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RACK1 调节血管紧张素 II 诱导的 SHR 肾小球前血管平滑肌细胞的收缩。

RACK1 regulates angiotensin II-induced contractions of SHR preglomerular vascular smooth muscle cells.

机构信息

Department of Pharmacology and Chemical Biology, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania.

Department of Pharmacology and Chemical Biology, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania

出版信息

Am J Physiol Renal Physiol. 2017 Apr 1;312(4):F565-F576. doi: 10.1152/ajprenal.00547.2016. Epub 2017 Jan 18.

Abstract

The preglomerular microcirculation of spontaneously hypertensive rats (SHR) is hypersensitive to angiotensin (ANG) II, and studies have shown that this is likely due to enhanced coincident signaling between G protein subunits α (Gα; released by ANG II) and βγ (Gβγ; released by G-coupled receptors) to active phospholipase C (PLC). Here we investigated the molecular basis for the enhanced coincident signaling between Gβγ and Gα in SHR preglomerular vascular smooth muscle cells (PGVSMCs). Because receptor for activated C kinase 1 (RACK1; a scaffolding protein) organizes interactions between Gβγ, Gα, and PLC, we included RACK1 in this investigation. Cell fractionation studies demonstrated increased levels of membrane (but not cytosolic) Gβ, Gα, PLCβ, and RACK1 in SHR PGVSMCs compared with Wistar-Kyoto rat PGVSMCs. In SHR PGVSMCs, coimmunoprecipitation demonstrated RACK1 binding to Gβ and PLCβ, but only at cell membranes. Pertussis toxin (which blocks Gβγ) and U73122 (which blocks PLC) reduced membrane RACK1; however, RACK1 knockdown (shRNA) did not affect membrane levels of Gβ, Gα, or PLCβ In a novel gel contraction assay, RACK1 knockdown in SHR PGVSMCs attenuated contractions to ANG II and abrogated the ability of neuropeptide Y (which signals via Gβγ) to enhance ANG II-induced contractions. We conclude that in SHR PGVSMCs the enlarged pool of Gβγ and PLCβ recruits RACK1 to membranes and RACK1 then organizes signaling. Consequently, knockdown of RACK1 prevents coincident signaling between ANG II and the G pathway. This is the first study to implicate RACK1 in vascular smooth muscle cell contraction and suggests that RACK1 inhibitors could be effective cardiovascular drugs.

摘要

自发性高血压大鼠(SHR)的肾小球前微循环对血管紧张素 II(ANG)II 敏感,研究表明这可能是由于 G 蛋白亚单位α(ANG II 释放)和βγ(G 蛋白偶联受体释放)与活性磷脂酶 C(PLC)之间的协同信号增强所致。在这里,我们研究了 SHR 肾小球血管平滑肌细胞(PGVSMC)中 Gβγ 与 Gα 之间协同信号增强的分子基础。由于激活的 C 激酶 1 受体(RACK1;一种支架蛋白)组织 Gβγ、Gα 和 PLC 之间的相互作用,我们将 RACK1 纳入了这项研究。细胞分级研究表明,与 Wistar-Kyoto 大鼠 PGVSMC 相比,SHR PGVSMC 中膜(而非胞质)Gβ、Gα、PLCβ 和 RACK1 水平升高。在 SHR PGVSMC 中,共免疫沉淀表明 RACK1 与 Gβ 和 PLCβ 结合,但仅在细胞膜上。百日咳毒素(阻断 Gβγ)和 U73122(阻断 PLC)减少了膜 RACK1;然而,RACK1 敲低(shRNA)并未影响 Gβ、Gα 或 PLCβ 的膜水平。在一项新的凝胶收缩测定中,SHR PGVSMC 中的 RACK1 敲低减弱了对 ANG II 的收缩反应,并消除了神经肽 Y(通过 Gβγ 信号)增强 ANG II 诱导的收缩的能力。我们得出结论,在 SHR PGVSMC 中,扩大的 Gβγ 和 PLCβ 池招募 RACK1 到膜上,然后 RACK1 组织信号。因此,RACK1 的敲低可防止 ANG II 与 G 途径之间的协同信号。这是第一项表明 RACK1 参与血管平滑肌细胞收缩的研究,并表明 RACK1 抑制剂可能是有效的心血管药物。

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