If you're working with a RNA virus, remember you'll have to find a way to differentiate between genome (and any genomic intermediates) and viral mRNA.

I am not sure I understand. When you say variant, do you mean at the level of DESeq 2 or prior to that?

Also, I am not sure I understand how to do the DE only for the viral genes when the counts include both viral + host. Can you help me with that?

Thanks!

I have a doubt about the method you have recommended for DeSeq2. Is there a way to estimate size factors using the entire data (host+viral) but then calculate differential expression for only the viral genes?

The way I am doing it right now is using the entire counts (host+viral) that I got from htSeq and used it to calculate differential expression for all the genes and then extracted out the data for just the viral genes.. Will the fold change be different between the 2 methods (if method 1 is possible at all).

Thank you for your help!

I find this discussion very useful for my question. Can we use the same method to calculate DE of host genes? We have few virus infected sheep samples but each sample has different amount of virus present in tissue, so I am thinking it may effect on finding significant gene expression in infected sheep vs normal sheep. My idea is to use virus and host combined counts in DESeq2 and normalise them and then run DE part for sheep(host). Will it help? I am afraid how it will effect on normalising control samples where there is no virus present.