does anyone have experience with this?
Thank you for your time!

In my experience with very similar calculations, there is something about the RPKM normalization which makes ERCC spike-ins behave abnormally in cases with widely-disparate RNA content, which i imagine that nucleus vs cytosol would fall into the category of. I can point you to some figures demonstrating this, if you'd like.

Your calculation is, I believe, an accurate one to do, if you're dealing with unnormalized data to begin with (raw counts, for example). One similar calculation which i use to determine the relative RNA content of two cells follows:

ρ=(<Total mass of spike-in>/<Total mass of sample>) * (<Total non-spike-in counts>/<Total counts of spike-in>)

It's a little unclear what you mean by "average NIST 14 spike in", but if you're referring to ERCC-00014, i wouldn't recommend choosing that particular spike in to normalize against, since it is present at a very low concentration in the commonly-used pools and therefore more affected by noise. In the above calculation, i actually use the *sum* of all 96 spike-ins for the mass and count calculations, although they don't vary too significantly if you choose a subset or even a single highly-expressed control to normalize to.