My feeling is that this would be very much dependent on the expression levels of the gene. If gene you are looking at is lowly expressed then chances of being able to see counts for it are close to nil. In best of circumstances you will likely detect 20-30% of expressed genes in a single cell experiment. At least that is my peripheral understanding.

I am trying to determine if the amount of these cells is greater in one type of patient with skin disease compared with another patient with a slightly different subtype of the disease.

That is a different question that can't be easily answered by RNAseq of any type.

In addition to that, you will need good experimental replication to show differences of cellular proportions, especially in humans that can be confounded by a lot of factors, and with single-cell technology this is going to be very expensive. Frankly, as a reviewer I would ask for FACS-based validation of this if you do it with NGS technology because all the enrichment and preparation steps in scRNA-seq can lead to all kinds of biases. I think a simple FACS-based assessment is much cheaper, more straight-forward and in this context more reliable. @OP, since you ask about NGS, is there any reason the more traditional techniques like FACS or IHC do not work here? Are there no antibodies for the particular markers you identified or are there no markers that are targetable in general?

thank you jared.andrews07 for taking the time to reply and provide your insights which are most helpful. I am also finding staining for intracellular IL22 extremely difficult with flow ! I hopefully will find a way forward!