an interesting approach that might help.
I don' think that there is an example of taking a sequence, say for a
cDNA and then finding whether a corresponding affy probe set map to a
similar region, but once you are done I'm sure you will contribute one :-)
I would use Biostrings, and the corresponding Affy probe package - and
do exact matching.
If you end up with many-to-many or many-to-one matches I would match
them all and then pick the best one.
some code snippets,
library(annotate)
library(hgu95av2probe)
##here you would use the Acc. Num for the gen of interest
myseq = getSEQ("D45132")
##here you would use the Affy probe id, for the putative match
wp= hgu95av2probe$Probe.Set.Name == "316_g_at"
myPr = hgu95av2probe[wp,]
nchar(myseq)
library(Biostrings)
mybs = NucleotideString(myseq, "DNA")
##do this once for each of the probes - and count how many actually ##match
match1 = matchDNAPattern(as.character(myPr[1,1]), mybs)
as.matrix(match1)
Does that help?
Robert
> I know match probes maps between Affy batches. Can I load IMAGE
> sequences into this to map to a Affy cdf package. Is there any example
> of this in the BioC help?
>
> Thanks again BioC for all your help,
> Aedin
>
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