Pseudorenin: A NEW ANGIOTENSIN-FORMING ENZYME

Skeggs, Leonard T.; Lentz, Kenneth E.; Kahn, Joseph R.; Dorer, Frederic E.; Levine, Martin

doi:10.1161/01.res.25.4.451

Cited by 88 publications

(28 citation statements)

References 8 publications

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“…Our preliminary experiments (unpublished observations) as well as experiments reported by others 17 ' 18 demonstrated the presence of acid proteases in preparations of vascular enzymes. Since acid proteases can cleave angiotensin I from angiotensinogen, 17 ' I823U methods were used to: 1) remove acid proteases from preparations of vascular renin-like activity; 2) minimize the angiotensin I-generating activity of nonspecific acid proteases; and 3) quantitate any residual proteolytic activity.…”

Section: Methodssupporting

confidence: 78%

“…When incubated with nephrectomized rat plasma, the acid proteases generated no AI. Although in previous studies 17 ' ' *• " • " and in our own unpublished experiments acid proteases can generate AI from angiotensinogen, in the current study the use of proteolytic inhibitors throughout isolation and assay procedures minimized the capacity of acid proteases to generate AI.…”

Section: Results Experiments 1: Aortas From Normal Ratsmentioning

confidence: 65%

“…To maximize detection of vascular renin, activity was assayed near the pH optimum of renin. "• 19~22 Since nonspecific acid proteases can generate AI from angiotensinogen at near the optimal pH for renin activity, 17 ' 18 ' a all samples were incubated with proteolytic inhibitors and any residual activity was removed by chromatography over immobilized bovine hemoglobin. Activity of nonspecific acid proteases was monitored by radiochemical assay.…”

mentioning

confidence: 99%

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Absence of renin-like activity in rat aorta and microvessels.

Fordis¹,

Megorden²,

Ropchak³

et al. 1983

Hypertension

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SUMMARY Vascular renln-llke activity was studied in the aortas and the cerebral microvessels of Sprague-Dawley rats and in the aortas of spontaneously hypertensive rats. Methods were employed to maximize detection of tissue renin and to simultaneously minimize contamination of that activity by either plasma renin or nonspecific proteases capable of angiotensin I generation. To this end, renin activity was measured near its pH optimum; plasma renin was eliminated by nephrectomy; and nonspecific proteases such as cathepsin D were either inhibited by proteolytic blockers or removed by chromatography over immobilized bovine hemoglobin. Aortic vascular renin-like activity was detected in rats not subjected to nephrectomy and could be inhibited by preincubation of samples with antimouse renin antibody shown to cross-react and inhibit rat plasma renin activity. extrarenal vessels may be a source of renin;'" 16 but measurement of vascular renin (i.e., renin arising in vessel wall) can be complicated by the presence in vessel wall of other enzymatic activities capable of generating angiotensin I (AI) in the renin assay. 1718 In the present study, methods were used to maximize detection of vascular renin and to simultaneously minimize contamination of that activity by either nonspecific proteases or plasma renin. To maximize detection of vascular renin, activity was assayed near the pH optimum of renin. "• 19~22 Since nonspecific acid proteases can generate AI from angiotensinogen at near the optimal pH for renin activity, 17 ' 18 ' a all samples were incubated with proteolytic inhibitors and any residual activity was removed by chromatography over immobilized bovine hemoglobin. Activity of nonspecific acid proteases was monitored by radiochemical assay. 24 Despite the removal of nonspecificFrom the Hypertension-Endocrine Branch, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda, Maryland.Current address for Dr. Fordis: Laboratory of Chemical Biology, N1ADDK, Bldg. 10, Room 9N-321, National Institute of Health, Bethesda, Maryland 20205.Address for reprints: Dr. Harry R. Keiser, National Heart, Lung, and Blood Institute, Building 10, Room 8C-1O3, Bethesda, Maryland 20205.Received March 2, 1982; revision accepted April 18, 1983. acid proteases, a renin-like activity could be detected in rat aorta. To eliminate the possibility that the reninlike activity in rat aorta represented plasma renin contamination, rats were nephrectomized; and plasma renin activity and vascular renin-like activity were measured at 2, 6, and 24 hours after nephrectomy. After the disappearance of plasma renin activity, no vascular renin-like activity could be detected in aortas collected from either Sprague-Dawley or spontaneously hypertensive rats (SHR). Vascular renin-like activity was also absent from microvessels collected from the rat cerebral cortex. Materials and MethodsExperiments were designed to examine vascular renin-like activity in both large vessels (aortas) and small resistance vessels (cerebral micr...

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Section: Methodssupporting

confidence: 78%

Section: Results Experiments 1: Aortas From Normal Ratsmentioning

confidence: 65%

mentioning

confidence: 99%

See 1 more Smart Citation

Absence of renin-like activity in rat aorta and microvessels.

Fordis¹,

Megorden²,

Ropchak³

et al. 1983

Hypertension

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“…Considerable debate exists in the literature concerning the identity of renin-like enzymes (based upon the ability to generate angiotensin I) in extra- (Day and Reid, 1976;Dorer et al, 1978;Ganten et al, 1976;Hackenthal et al, 1978;Skeggs et al, 1969). Pseudorenin and isorenin (Skeggs et al, 1969), an angiotensin-forming enzyme with an acidic pH optimum, are widely distributed in mammalian tissues.…”

Section: Discussionmentioning

confidence: 99%

“…Pseudorenin and isorenin (Skeggs et al, 1969), an angiotensin-forming enzyme with an acidic pH optimum, are widely distributed in mammalian tissues. Pseudorenin recently has been identified as cathepsin D (Dorer et al, 1978); the predominant portion of brain isorenin activity also has been identified as cathepsin D (Hackenthal et al, 1978).…”

Section: Discussionmentioning

confidence: 99%

Specific antibody to hog renal renin and its application to the direct radioimmunoassay of renin in various organs.

Hirose¹,

Workman²,

Inagami³

1979

Circulation Research

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SUMMARY We produced anti-hog renin antibodies using as antigens pure hog renal renin that either had been insolubilized or conjugated to tetanus toxoid. High titer antibodies were obtained, which demonstrated different cross-reactivity with renins from other species. A direct radioimmunoassay for renin was developed using antibody, monoiodinated lu I-hog renin, and various methods for separating free and antibody-bound trace. This assay was capable of detecting 40 pg of hog renin and was applied to the determination of renin in hog blood and other organs. Based on the direct measurement of renin by this radioimmunoassay, the renin-like activity (i.e., the ability to generate angiotensin I from renin substrate preparations) of the pituitary gland was found to be due mostly to true renin, whereas the renin activity of other hog tissues, including the adrenal gland, liver, lung, spleen, and submaxillary gland, was not identified as renin and may have been due to cathepsins. Cire Ret 45: 275-281, 1979

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The renin-angiotensin system

Peart

1976

Peptide Hormones

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Pseudorenin: A NEW ANGIOTENSIN-FORMING ENZYME

Cited by 88 publications

References 8 publications

Absence of renin-like activity in rat aorta and microvessels.

Absence of renin-like activity in rat aorta and microvessels.

Specific antibody to hog renal renin and its application to the direct radioimmunoassay of renin in various organs.

The renin-angiotensin system

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