well, no magic here. The package assumes that you know in advance genes that do not change the expression due to treatments, and if you see the change, then its caused by the batch effect. Here is the manual http://bioconductor.org/packages/release/bioc/vignettes/RUVSeq/inst/doc/RUVSeq.pdf

Hi Ahill, two treatments are 3 and 3d, i.e. human cells at 3 hours incubated with viable fungal cells (3) and human cells incubated with dead fungal cells (3d). So basically time effect cancels out. I did not receive any feedback from the developer and Bioconductor community, but anyways used the package and it actually gave biologically meaningful results, so I tend to trust them. Regarding the control genes, so I chose the genes which are not differential expressed during the whole time course of infection, on top of that we have the same design with 3 other fungal species, so I took the common non-DE genes across the infection with 4 species (we see that the human response is quite similar to all of them). Of course I can not be 100% sure that these control genes (around 200 highly expressed genes) are completely intact, but I guess there is a pretty high chance for that - if these genes do not change the expression levels when exposed to 4 different fungal pathogens, I assume they still will be intact when exposed to dead fungal cells of that same species. Does it sound reasonable? Regarding if the batch effect is gene-dependent, so my assumption (which might be wrong) that the batch effect is systematic across all genes, but to be honest I have no idea. In our case there could be many sources of the effect - experiments were done 1 year apart from each other (we basically are testing a hypothesis based on the 1st batch data), though by the same person, but library preps and sequencing was done by different people.