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肾小管细胞中的钠泵受来自下丘脑的内源性钠钾ATP酶抑制剂调控。

Na+ pump in renal tubular cells is regulated by endogenous Na+-K+-ATPase inhibitor from hypothalamus.

作者信息

Cantiello H F, Chen E, Ray S, Haupert G T

机构信息

Medical Services, Massachusetts General Hospital, Harvard Medical School, Boston 02114.

出版信息

Am J Physiol. 1988 Oct;255(4 Pt 2):F574-80. doi: 10.1152/ajprenal.1988.255.4.F574.

Abstract

Bovine hypothalamus contains a high affinity, specific, reversible inhibitor of mammalian Na+-K+-ATPase. Kinetic analysis using isolated membrane fractions showed binding and dissociation rates of the hypothalamic factor (HF) to be (like ouabain) relatively long (off rate = 60 min). To determine whether the kinetics of inhibition in intact cells might be more consistent with regulation of physiological processes in vivo, binding and dissociation reactions of HF in intact renal epithelial cells (LLC-PK1) were studied using 86Rb+ uptake and [3H]ouabain binding. As with membranes, a 60-min incubation with HF inhibited Na+-K+-ATPase in LLC-PK1 cells. In contrast to membrane studies, no prolonged incubation with LLC-PK1 was needed to observe inhibition of Na+-K+-ATPase. HF caused a 33% inhibition of ouabain-sensitive 86Rb+ influx within 10 min. Incubation of cells with HF followed by washout showed rapid reversal of pump inhibition and a doubling of pump activity. The dose-response curve for HF inhibition of LLC-PK1 86Rb+ uptake showed a sigmoidal shape consistent with an allosteric binding reaction. Thus HF is a potent regulator of Na+-K+-ATPase activity in intact renal cells, with binding and dissociation reactions consistent with relevant physiological processes.

摘要

牛下丘脑含有一种对哺乳动物钠钾ATP酶具有高亲和力、特异性、可逆性的抑制剂。使用分离的膜组分进行的动力学分析表明,下丘脑因子(HF)的结合和解离速率(与哇巴因类似)相对较长(解离速率 = 60分钟)。为了确定完整细胞中抑制作用的动力学是否可能与体内生理过程的调节更一致,利用86Rb +摄取和[3H]哇巴因结合研究了完整肾上皮细胞(LLC-PK1)中HF的结合和解离反应。与膜的情况一样,用HF孵育60分钟可抑制LLC-PK1细胞中的钠钾ATP酶。与膜研究不同的是,观察到钠钾ATP酶的抑制作用不需要对LLC-PK1进行长时间孵育。HF在10分钟内使哇巴因敏感的86Rb +内流受到33%的抑制。用HF孵育细胞后冲洗,显示泵抑制作用迅速逆转,泵活性加倍。HF抑制LLC-PK1 86Rb +摄取的剂量反应曲线呈S形,与别构结合反应一致。因此,HF是完整肾细胞中钠钾ATP酶活性的有效调节剂,其结合和解离反应与相关生理过程一致。

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