Epoxide hydrolases (EHs) are attractive enzymes for producing enantiopure epoxides and diols, but do not display enough stability when lysates or?Escherichia coli?whole cells are used as biocatalysts. In this work, an organic-solvent tolerant strain?Rhodococcus ruber?THdAdN was utilized to overexpress an epoxide hydrolase from?Agrobacterium radiobacter?(ArEH), using?E. coli?BL21(DE3) as a control. The proportion of ArEH in all soluble proteins of?R. ruber?THdAdN(ArEH) reached 30.3%, which was comparable to that of?E. coli?BL21(DE3)(ArEH). Due to a higher cell density in flask cultivation, the maximum ArEH activity of?R. ruber?THdAdN(ArEH) toward epichlorohydrin (ECH) reached 5.4 U/mL, approximately 5-fold higher than that of?E. coli?BL21(DE3)(ArEH). More importantly, compared with?E. coli?BL21(DE3)(ArEH), ArEH in?R. ruber?THdAdN(ArEH) showed a 10-fold enhanced thermostability, better tolerance against alkali pH, and reduced substrate and product inhibition, which significantly improved its performance in the resolution of high concentration ECH. By substrate feeding, 98.5%?ee?(R)-ECH was obtained with a 35.5% yield from 512?mM racemic ECH hydrolyzed by?R. ruberTHdAdN(ArEH). Compared with using free enzyme as biocatalysts, utilization of the?R. ruber?cells harboring ArEH improved the final (R)-ECH concentration by 46%.