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Phosphorylation Regulates NCC Stability and Transporter Activity In Vivo

远曲小管 磷酸化 内科学 内分泌学 共转运蛋白 化学 激酶 协同运输机 生物 细胞生物学 运输机 生物化学 重吸收 医学 有机化学 基因
作者
Sung‐Sen Yang,Yu‐Wei Fang,Min‐Hua Tseng,Pei-Yi Chu,I‐Shing Yu,Han‐Chung Wu,Shu‐Wha Lin,Tom Chau,Shinichi Uchida,Sei Sasaki,Yuh‐Feng Lin,Huey‐Kang Sytwu,Shih‐Hua Lin
出处
期刊:Journal of The American Society of Nephrology 卷期号:24 (10): 1587-1597 被引量:52
标识
DOI:10.1681/asn.2012070742
摘要

A T60M mutation in the thiazide-sensitive sodium chloride cotransporter (NCC) is common in patients with Gitelman’s syndrome (GS). This mutation prevents Ste20-related proline and alanine-rich kinase (SPAK)/oxidative stress responsive kinase-1 (OSR1)–mediated phosphorylation of NCC and alters NCC transporter activity in vitro. Here, we examined the physiologic effects of NCC phosphorylation in vivo using a novel Ncc T58M (human T60M) knock-in mouse model. NccT58M/T58M mice exhibited typical features of GS with a blunted response to thiazide diuretics. Despite expressing normal levels of Ncc mRNA, these mice had lower levels of total Ncc and p-Ncc protein that did not change with a low-salt diet that increased p-Spak. In contrast to wild-type Ncc, which localized to the apical membrane of distal convoluted tubule cells, T58M Ncc localized primarily to the cytosolic region and caused an increase in late distal convoluted tubule volume. In MDCK cells, exogenous expression of phosphorylation-defective NCC mutants reduced total protein expression levels and membrane stability. Furthermore, our analysis found diminished total urine NCC excretion in a cohort of GS patients with homozygous NCC T60M mutations. When Wnk4D561A/+ mice, a model of pseudohypoaldosteronism type II expressing an activated Spak/Osr1-Ncc, were crossed with NccT58M/T58M mice, total Ncc and p-Ncc protein levels decreased and the GS phenotype persisted over the hypertensive phenotype. Overall, these data suggest that SPAK-mediated phosphorylation of NCC at T60 regulates NCC stability and function, and defective phosphorylation at this residue corrects the phenotype of pseudohypoaldosteronism type II.

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