Tanemoto Masayuki, Abe Takaaki, Onogawa Tohru, Ito Sadayoshi
Division of Nephrology, Hypertension and Endocrinology, Department of Medicine, Tohoku University Graduate School of Medicine, 1-1 Seiryo-cho, Aoba-ku, Sendai 980-8574, Japan.
Am J Physiol Renal Physiol. 2004 Dec;287(6):F1148-53. doi: 10.1152/ajprenal.00203.2004. Epub 2004 Aug 3.
Kir5.1, a nonfunctional inwardly rectifying K(+) channel by itself, can form functional channels by assembling with other proteins. We previously showed that Kir5.1 assembled with Kir4.1 and functioned as an acid-base regulator in the kidney. In this study, we examined the intrarenal distribution of Kir5.1 by RT-PCR analysis on dissected nephron segments and immunohistochemical analysis with the specific anti-Kir5.1 antibody. Strong expression of Kir5.1 was detected in distal convoluted tubules, and weak expression was also detected in thick ascending limb of Henle's loop. Colocalization of Kir5.1 with Kir4.1 indicated expression of Kir5.1/Kir4.1 heteromer in these nephron segments. In a renal epithelial cell line, Madin-Darby canine kidney cells, heteromer formation with Kir4.1 changed the localization of Kir5.1 from intracellular components to the cell surface. The COOH-terminal cytoplasmic portion that includes the PDZ binding motif of Kir4.1 was responsible for this intracellular localization. These data suggest the signals on the COOH terminus of Kir4.1, including PDZ binding motif, determine the intracellular localization of Kir5.1/Kir4.1 heteromer in distal tubules.
Kir5.1本身是一种无功能的内向整流钾通道,它可以与其他蛋白质组装形成功能性通道。我们之前表明,Kir5.1与Kir4.1组装并在肾脏中作为酸碱调节剂发挥作用。在本研究中,我们通过对解剖的肾单位节段进行RT-PCR分析以及使用特异性抗Kir5.1抗体进行免疫组织化学分析,研究了Kir5.1在肾脏内的分布。在远曲小管中检测到Kir5.1的强表达,在亨氏袢厚升支中也检测到弱表达。Kir5.1与Kir4.1的共定位表明在这些肾单位节段中存在Kir5.1/Kir4.1异聚体的表达。在一种肾上皮细胞系——Madin-Darby犬肾细胞中,与Kir4.1形成异聚体改变了Kir5.1从细胞内成分到细胞表面的定位。包含Kir4.1的PDZ结合基序的COOH末端细胞质部分负责这种细胞内定位。这些数据表明,Kir4.1的COOH末端上包括PDZ结合基序的信号决定了Kir5.1/Kir4.1异聚体在远曲小管中的细胞内定位。
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