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细胞内和细胞外碳酸酐rase 非酶合作增强单羧酸转运蛋白的活性。

Intracellular and extracellular carbonic anhydrases cooperate non-enzymatically to enhance activity of monocarboxylate transporters.

机构信息

From the Division of General Zoology, Department of Biology, University of Kaiserslautern D-67653 Kaiserslautern, Germany and.

出版信息

J Biol Chem. 2014 Jan 31;289(5):2765-75. doi: 10.1074/jbc.M113.537043. Epub 2013 Dec 12.

Abstract

Proton-coupled monocarboxylate transporters (MCTs) are carriers of high-energy metabolites such as lactate, pyruvate, and ketone bodies and are expressed in most tissues. It has previously been shown that transport activity of MCT1 and MCT4 is enhanced by the cytosolic carbonic anhydrase II (CAII) independent of its catalytic activity. We have now studied the influence of the extracellular, membrane-bound CAIV on transport activity of MCT1/4, heterologously expressed in Xenopus oocytes. Coexpression of CAIV with MCT1 and MCT4 resulted in a significant increase in MCT transport activity, even in the nominal absence of CO2/HCO3(-). CAIV-mediated augmentation of MCT activity was independent of the CAIV catalytic function, since application of the CA-inhibitor ethoxyzolamide or coexpression of the catalytically inactive mutant CAIV-V165Y did not suppress CAIV-mediated augmentation of MCT transport activity. The interaction required CAIV at the extracellular surface, since injection of CAIV protein into the oocyte cytosol did not augment MCT transport function. The effects of cytosolic CAII (injected as protein) and extracellular CAIV (expressed) on MCT transport activity, were additive. Our results suggest that intra- and extracellular carbonic anhydrases can work in concert to ensure rapid shuttling of metabolites across the cell membrane.

摘要

质子偶联单羧酸转运体(MCTs)是高能代谢物如乳酸盐、丙酮酸和酮体的载体,在大多数组织中表达。先前已经表明,MCT1 和 MCT4 的转运活性通过细胞质碳酸酐酶 II(CAII)增强,而不依赖其催化活性。我们现在已经研究了细胞外、膜结合的 CAIV 对在非洲爪蟾卵母细胞中异源表达的 MCT1/4 转运活性的影响。CAIV 与 MCT1 和 MCT4 的共表达导致 MCT 转运活性显著增加,即使在不存在 CO2/HCO3(-)的情况下也是如此。CAIV 介导的 MCT 活性增强不依赖于 CAIV 的催化功能,因为 CA 抑制剂乙氧唑胺的应用或催化活性丧失的 CAIV-V165Y 突变体的共表达并未抑制 CAIV 介导的 MCT 转运活性增强。这种相互作用需要 CAIV 在细胞外表面,因为将 CAIV 蛋白注入卵母细胞胞质中不会增强 MCT 转运功能。细胞质 CAII(作为蛋白注射)和细胞外 CAIV(表达)对 MCT 转运活性的影响是相加的。我们的结果表明,细胞内和细胞外碳酸酐酶可以协同工作,以确保代谢物快速穿过细胞膜。

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