Inhibitory Effect Of Reactive Oxygen Species On Angiotensin I‐Converting Enzyme (Kininase II)

SUMMARY 1. Somatic angiotensin I‐converting enzyme (ACE) is a protein that contains two similar domains (N‐ and C‐terminal), each possessing an active site. We have examined the effects of a generator of hydroxyl radicals (g • OH: 2,2′‐azo‐bis(2‐amidinopropane)) and hydrogen peroxide (H 2 O 2 ) on ACE using an in vitro approach. 2. The generator of hydroxyl radicals inactivated ACE in a time (2–6 h)‐ and concentration (0.3–3 mmol/L)‐dependent manner at 37°C. When ACE was coincubated for 4 h with g • OH (3 mmol/L), its activity decreased by 70%. Addition of dimethylthiourea or mannitol + methionine, two • OH scavengers, resulted in a significant protection of ACE activity. Mercaptoethanol and dithiotreitol, two thiol‐reducing agents, also efficiently protected ACE activity. 3. The hydrolysis of two natural and domain‐specific substrates was explored. The hydrolysis of angiotensin I, preferentially cleaved by the C‐domain, was significantly inhibited (57–58%) after 4 h exposure to g • OH (0.3–1 mmol/L). Under the same conditions of exposure, the hydrolysis of N ‐acetyl‐Ser‐Asp‐Lys‐Pro, a specific substrate for the N‐domain, was only slightly inhibited by 1 mmol/L g • OH. 4. Hydrogen peroxide, another source of • OH, was used. After exposure to H 2 O 2 (3 mmol/L; 4 h), an 89% decrease in ACE activity was observed. Pretreatment with the iron chelator deferoxamine (1 mmol/L) attenuated H 2 O 2 ‐mediated ACE inactivation, demonstrating that the effect of H 2 O 2 was partly due to its conversion into • OH (Fenton reaction). 5. In summary, our findings demonstrate that g • OH and H 2 O 2 inhibit ACE activity and suggest a preferential action of g • OH on the C‐domain of the enzyme.