Abstract MP05: Mineralocorticoid And Angiotensin II Type 1 Receptors In The Subfornical Organ Mediate Angiotensin II Hypertension In Rats

Abstract

Circulating Ang II increases BP through both peripheral and central mechanisms. Activation of both AT 1 R and MR in the CNS plays a critical role in Ang II-induced hypertension. The subfornical organ (SFO) contains both MR and AT 1 R and can relay the signals of circulating Ang II to downstream nuclei such as the PVN. In this study, we evaluated the effect of intra-SFO infusion of AAV-MR-siRNA or AAV-AT 1a R-siRNA on MR or AT 1 R mRNA expression in the SFO and PVN and Ang II induced hypertension as assessed by telemetry. Two week sc infusion of Ang II at 500 ng/kg/min in Wistar rats on regular salt diet increased BP by 60~65 mmHg. This pressor effect of Ang II was largely prevented by AAV-MR-siRNA or AAV-AT 1 R-siRNA in the SFO (Figure). Ang II increased AT 1 R mRNA expression (1.7± 0.4 vs 0.8 ± 0.04 х10 -1 , p<0.05) in the SFO. Both MR- and AT 1 R-siRNA in the SFO prevented this increase (1.1 ± 0.2х10 -1 and 1.0± 0.3х10 -1 ). In contrast, Ang II decreased MR mRNA expression (3.2 ± 0.2 vs. 4.1 ± 0.2х10 -2 , p<0.05) in the SFO. Both MR- and AT 1 R-siRNA further decreased MR mRNA expression (2.7 ± 0.2 х10 -2 and 2.3 ± 0.3 х10 -2 ). In the PVN, Ang II increased AT 1 R mRNA by ~100% and MR mRNA by ~20%. Only AT 1 R-siRNA in the SFO prevented these increases in the PVN. AAV mediated eGFP fluorescence expression was observed in the SFO but not the PVN. These results suggest that circulating Ang II differentially regulates MR and AT 1 R expression in the SFO. Prevention of Ang II induced AT 1 R up-regulation by knockdown of either AT 1 R or MR suggests a MR dependent regulation of AT 1 R in the SFO. MR-AT 1 R signaling in the SFO appears to play a major role in Ang II-induced hypertension in rats. * p<0.05, vs. baseline values; a: p<0.05, vs. AAV-SCM-siRNA