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I'm trying to use biomaRt to convert a list of more than 90k probe IDs to the gene symbols, but am having problems. Using the getBM function, I can see that only 22k of those have corresponding gene symbols, but the output is a vector of length 22k, and I am unable to see the correspondence to the initial probe ID list. Using getBMlist, I can get an output with na values specified for those probes that don't match, but the function gives a warning message that getBMlist isn't for large lists. How do I get an output of 90k gene symbols and na values?

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What do you have when you set uniqueRows = FALSE, I mean getBM(attributes=...,uniqueRows = FALSE)? – agstudy Mar 14 '13 at 18:26
    
I get repeats of the same gene symbol. It doesn't help in terms of inserting na values for those probes that aren't found. – user794479 Mar 15 '13 at 4:02
1  
It is not clear for me what you try to do so? Can you please add your getBM reaquest to the OP, and what do you get as result. Quickly Reading the documentation , you should get a data.frame with 2 columns... – agstudy Mar 15 '13 at 4:13

To get the mappings between probeID and gene symbol you need to include the probeID in the biomaRt attributes.

Here's how I did it for some of my work using agilent microarrays:

genes<-c("A_23_P10060", "A_23_P10091", "A_23_P103951", "A_23_P10525", "A_23_P105732", "A_23_P10605", "NM_005325")

library(biomaRt)
ensembl<-useMart("ensembl", dataset="hsapiens_gene_ensembl")

ensembl.id<-grep("ENST", genes, value=T)
agilent.df<-getBM(attributes = c("hgnc_symbol","efg_agilent_wholegenome_4x44k_v1"), filters=c("efg_agilent_wholegenome_4x44k_v1"),values=genes, mart=ensembl)

genes<-merge(x = as.data.frame(genes),y =  agilent.df, by.y="efg_agilent_wholegenome_4x44k_v1", all.x=T, by.x="genes")

There is a very good biomaRt tutorial that walks you though the same process. If you run this code you'll notice that one probe will have "" for a hgnc_symbol, that's because it exists in the ensemble mart but has no designated gene symbol.

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