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加压素增加了具有浓缩尿液缺陷的小鼠肾髓质中 UT-A1、UT-A3 和 ER 伴侣蛋白 GRP78 的表达。

Vasopressin increases expression of UT-A1, UT-A3, and ER chaperone GRP78 in the renal medulla of mice with a urinary concentrating defect.

机构信息

Dept. of Physiology, College of Medicine, Univ. of Arizona, Tucson, AZ 85724-5218, USA.

出版信息

Am J Physiol Renal Physiol. 2010 Oct;299(4):F712-9. doi: 10.1152/ajprenal.00690.2009. Epub 2010 Jul 28.

Abstract

Activation of V2 receptors (V2R) during antidiuresis increases the permeability of the inner medullary collecting duct to urea and water. Extracellular osmolality is elevated as the concentrating capacity of the kidney increases. Osmolality is known to contribute to the regulation of collecting duct water (aquaporin-2; AQP2) and urea transporter (UT-A1, UT-A3) regulation. AQP1KO mice are a concentrating mechanism knockout, a defect attributed to the loss of high interstitial osmolality. A V2R-specific agonist, deamino-8-D-arginine vasopressin (dDAVP), was infused into wild-type and AQP1KO mice for 7 days. UT-A1 mRNA and protein abundance were significantly increased in the medullas of wild-type and AQP1KO mice following dDAVP infusion. The mRNA and protein abundance of UT-A3, the basolateral urea transporter, was significantly increased by dDAVP in both wild-type and AQP1KO mice. Semiquantitative immunoblots revealed that dDAVP infusion induced a significant increase in the medullary expression of the endoplasmic reticulum (ER) chaperone GRP78. Immunofluorescence studies demonstrated that GRP78 expression colocalized with AQP2 in principal cells of the papillary tip of the renal medulla. Using immunohistochemistry and immunogold electron microscopy, we demonstrate that vasopressin induced a marked apical targeting of GRP78 in medullary principal cells. Urea-sensitive genes, GADD153 and ATF4 (components of the ER stress pathway), were significantly increased in AQP1KO mice by dDAVP infusion. These findings strongly support an important role of vasopressin in the activation of an ER stress response in renal collecting duct cells, in addition to its role in activating an increase in UT-A1 and UT-A3 abundance.

摘要

V2 受体(V2R)的激活在抗利尿作用期间增加了内髓集合管对尿素和水的通透性。随着肾脏浓缩能力的增加,细胞外渗透压升高。渗透压已知有助于调节集合管水(水通道蛋白-2;AQP2)和尿素转运体(UT-A1、UT-A3)的调节。AQP1KO 小鼠是一种浓缩机制敲除小鼠,缺陷归因于间质高渗透压的丧失。一种 V2R 特异性激动剂,去氨基-8-D-精氨酸血管加压素(dDAVP),被输注到野生型和 AQP1KO 小鼠中 7 天。dDAVP 输注后,野生型和 AQP1KO 小鼠的髓质中 UT-A1mRNA 和蛋白丰度显著增加。dDAVP 显著增加了两种野生型和 AQP1KO 小鼠中基底外侧尿素转运体 UT-A3 的 mRNA 和蛋白丰度。半定量免疫印迹显示,dDAVP 输注诱导 ER 伴侣 GRP78 在髓质中的表达显著增加。免疫荧光研究表明,GRP78 表达与主细胞中的 AQP2 共定位在肾髓质乳头尖端的主细胞中。通过免疫组织化学和免疫金电子显微镜,我们证明血管加压素诱导 GRP78 在髓质主细胞中明显的顶端靶向。dDAVP 输注显著增加了 AQP1KO 小鼠中尿素敏感基因 GADD153 和 ATF4(内质网应激途径的组成部分)的表达。这些发现强烈支持血管加压素在激活肾集合管细胞中 ER 应激反应中的重要作用,除了其激活 UT-A1 和 UT-A3 丰度增加的作用之外。

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