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(钠,钾)-共转运在麦迪逊-达比犬肾细胞系中的研究。钠与钾相互作用的动力学特征。

(Na+,K+)-cotransport in the Madin-Darby canine kidney cell line. Kinetic characterization of the interaction between Na+ and K+.

作者信息

Rindler M J, McRoberts J A, Saier M H

出版信息

J Biol Chem. 1982 Mar 10;257(5):2254-9.

PMID:6277889
Abstract

Confluent monolayer cultures of the differentiated kidney epithelial cell line, Madin-Darby canine kidney cells (MDCK), have been used to study ion transport mechanisms involved in transepithelial transport. We have investigated the previously reported K+-stimulation of 22Na+ uptake by confluent monolayers of Na+ depleted cells (Rindler, M. J., Taub, M., and Saier, M. H., Jr. (1979) J. Biol. Chem. 254, 11431-11439). This component of Na+ uptake was insensitive to ouabain and amiloride, but was strongly inhibited by furosemide or bumetanide. Ouabain-insensitive 86Rb+ uptake was also inhibitable by furosemide or bumetanide and stimulated by extracellular Na+. The synergistic effect of Na+ and 86Rb+ uptake and K+ on 22Na+ uptake was reflected by an increase in the apparent Vmax and a decrease in the apparent Km as the concentration of the other cation was increased. The extrapolated Km for either 86Rb+ or 22Na+ uptake in the absence of the other cation was 30 mM while the Km in the presence of a saturating concentration of the other cation was 9 mM. The absolute Vmax values for 22Na+ and 86Rb+ uptake suggest a cotransport system with a stoichiometry of 2Na+:3K+. However, because of the experimental design, the actual ratio may be closer to 1:1. Competition with, and stimulation by, a variety of unlabeled cations indicated that Na+ could be partially replaced by Li+, while K+ could be fully replaced by Rb+ and partially replaced by NH4+ and CS+. Uptake by this system was dependent upon cellular ATP. Reduction of intracellular ATP to 3% of normal abolished both K+-stimulated 22Na+ uptake and Na+-stimulated 86Rb+ uptake.

摘要

分化的肾上皮细胞系——麦氏犬肾细胞(MDCK)的汇合单层培养物已被用于研究跨上皮运输中涉及的离子转运机制。我们研究了先前报道的钠缺乏细胞的汇合单层对22Na+摄取的钾刺激作用(林德勒,M. J.,陶布,M.,以及赛厄尔,M. H.,Jr.(1979年)《生物化学杂志》254,11431 - 11439)。钠摄取的这一成分对哇巴因和氨氯吡脒不敏感,但被呋塞米或布美他尼强烈抑制。哇巴因不敏感的86Rb+摄取也可被呋塞米或布美他尼抑制,并受细胞外钠刺激。随着另一种阳离子浓度的增加,钠和86Rb+摄取以及钾对22Na+摄取的协同作用表现为表观Vmax增加和表观Km降低。在不存在另一种阳离子时,86Rb+或22Na+摄取的外推Km为30 mM,而在存在饱和浓度的另一种阳离子时,Km为9 mM。22Na+和86Rb+摄取的绝对Vmax值表明存在一个化学计量比为2Na+:3K+的协同转运系统。然而,由于实验设计,实际比例可能更接近1:1。与多种未标记阳离子的竞争和刺激表明,钠可部分被锂取代,而钾可被铷完全取代,部分被铵和铯取代。该系统的摄取依赖于细胞ATP。将细胞内ATP降低至正常水平的3%可消除钾刺激的22Na+摄取和钠刺激的86Rb+摄取。

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