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Distal potassium handling based on flow modulation of maxi-K channel activity.基于大电导钾通道活动流量调节的远端钾处理
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Akt mediates the effect of insulin on epithelial sodium channels by inhibiting Nedd4-2.Akt通过抑制Nedd4-2介导胰岛素对上皮钠通道的作用。
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Liver-derived IGF-I regulates kidney size, sodium reabsorption, and renal IGF-II expression.肝脏来源的胰岛素样生长因子-I调节肾脏大小、钠重吸收及肾脏胰岛素样生长因子-II的表达。
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Intersectin links WNK kinases to endocytosis of ROMK1.相交蛋白将WNK激酶与ROMK1的内吞作用联系起来。
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An SGK1 site in WNK4 regulates Na+ channel and K+ channel activity and has implications for aldosterone signaling and K+ homeostasis.WNK4中的一个SGK1位点调节钠通道和钾通道活性,并对醛固酮信号传导和钾稳态有影响。
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Renal function of gene-targeted mice lacking both SGK1 and SGK3.缺乏SGK1和SGK3的基因靶向小鼠的肾功能。
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Antagonistic regulation of ROMK by long and kidney-specific WNK1 isoforms.长链和肾脏特异性WNK1亚型对ROMK的拮抗调节作用。
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10
Modest dietary K+ restriction provokes insulin resistance of cellular K+ uptake and phosphorylation of renal outer medulla K+ channel without fall in plasma K+ concentration.适度的饮食钾限制会引发细胞钾摄取的胰岛素抵抗以及肾外髓质钾通道的磷酸化,而血浆钾浓度并不降低。
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PI3-激酶的激活通过 Akt1/SGK1 依赖性的 WNK1 磷酸化来刺激 ROMK 的内吞作用。

Activation of PI3-kinase stimulates endocytosis of ROMK via Akt1/SGK1-dependent phosphorylation of WNK1.

机构信息

Department of Medicine, UT Southwestern Medical Center, 5323 Harry Hines Boulevard, Dallas, TX 75390-8856, USA.

出版信息

J Am Soc Nephrol. 2011 Mar;22(3):460-71. doi: 10.1681/ASN.2010060681. Epub 2011 Feb 25.

DOI:10.1681/ASN.2010060681
PMID:21355052
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3060440/
Abstract

WNK kinases stimulate endocytosis of ROMK channels to regulate renal K+ handling. Phosphatidylinositol 3-kinase (PI3K)-activating hormones, such as insulin and IGF 1, phosphorylate WNK1, but how this affects the regulation of ROMK abundance is unknown. Here, serum starvation of ROMK-transfected HEK cells led to an increase of ROMK current density; subsequent addition of insulin or IGF1 inhibited ROMK currents in a PI3K-dependent manner. Serum and insulin also increased phosphorylation of the downstream kinases Akt1 and SGK1 as well as WNK1. A biotinylation assay suggested that insulin and IGF1 inhibit ROMK by enhancing its endocytosis, a process that WNK1 may mediate. Knockdown of WNK1 with siRNA or expression of a phospho-deficient WNK1 mutant (T58A) both prevented insulin-induced inhibition of ROMK currents, suggesting that phosphorylation at Threonine-58 of WNK1 is important to mediate the inhibition of ROMK by PI3K-activating hormones or growth factors. In vitro and in vivo kinase assays supported the notion that Akt1 and SGK1 can phosphorylate WNK1 at this site, and we established that Akt1 and SGK1 synergistically inhibit ROMK through WNK1. We used dominant-negative intersectin and dynamin constructs to show that SGK1-mediated phosphorylation of WNK1 inhibits ROMK by promoting its endocytosis. Taken together, these results suggest that PI3K-activating hormones inhibit ROMK by enhancing its endocytosis via a mechanism that involves phosphorylation of WNK1 by Akt1 and SGK1.

摘要

WNK 激酶刺激 ROMK 通道内吞以调节肾脏 K+处理。激活磷脂酰肌醇 3-激酶 (PI3K) 的激素,如胰岛素和 IGF1,磷酸化 WNK1,但这如何影响 ROMK 丰度的调节尚不清楚。本文中,血清饥饿转染 ROMK 的 HEK 细胞导致 ROMK 电流密度增加;随后添加胰岛素或 IGF1 以 PI3K 依赖性方式抑制 ROMK 电流。血清和胰岛素还增加了下游激酶 Akt1 和 SGK1 以及 WNK1 的磷酸化。生物素标记测定表明,胰岛素和 IGF1 通过增强其内吞作用来抑制 ROMK,WNK1 可能介导此过程。用 siRNA 敲低 WNK1 或表达磷酸化缺陷的 WNK1 突变体 (T58A) 均阻止了胰岛素诱导的 ROMK 电流抑制,表明 WNK1 的苏氨酸 58 位磷酸化对于 PI3K 激活激素或生长因子介导的 ROMK 抑制很重要。体外和体内激酶测定支持 Akt1 和 SGK1 可在该位点磷酸化 WNK1 的观点,我们确定 Akt1 和 SGK1 通过 WNK1 协同抑制 ROMK。我们使用显性负性 intersectin 和 dynamin 构建体表明,SGK1 介导的 WNK1 磷酸化通过促进其内吞来抑制 ROMK。总之,这些结果表明,PI3K 激活激素通过 Akt1 和 SGK1 磷酸化 WNK1 增强其内吞作用来抑制 ROMK。