Estrogen Modulates AT 1 Receptor Gene Expression In Vitro and In Vivo

Author:

Nickenig Georg1,Bäumer Anselm T.1,Grohè Christian1,Kahlert Stefan1,Strehlow Kerstin1,Rosenkranz Stephan1,Stäblein Alexander1,Beckers Frank1,Smits Jos F. M.1,Daemen Mat J. A. P.1,Vetter Hans1,Böhm Michael1

Affiliation:

1. From the Klinik III für Innere Medizin, Universität zu Köln (G.N., A.T.B., K.S., S.R., A.S., F.B., M.B.), and the Medizinische Universitäts-Poliklinik, Bonn (C.G., S.K., H.V.), Germany; and the Departments of Pharmacology (J.F.M.S.) and Pathology (M.J.A.P.D.), Cardiovascular Research Institute, University of Maastricht, the Netherlands. Drs Nickenig and Bäumer contributed equally to this study.

Abstract

Background —The AT 1 receptor has been implicated in the pathogenesis of hypertension and atherosclerosis. Estrogen deficiency is also associated with cardiovascular diseases. Therefore, we examined the AT 1 receptor gene expression in ovariectomized rats with and without estrogen replacement therapy and the influence of estrogen on AT 1 receptor expression in cultured vascular smooth muscle cells. Methods and Results —Rat aortic tissue was examined 5 weeks after ovariectomy. In one group, estrogen (1.7 mg estradiol) was administered during the 5-week period. Functional experiments assessed angiotensin II–induced contraction of aortic rings. AT 1 receptor mRNA levels were measured by quantitative polymerase chain reaction and Northern blotting. AT 1 receptor density was assessed by radioligand binding assays. These techniques were also applied in cultured vascular smooth muscle cells. The efficacy of angiotensin II on vasoconstriction was significantly increased in aortas from ovariectomized rats. As assessed by radioligand binding assays, AT 1 receptor density was increased to 160% without changes in receptor affinity during estrogen deficiency. AT 1 receptor mRNA levels were consistently increased to 187% in ovariectomized rats compared with sham-operated animals. Estrogen substitution therapy in ovariectomized rats reversed this AT 1 receptor overexpression. To explore the underlying mechanisms, the direct influence of estradiol on AT 1 receptor expression was investigated in VSMCs. Estradiol (1 μmol/L) led to a time-dependent downregulation of AT 1 receptor mRNA, with a maximum of 33.3% at 12 hours. There was a correlative decrease in AT 1 receptor density. Conclusions —This novel observation of estrogen-induced downregulation of AT 1 receptor expression could explain the association of estrogen deficiency with hypertension and atherosclerosis, because activation of the AT 1 receptor plays a key role in the regulation of blood pressure, fluid homeostasis, and vascular cell growth.

Publisher

Ovid Technologies (Wolters Kluwer Health)

Subject

Physiology (medical),Cardiology and Cardiovascular Medicine

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