I'm looking to validate key DEGs using qPCR after performing DGE analysis using RNAseq data. Instead of selecting canonical housekeeping genes as a reference I would like to use my RNAseq data to determine the most stable genes. How are people doing this? I'm looking at Normfinder, but the macros neither works for the Mac version of excel and the R package doesn't seem to work for me either. Importantly, I want to make an evidence based decision before obtaining qPCR data.

Please let me know!

Marina

There is a lot of references about the subject. E.g., two practical examples:

Use of RNA-seq data to identify and validate RT-qPCR reference genes for studying the tomato-Pseudomonas pathosystem

Systematic identification and validation of the reference genes from 60 RNA-Seq libraries in the scallop Mizuhopecten yessoensis

Some authors claim RNAseq is not necessary to find good reference genes:

RNA-Seq is not required to determine stable reference genes for qPCR normalization

But, as you already have the RNAseq, it doesn't hurt, either.