Normally you do it after normalization, though there's typically not much difference to doing it before vs. after. Regarding the cut off, please see the genefilter package and the accompanying paper in PNAS.

Hello!

(Assuming you want to do differential gene expression expression analysis and you have RNAseq or similar type of data)

The edegR vignettes is a document where filtering is applied. I don't know of systemic studies addressing where to set the cutoff.

The vignettes quoted above apply the filter after transforming raw counts to counts per million.
In practice I think most of us apply a common sense threshold. If say a gene has 1 cpm (counts per million) in all the libraries, that gene can't be biologically interesting. The reason to reject genes early, i.e. before testing for de, is to make the adjustment for multiple testing less "aggressive".

See the Bourgon et al. 2010 paper in PNAS. That described microarrays, but the same applies to RNAseq. Detection power is optimized by performing the filtering on the p-values after testing. I do occasionally prefilter, but only with limma/voom when I get weird fits (sometimes that happens and you have to remove low expressors to get appropriate results).

BTW, this is why I use DESeq2, it does all of this for me.

Thanks - I'll have a look!