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镁对人红细胞糖酵解通量的调节作用。

The regulatory role for magnesium in glycolytic flux of the human erythrocyte.

作者信息

Laughlin M R, Thompson D

机构信息

Department of Surgery, George Washington University Medical Center, Washington, D. C. 20037, USA.

出版信息

J Biol Chem. 1996 Nov 15;271(46):28977-83. doi: 10.1074/jbc.271.46.28977.

Abstract

31P NMR was used to measure the intracellular free magnesium concentration ([Mg2+]i) in human erythrocytes while [Mg2+]i was changed between 0.01 and 1.2 mM using the divalent cationophore A23187. 13C NMR and [2-13C]glucose were used to determine the kinetic effects of [Mg2+]i by measuring the flux through several parts of the glucose pathway. Glucose utilization was strongly dependent on [Mg2+]i, with half-maximal flux occurring at 0.03 mM. The rate-limiting step was most likely at phosphofructokinase, which has a Km(Mg2+) of 0.025 mM in the purified enzyme. Phosphorylated glycolytic intermediate concentration was also strongly dependent on [Mg2+]i and [MgATP], and glucose transport plus hexokinase may have been partially rate-determining at [Mg2+]i below approximately 0.1 mM. The pentose phosphate shunt activity was too low to determine the dependence on [Mg2+]i. Phosphoglycerate kinase and 2, 3-diphosphoglycerate mutase fluxes were also measured, but were not rate-limiting for glycolysis and showed no Mg2+ dependence. Human erythrocyte [Mg2+]i varies between 0.2 mM (oxygenated) and 0.6 mM (deoxygenated), well above the measured [Mg2+]i(1/2). It is unlikely, then, that [Mg2+]i plays a regulatory role in normal erythrocyte glycolysis.

摘要

采用31P核磁共振技术测定人红细胞内游离镁离子浓度([Mg2+]i),同时使用二价阳离子载体A23187将[Mg2+]i在0.01至1.2 mM之间进行改变。利用13C核磁共振技术和[2-13C]葡萄糖,通过测量葡萄糖途径几个部分的通量来确定[Mg2+]i的动力学效应。葡萄糖利用强烈依赖于[Mg2+]i,半数最大通量出现在0.03 mM时。限速步骤很可能位于磷酸果糖激酶,其在纯化酶中的Km(Mg2+)为0.025 mM。磷酸化糖酵解中间产物浓度也强烈依赖于[Mg2+]i和[MgATP],在[Mg2+]i低于约0.1 mM时,葡萄糖转运加己糖激酶可能部分决定了反应速率。磷酸戊糖途径的活性过低,无法确定其对[Mg2+]i的依赖性。还测量了磷酸甘油酸激酶和2,3-二磷酸甘油酸变位酶的通量,但它们对糖酵解不是限速步骤,且未显示出对Mg2+的依赖性。人红细胞的[Mg2+]i在0.2 mM(氧合)至0.6 mM(脱氧)之间变化,远高于测量的[Mg2+]i(1/2)。因此,[Mg2+]i不太可能在正常红细胞糖酵解中起调节作用。

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