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Pivotal role of the renin/prorenin receptor in angiotensin II production and cellular responses to renin
Genevieve Nguyen, … , Thomas Giller, Jean-Daniel Sraer
Genevieve Nguyen, … , Thomas Giller, Jean-Daniel Sraer
Published June 1, 2002
Citation Information: J Clin Invest. 2002;109(11):1417-1427. https://doi.org/10.1172/JCI14276.
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Article Vascular biology

Pivotal role of the renin/prorenin receptor in angiotensin II production and cellular responses to renin

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Abstract

Renin is an aspartyl protease essential for the control of blood pressure and was long suspected to have cellular receptors. We report the expression cloning of the human renin receptor complementary DNA encoding a 350–amino acid protein with a single transmembrane domain and no homology with any known membrane protein. Transfected cells stably expressing the receptor showed renin- and prorenin-specific binding. The binding of renin induced a fourfold increase of the catalytic efficiency of angiotensinogen conversion to angiotensin I and induced an intracellular signal with phosphorylation of serine and tyrosine residues associated to an activation of MAP kinases ERK1 and ERK2. High levels of the receptor mRNA are detected in the heart, brain, placenta, and lower levels in the kidney and liver. By confocal microscopy the receptor is localized in the mesangium of glomeruli and in the subendothelium of coronary and kidney artery, associated to smooth muscle cells and colocalized with renin. The renin receptor is the first described for an aspartyl protease. This discovery emphasizes the role of the cell surface in angiotensin II generation and opens new perspectives on the tissue renin-angiotensin system and on renin effects independent of angiotensin II.

Authors

Genevieve Nguyen, Françoise Delarue, Céline Burcklé, Latifa Bouzhir, Thomas Giller, Jean-Daniel Sraer

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Figure 3

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Membrane expression of N14F protein and renin binding by HMC cells trans...
Membrane expression of N14F protein and renin binding by HMC cells transformed with N14F. (a) Saturation of binding on the HMC clone 2 (HMC2) expressing the receptor (squares, total; circles, nonspecific) and on HMC control cells (+, total; ×, nonspecific). The nonspecific binding was determined in the presence of 100 nM cold renin. Inset: Scatchard plot of the binding of renin to HMC2. (b) Immunofluorescence and confocal analysis of the expression of N14F on HMC2 cells stably expressing N14F (upper panel) and by HMC control cells transfected with empty vector (lower panel). The cells were stained with anti-receptor Ab (dilution 1:1,000) and with TRITC–conjugated secondary Ab.

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