人红细胞中的钾激活磷酸酶。对硝基苯磷酸酯对碳通量的影响。

Potassium activated phosphatase from human red blood cells. The effects of p-nitrophenylphosphate on carbon fluxes.

作者信息

Garrahan P J, Rega A F

出版信息

J Physiol. 1972 Jun;223(2):595-617. doi: 10.1113/jphysiol.1972.sp009864.

DOI:10.1113/jphysiol.1972.sp009864

PMID:4339052

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1331464/

Abstract

When red cells are incubated in solutions containing p-nitrophenyl-phosphate (p-NPP), intracellular p-NPP quickly builds up reaching with a half-time of 3 min a concentration in cell water equal to one fourth the external concentration, which under the conditions used is the expected value for a divalent anion in Gibbs-Donnan equilibrium. Hence p-NPP added to the incubation media in red cells has quick access to the active centre of the membrane phosphatase which is located at the inner surface of the cell membrane.2. When p-NPP is added to the incubation media of ATP-free red cells or reconstituted ghosts, no ouabain-sensitive cation movements are detectable, suggesting that hydrolysis of p-NPP by the active transport system is unable to energize active ion translocation.3. When p-NPP concentration in the incubation media of ATP-containing cells is progressively raised, both ouabain-sensitive Na loss and ouabain-sensitive Rb uptake tend to zero along rectangular hyperbolae. For both movements inhibition is half-maximal at 77 mM external p-NPP (i.e. 19 mM internal p-NPP).4. p-NPP inhibits with equal effectiveness the Na:K and the Na:Na exchanges catalysed by the Na pump.5. The inhibitory effect of p-NPP cannot be attributed to the products of its hydrolysis, is inversely related to the intracellular ATP concentration and seems to be exerted at the inner surface of the cell membrane with an apparent affinity similar to that of the membrane phosphatase. These facts suggest that inhibition is mediated by the combination of p-NPP with the active centre of the membrane phosphatase.6. Apart from affecting the ouabain-sensitive cation movements, p-NPP increases the ouabain-resistant uptake and loss of both Na and Rb. This effect is about 4 times larger for Rb than for Na, and its kinetic analysis suggests that it is due to an increase in the passive permeability of the cell membrane.7. The increase in passive cation permeability upon addition of p-NPP cannot be attributed to the products of its hydrolysis. It seems to be due to the combination of p-NPP with a site which, like the active centre of the ouabain-resistant membrane phosphatase, faces the inner surface of the cell membrane, is unaffected by ATP and is half saturated by about 15 mM-p NPP.

摘要

当红细胞在含有对硝基苯磷酸酯（p-NPP）的溶液中孵育时，细胞内的p-NPP会迅速积累，在3分钟的半衰期内，细胞内水中的浓度达到外部浓度的四分之一，在所用条件下，这是吉布斯-唐南平衡中一种二价阴离子的预期值。因此，添加到红细胞孵育培养基中的p-NPP能够快速进入位于细胞膜内表面的膜磷酸酶的活性中心。
当将p-NPP添加到无ATP的红细胞或重构血影的孵育培养基中时，未检测到哇巴因敏感的阳离子移动，这表明活性运输系统对p-NPP的水解无法为活性离子转运提供能量。
当含ATP细胞的孵育培养基中p-NPP浓度逐渐升高时，哇巴因敏感的钠流失和哇巴因敏感的铷摄取均沿矩形双曲线趋于零。对于这两种移动，在外部p-NPP浓度为77 mM（即内部p-NPP浓度为19 mM）时抑制作用达到半数最大。
p-NPP对钠泵催化的钠钾交换和钠钠交换具有同等有效的抑制作用。
p-NPP的抑制作用不能归因于其水解产物，与细胞内ATP浓度呈负相关，似乎作用于细胞膜的内表面，其表观亲和力与膜磷酸酶相似。这些事实表明，抑制作用是由p-NPP与膜磷酸酶的活性中心结合介导的。
除了影响哇巴因敏感的阳离子移动外，p-NPP还增加了钠和铷的哇巴因抗性摄取和流失。这种效应对于铷来说比对钠大约大4倍，其动力学分析表明这是由于细胞膜被动通透性增加所致。
添加p-NPP后被动阳离子通透性的增加不能归因于其水解产物。这似乎是由于p-NPP与一个位点结合，该位点与哇巴因抗性膜磷酸酶的活性中心一样，面向细胞膜的内表面，不受ATP影响，在约15 mM-p NPP时达到半数饱和。