You can use RNA-seq data to mine genetic markers (SNPs & indels) and also to generate expression profiles and perform an eQTL analysis. However, if your are using exon/CDS data, I think your are going to have a very small number of markers in comparison to that you could obtain from whole genome sequencing, whole exome or tGBS. In our lab we have a simple pipeline, we generate expression profiles via RNA-seq (10 million reads p library) and from the same individuals, we generate markers via tGBs (targeted genotyping by sequencing). This methods is relatively cheap (17k RNA-seq + 9 k tGBS) for ~96 individuals. But, if the mice your are testing for regulatory divergence have enough genetic differentiation, I think that RNA-seq-derived markers could be enough to build a linkage map. Happy bioinformatics!