Cardiac hypertrophy induced by volume overload significantly downregulated AT1 receptors on fibroblasts (42,970 vs 73,870 sites/cell, P<0.01) and enhanced Ang II [Ca2+]i sensitivity in cardiomyocytes.
This study investigates the cellular localization and regulation of endothelin-1 (ET-1) and angiotensin II (Ang II) receptors and the effects of ET-1 and Ang II on Ca2+i in cardiac hypertrophy due to volume overload in the rat. Radioligand binding assays and Ca2+i measurements by fura 2 methodology were performed on isolated ventricular cardiomyocytes and fibroblasts from the heart of rats with a 4-week aortocaval shunt. In the hypertrophied myocardium, ET-1 and Ang II concentrations were unchanged in ventricles. Ventricular ET-1 receptors had a cell-specific distribution: > 90% of ET receptors in cardiomyocytes are of the ETA subtype, whereas fibroblasts had a nearly equal proportion of the ETA and ETB subtypes. ET-1 receptor densities, affinities, and ET-1-induced Ca2+i were not significantly different from control in both ventricular cell types from hypertrophied myocardium. Ang II specific binding was very low on isolated ventricular cardiomyocytes, suggesting few receptors in control conditions. However, Ca2+i responses induced by Ang II at concentrations > 10(-8) mol/L were detectable and were significantly higher in hypertrophied cardiomyocytes. Ang II receptor density (exclusively AT1) on fibroblasts was significantly reduced (42,970 +/- 3330 versus 73,870 +/- 7940 sites per cell for control cells, P < .01), but AT1 receptor affinity was unchanged after volume overload. The maximum increase in Ca2+i evoked by 10(-6) to 10(-4) mol/L Ang II was significantly lower in fibroblasts from overloaded hearts. In conclusion, ET-1 receptor proportion is cell specific, with cardiomyocytes possessing predominantly the ETA subtype and fibroblasts possessing both ETA and ETB receptors. Plasma and cardiac ET-1 concentrations and ET-1 receptor regulation on both ventricular cell types are not altered in cardiac volume overload, suggesting that cardiac ET-1 may not play a significant role in this model. Cardiac hypertrophy induced a significant downregulation of AT1 receptors on fibroblasts, whereas total binding and Ca2+i sensitivity to Ang II were significantly enhanced in hypertrophied cardiomyocytes. This suggests that cardiac Ang II may be involved in the pathophysiology of the cardiac hypertrophy of volume overload.
Fareh et al. (Thu,) conducted a other in Cardiac hypertrophy due to volume overload. Volume overload (aortocaval shunt) vs. Control was evaluated on Cellular localization and regulation of ET-1 and Ang II receptors and effects on [Ca2+]i. Cardiac hypertrophy induced by volume overload significantly downregulated AT1 receptors on fibroblasts (42,970 vs 73,870 sites/cell, P<0.01) and enhanced Ang II [Ca2+]i sensitivity in cardiomyocytes.
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