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Am J Physiol Heart Circ Physiol 294: H2421-H2427, 2008. First published April 25, 2008; doi:10.1152/ajpheart.01225.2007
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Sex Steroids and Gender in Cardiovascular-Renal Physiology and Pathophysiology

Genomic deletion of estrogen receptors ER{alpha} and ERβ does not alter estrogen-mediated inhibition of Ca2+ influx and contraction in murine cardiomyocytes

Nina D. Ullrich,1 Andree Krust,2 Peter Collins,1 and Kenneth T. MacLeod1

1Imperial College London, Cardiac Medicine, National Heart and Lung Institute, London, United Kingdom; and 2Université Louis Pasteur, Institut de Génétique et Biologie Moléculaire et Cellulaire, Centre National de la Recherche Scientifique, Illkirch, Communauté Urbaine de Strasbourg, France

Submitted 22 October 2007 ; accepted in final form 21 April 2008

Estrogens modify contraction of vascular smooth muscle and cardiomyocytes, but suggestions that they confer protective effects on the cardiovascular system remain controversial. The negative inotropic effects of estrogens are a consequence of L-type Ca2+ channel inhibition, but the underlying mechanisms remain elusive. We tested the hypothesis that membrane-associated estrogen receptors (ER)-{alpha} and -β are involved. We measured the effect of estrogens on Ca2+ current (ICaL) in isolated ventricular cardiomyocytes of wild-type (WT), ER{alpha} knockout (ER{alpha}KO), and ERβKO mice using the whole cell patch-clamp technique at 37°C. No differences in current densities or inactivation profiles of ICaL were found under control conditions in WT, ER{alpha}KO, and ERβKO cardiomyocytes, suggesting that absence of either ER has no effect on functional properties of ICaL. In all groups, application of raloxifene (2 µM) or 17{alpha}- or 17β-estradiol (50 µM) reduced ICaL (P < 0.001). Raloxifene decreased ICaL by 44 ± 9% (mean ± SE) in WT (n = 5), 34 ± 5% in ER{alpha}KO (n = 5), and 30 ± 5% in ERβKO mice (n = 8). 17{alpha}-Estradiol reduced ICaL by 41 ± 10% in WT (n = 4), 34 ± 12% in ER{alpha}KO (n = 7), and 38 ± 8% in ERβKO mice (n = 7). 17β-Estradiol inhibited ICaL by 31 ± 4% in WT (n = 4), 28 ± 6% in ER{alpha}KO (n = 3), and 42 ± 3% in ERβKO mice (n = 5). Decreases in cell shortening occurred in parallel with these findings. Our results suggest that inhibition of ICaL and the decrease in contraction by estrogens do not depend on ER{alpha} or ERβ.

L-type calcium channel; excitation-contraction coupling; cardiac electrophysiology





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