That's not a meaningful metric in RNAseq, for the reason you mentioned and the fact that even if the exact transcriptome size of a particular cell type were known you'd want enough reads to properly handle the dynamic range in expression levels, rather than caring about an average level.

Thanks Dpryan for your reply. So let me to get it right, in your opinions, you would rather to look at the number of reads/ sample from a run than the coverage depth as we commonly look at when dealing with transcriptome sequencing? Actually, I had a similar thought as you. I was taught that the number of reads is important when handling the RNAse, but, I was confused when my PI wanted me to do a transcriptome sequencing on human total RNA to generate a 30-50millions reads and read depth of 50x. I have no issue with the number of reads but I was confused with the read depth. How should I calculate the depth? Can I use the normal human genome size (~3billions) for it?

Thanks again for the advice
Ed

Just ignore the "50x" part, there's no worthwhile way to calculate it (if your PI complains, just send him/her here to ask).