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选择性剪接的富含脯氨酸的片段将WNK1与醛固酮作用联系起来。

Alternatively spliced proline-rich cassettes link WNK1 to aldosterone action.

作者信息

Roy Ankita, Al-Qusairi Lama, Donnelly Bridget F, Ronzaud Caroline, Marciszyn Allison L, Gong Fan, Chang Y P Christy, Butterworth Michael B, Pastor-Soler Núria M, Hallows Kenneth R, Staub Olivier, Subramanya Arohan R

出版信息

J Clin Invest. 2015 Sep;125(9):3433-48. doi: 10.1172/JCI75245. Epub 2015 Aug 4.

Abstract

The thiazide-sensitive NaCl cotransporter (NCC) is important for renal salt handling and blood-pressure homeostasis. The canonical NCC-activating pathway consists of With-No-Lysine (WNK) kinases and their downstream effector kinases SPAK and OSR1, which phosphorylate NCC directly. The upstream mechanisms that connect physiological stimuli to this system remain obscure. Here, we have shown that aldosterone activates SPAK/OSR1 via WNK1. We identified 2 alternatively spliced exons embedded within a proline-rich region of WNK1 that contain PY motifs, which bind the E3 ubiquitin ligase NEDD4-2. PY motif-containing WNK1 isoforms were expressed in human kidney, and these isoforms were efficiently degraded by the ubiquitin proteasome system, an effect reversed by the aldosterone-induced kinase SGK1. In gene-edited cells, WNK1 deficiency negated regulatory effects of NEDD4-2 and SGK1 on NCC, suggesting that WNK1 mediates aldosterone-dependent activity of the WNK/SPAK/OSR1 pathway. Aldosterone infusion increased proline-rich WNK1 isoform abundance in WT mice but did not alter WNK1 abundance in hypertensive Nedd4-2 KO mice, which exhibit high baseline WNK1 and SPAK/OSR1 activity toward NCC. Conversely, hypotensive Sgk1 KO mice exhibited low WNK1 expression and activity. Together, our findings indicate that the proline-rich exons are modular cassettes that convert WNK1 into a NEDD4-2 substrate, thereby linking aldosterone and other NEDD4-2-suppressing antinatriuretic hormones to NCC phosphorylation status.

摘要

噻嗪类敏感的氯化钠协同转运蛋白(NCC)对于肾脏的盐处理和血压稳态至关重要。经典的NCC激活途径由无赖氨酸(WNK)激酶及其下游效应激酶SPAK和OSR1组成,它们直接使NCC磷酸化。将生理刺激与该系统联系起来的上游机制仍不清楚。在这里,我们已经表明醛固酮通过WNK1激活SPAK/OSR1。我们在WNK1富含脯氨酸的区域内鉴定出2个选择性剪接外显子,其中包含PY基序,这些基序可结合E3泛素连接酶NEDD4-2。含PY基序的WNK1异构体在人肾脏中表达,并且这些异构体被泛素蛋白酶体系统有效降解,醛固酮诱导的激酶SGK1可逆转这种作用。在基因编辑的细胞中,WNK1缺陷消除了NEDD4-2和SGK1对NCC的调节作用,这表明WNK1介导了WNK/SPAK/OSR1途径的醛固酮依赖性活性。醛固酮输注增加了野生型小鼠中富含脯氨酸的WNK1异构体丰度,但未改变高血压Nedd4-2基因敲除小鼠中WNK1的丰度,这些小鼠对NCC表现出高基线WNK1和SPAK/OSR1活性。相反,低血压的Sgk1基因敲除小鼠表现出低WNK1表达和活性。总之,我们的研究结果表明,富含脯氨酸的外显子是模块化盒式结构,可将WNK1转化为NEDD4-2底物,从而将醛固酮和其他抑制NEDD4-2的利钠激素与NCC磷酸化状态联系起来。

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