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Title: Participation of neutral endopeptidase 24. 11 (NEP; enkephalinase A) in kinin metabolism in vitro and in vivo

Conference · · Fed. Proc., Fed. Am. Soc. Exp. Biol.; (United States)
OSTI ID:6943145

Studies were done in 2 phases in rats. (1) Bradykinin was added catheter-collected urine, and its hydrolysis was determined by RIA. Three different kiniases were found by application of specific inhibitors. Kininase I-type carboxypeptidase was inhibited by 2-mercaptomethyl-3-guanidinoethyl-thiopropanoic acid, kiniase II by captopril and NEP by phosphoramidon (PA). Surprisingly, NEP was responsible for 68% of total kininase, while kininase I and II contributed only 9 and 23%. (2) To study the effects of inhibition of NEP on renal function, rats were infused with PA (330 ..mu..g/hr/kg, n=6). Urinary kinin level, kininase, GFR, RBF, U/sub Na/V, U/sub K/V and UV were measured. PA decreased total urinary kininase activity from 284 to 58 ng/min/kg (77%, p < 0.01) and increased urinary kinin excretion from 74 to 128 pg/min/kg (73%, p < 0.02), UV from 72 to 82 ..mu..l/min/kg (15%, p < 0.01) and U/sub Na/V from 12 to 17 ..mu.. Eq/min/kg (37%, p < 0.02). PA did not change BP, RBF, GFR or U/sub K/V. /sup 125/I-Tyr-bradykinin infused into the aorta did not appear in urine intact during PA administration. In conclusion, this is the first demonstration of NEP catabolizing kinins in vivo; its inhibition increased the excretion of intrarenally generated kinins. Changes in water and electrolyte excretion may be caused by kinins generated in the distal nephron.

Research Organization:
Henry Ford Hospital, Detroit, MI
OSTI ID:
6943145
Report Number(s):
CONF-8604222-; TRN: 87-007015
Journal Information:
Fed. Proc., Fed. Am. Soc. Exp. Biol.; (United States), Vol. 45:4; Conference: 70. annual meeting of the Federation of American Society for Experimental Biology, St. Louis, MO, USA, 13 Apr 1986
Country of Publication:
United States
Language:
English