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低血钾表型绵羊红细胞膜内翻小泡中的容积敏感性钾氯协同转运

Volume-sensitive K-Cl cotransport in inside-out vesicles made from erythrocyte membranes from sheep of low-K phenotype.

作者信息

Kracke G R, Dunham P B

机构信息

Department of Biology, Syracuse University, NY 13244-1220.

出版信息

Proc Natl Acad Sci U S A. 1990 Nov;87(21):8575-9. doi: 10.1073/pnas.87.21.8575.

Abstract

Unidirectional K ion effluxes were measured from inside-out vesicles prepared from erythrocyte membranes from sheep of the low-K phenotype. Total K efflux was 150 nmol per mg of protein per hr in a Cl medium of 295 mosmol/kg (with the Na/K pump inhibited). Cl-dependent K efflux (determined with methanesulfonate replacing Cl) was 54 nmol/(mg.hr). Cl-dependent K efflux (K-Cl cotransport) increased to 77 nmol/(mg.hr) with osmotic swelling of approximately 30% in 230-mosmol/kg medium and decreased to 13 nmol/(mg.hr) after shrinkage of approximately 60% in 430-mosmol/kg medium. Osmotically induced changes in transport and vesicle volume were reversible. K-Cl cotransport was enhanced by ATP. Nonhydrolyzable ATP analogues failed to substitute for ATP, indicating that phosphorylation is involved. However, in the absence of added ATP there was significant K-Cl cotransport, suggesting that phosphorylation is not essential for function. The results provide clues about the nature of the signals detected by the sensor of cell volume changes and demonstrate that inside-out vesicles from sheep erythrocyte membranes provide an advantageous experimental system for investigation of the volume sensor.

摘要

从低血钾表型绵羊红细胞膜制备的内翻外囊泡中测量单向钾离子外流。在295 mosmol/kg的Cl介质中(钠钾泵被抑制),总钾外流为每毫克蛋白质每小时150 nmol。Cl依赖性钾外流(用甲磺酸盐替代Cl测定)为54 nmol/(mg·hr)。在230 mosmol/kg介质中,随着约30%的渗透性肿胀,Cl依赖性钾外流(钾氯共转运)增加到77 nmol/(mg·hr),而在430 mosmol/kg介质中约60%的收缩后,其减少到13 nmol/(mg·hr)。渗透诱导的转运和囊泡体积变化是可逆的。钾氯共转运被ATP增强。不可水解的ATP类似物不能替代ATP,表明磷酸化参与其中。然而,在没有添加ATP的情况下,仍有显著的钾氯共转运,这表明磷酸化对于功能并非必不可少。这些结果为细胞体积变化传感器所检测信号的性质提供了线索,并证明绵羊红细胞膜的内翻外囊泡为研究体积传感器提供了一个有利的实验系统。

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ATP dependence of K-Cl cotransport in dog red blood cells.犬红细胞中钾氯共转运体对ATP的依赖性
Am J Physiol. 1993 Dec;265(6 Pt 1):C1648-52. doi: 10.1152/ajpcell.1993.265.6.C1648.

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