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阴离子交换蛋白 Slc26a4(pendrin)缺失降低了肾集合管顶端的 Cl(-)/HCO3(-) 交换活性,损害了碳酸氢盐分泌。

Deletion of the anion exchanger Slc26a4 (pendrin) decreases apical Cl(-)/HCO3(-) exchanger activity and impairs bicarbonate secretion in kidney collecting duct.

机构信息

Research Services, Cincinnati Department of Veterans Affairs Medical Center, Cincinnati, OH, USA.

出版信息

Am J Physiol Cell Physiol. 2010 Jul;299(1):C33-41. doi: 10.1152/ajpcell.00033.2010. Epub 2010 Apr 7.

Abstract

The anion exchanger Pendrin, which is encoded by SLC26A4 (human)/Slc26a4 (mouse) gene, is localized on the apical membrane of non-acid-secreting intercalated (IC) cells in the kidney cortical collecting duct (CCD). To examine its role in the mediation of bicarbonate secretion in vivo and the apical Cl(-)/HCO(3)(-) exchanger in the kidney CCD, mice with genetic deletion of pendrin were generated. The mutant mice show the complete absence of pendrin expression in their kidneys as assessed by Northern blot hybridization, Western blot, and immunofluorescence labeling. Pendrin knockout (KO) mice display significantly acidic urine at baseline [pH 5.20 in KO vs. 6.01 in wild type (WT); P < 0.0001] along with elevated serum HCO(3)(-) concentration (27.4 vs. 24 meq/l in KO vs. WT, respectively; P < 0.02), consistent with decreased bicarbonate secretion in vivo. The urine chloride excretion was comparable in WT and KO mice. For functional studies, CCDs were microperfused and IC cells were identified by their ability to trap the pH fluorescent dye BCECF. The apical Cl(-)/HCO(3)(-) exchanger activity in B-IC and non-A, non-B-IC cells, as assessed by intracellular pH monitoring, was significantly reduced in pendrin-null mice. The basolateral Cl(-)/HCO(3)(-) exchanger activity in A-IC cells and in non-A, non-B-IC cells, was not different in pendrin KO mice relative to WT animals. Urine NH(4)(+) (ammonium) excretion increased significantly, consistent with increased trapping of NH(3) in the collecting duct in pendrin KO mice. We conclude that Slc26a4 (pendrin) deletion impairs the secretion of bicarbonate in vivo and reduces apical Cl(-)/HCO(3)(-) exchanger activity in B-IC and non-A, non-B-IC cells in CCD. Additional apical Cl(-)/HCO(3)(-) exchanger(s) is (are) present in the CCD.

摘要

阴离子交换蛋白 Pendrin 由 SLC26A4(人)/Slc26a4(鼠)基因编码,定位于肾脏皮质集合管(CCD)中非酸性分泌闰细胞的顶膜上。为了研究其在体内介导碳酸氢盐分泌以及肾脏 CCD 中顶端 Cl(-)/HCO(3)(-)交换体的作用,生成了 Pendrin 基因缺失的突变小鼠。通过 Northern blot 杂交、Western blot 和免疫荧光标记评估,突变小鼠肾脏中 Pendrin 的表达完全缺失。Pendrin 敲除(KO)小鼠的基础尿液呈明显酸性(KO 组 pH 为 5.20,WT 组为 6.01;P < 0.0001),同时血清 HCO(3)(-)浓度升高(KO 组为 27.4 meq/l,WT 组为 24 meq/l;P < 0.02),表明体内碳酸氢盐分泌减少。WT 组和 KO 组小鼠的尿氯排泄量相当。为了进行功能研究,CCD 进行微灌流,通过其摄取 pH 荧光染料 BCECF 的能力来鉴定闰细胞。使用细胞内 pH 监测评估顶膜 Cl(-)/HCO(3)(-)交换体活性,Pendrin 缺失小鼠 B-IC 和非-A、非-B-IC 细胞中的活性显著降低。与 WT 动物相比,Pendrin KO 小鼠 A-IC 细胞和非-A、非-B-IC 细胞中的基底外侧 Cl(-)/HCO(3)(-)交换体活性无差异。Pendrin KO 小鼠的尿 NH(4)(+)(铵)排泄显著增加,这与在 Pendrin KO 小鼠的集合管中 NH(3)捕获增加一致。我们得出结论,Slc26a4(Pendrin)缺失会损害体内碳酸氢盐的分泌,并降低 CCD 中 B-IC 和非-A、非-B-IC 细胞中的顶端 Cl(-)/HCO(3)(-)交换体活性。在 CCD 中还存在其他的顶端 Cl(-)/HCO(3)(-)交换体。

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