1 We have compared the expression of protein kinase C (PKC) activity and immuno-detectable isoenzymes in cytosolic and membrane extracts of rat and human cardiovascular tissues (heart, kidney, aorta, saphenous vein). Experiments were performed in raw extracts and upon combined diethylaminoethylcellulose (DEAE) and phenylsepharose column chromatography. 2 PKC activity that bound to DEAE mostly eluted with 200 mM NaCl. DEAE-puri®ed PKC from all tissues except rat kidney bound almost quantitatively to phenylsepharose and eluted with 0.5 ± 0 M NaCl. 3 Immunoblots with an antibody against classical PKCs and the activator pro®le for phosphatidylserine, diolein and Ca 2+ revealed that the PKC from rat kidney, which did not bind to phenylsepharose, was most probably due to a proteolytically-generated, constitutively active PKC which is not under the control of a regulatory subunit. 4 Studies in the reference tissue, rat brain, demonstrated that all PKC isoenzymes investigated (classical PKCs a, b, g, new PKCs d, e, Z, y, and atypial PKCs z, l, i) have similar DEAE and phenylsepharose chromatography elution pro®les. In the functional assay an inhibitor of all known PKC isoenzymes, bisindolylmaleimide, and a speci®c inhibitor of classical PKCs, GoÈ 6976, both inhibited PKC from rat brain completely and with high potency indicating that the functional assay preferentially detects classical PKC isoenzymes. 5 Each PKC isoenzyme had a tissue-speci®c expression pro®le which was similar in rat and man. The classical PKCa, the new PKCs d and e and all atypical PKCs were detectable in most tissues, whereas the PKCb and PKCg were not detected in any pheripheral tissue; PKCZ and PKCy were found in some tissues. 6 We conclude that combined DEAE and phenylsepharose chromatography is useful to enrich and detect PKC isoenzymes; no major species dierences in tissues-speci®c expression patterns appear to exist between rat and man.