肝细胞中葡萄糖激酶的细胞内结合以及葡萄糖、果糖和胰岛素介导的易位
Intracellular binding of glucokinase in hepatocytes and translocation by glucose, fructose and insulin.
作者信息
Agius L, Peak M
机构信息
Department of Medicine, University of Newcastle upon Tyne, U.K.
出版信息
Biochem J. 1993 Dec 15;296 ( Pt 3)(Pt 3):785-96. doi: 10.1042/bj2960785.
The release of glucokinase from digitonin-permeabilized hepatocytes shows different characteristics with respect to ionic strength and [MgCl2] from the release of other cytoplasmic enzymes. Release of glucokinase is most rapid at low ionic strength (300 mM sucrose, 3 mM Hepes) and is inhibited by increasing concentration of KCl [concn. giving half-maximal inhibition (I50) 25 mM] or Mg2+ (I50 0.5 mM). Release of phosphoglucoisomerase, phosphoglucomutase and glucose-6-phosphate dehydrogenase is independent of ionic strength, but shows a small inhibition by MgCl2 (20%, versus > 80% for glucokinase). Lactate dehydrogenase release increases with increasing ionic strength [concn. giving half-maximal activation (A50) 10 mM KCl] or [MgCl2]. The rate and extent of glucokinase release during permeabilization in 300 mM sucrose, 5 mM MgCl2 or in medium with ionic composition resembling cytoplasm (150 mM K+, 50 mM Cl-, 1 mM Mg2+) depends on the substrate concentrations with which the hepatocytes have been preincubated. In hepatocytes pre-cultured with 5 mM glucose the release of glucokinase was much slower than that of other cytoplasmic enzymes measured. However, preincubation with glucose (10-30 mM) or fructose (50 microM-1 mM) markedly increased glucokinase release. This suggests that, in cells maintained in 5 mM glucose, glucokinase is present predominantly in a bound state and this binding is dependent on the presence of Mg2+. The enzyme can be released or translocated from its bound state by an increase in [glucose] (A50 15 mM) or by fructose (A50 50 microM). The effects of glucose and fructose were rapid (t1/2 5 min) and reversible, and were potentiated by insulin and counteracted by glucagon. They were inhibited by cyanide, but not by cytochalasin D, phalloidin or colchicine. Mannose had a glucose-like effect (A50 approximately 15 mM), whereas galactose, 3-O-methyl-D-glucose and 2-deoxyglucose were ineffective. When hepatocytes were incubated with [2-3H, U-14C]glucose, the incorporation of 3H/14C label into glycogen correlated with the extent of glucokinase release. Since 2-3H is lost during conversion of glucose 6-phosphate into fructose 6-phosphate, substrate-induced translocation of glucokinase from a Mg(2+)-dependent binding site to an alternative site might favour the partitioning of glucose 6-phosphate towards glycogen, as opposed to phosphoglucoisomerase.
从洋地黄皂苷通透的肝细胞中释放葡萄糖激酶,与其他细胞质酶的释放相比,在离子强度和[MgCl₂]方面表现出不同的特性。葡萄糖激酶在低离子强度(300 mM蔗糖,3 mM Hepes)下释放最快,并受到KCl浓度增加(产生半数抑制的浓度(I₅₀)为25 mM)或Mg²⁺(I₅₀为0.5 mM)的抑制。磷酸葡萄糖异构酶、磷酸葡萄糖变位酶和葡萄糖-6-磷酸脱氢酶的释放与离子强度无关,但受到MgCl₂的轻微抑制(20%,而葡萄糖激酶为>80%)。乳酸脱氢酶的释放随着离子强度增加(产生半数激活的浓度(A₅₀)为10 mM KCl)或[MgCl₂]增加而增加。在300 mM蔗糖、5 mM MgCl₂或离子组成类似于细胞质的培养基(150 mM K⁺、50 mM Cl⁻、1 mM Mg²⁺)中通透处理期间,葡萄糖激酶的释放速率和程度取决于肝细胞预孵育时的底物浓度。在用5 mM葡萄糖预培养的肝细胞中,葡萄糖激酶的释放比所检测的其他细胞质酶慢得多。然而,用葡萄糖(10 - 30 mM)或果糖(50 μM - 1 mM)预孵育显著增加了葡萄糖激酶的释放。这表明,在维持于5 mM葡萄糖的细胞中,葡萄糖激酶主要以结合状态存在,且这种结合依赖于Mg²⁺的存在。该酶可通过[葡萄糖]增加(A₅₀为15 mM)或果糖(A₅₀为50 μM)从其结合状态释放或转位。葡萄糖和果糖的作用迅速(半衰期为5分钟)且可逆,并被胰岛素增强,被胰高血糖素抵消。它们被氰化物抑制,但不被细胞松弛素D、鬼笔环肽或秋水仙碱抑制。甘露糖具有类似葡萄糖的作用(A₅₀约为15 mM),而半乳糖、3 - O - 甲基 - D - 葡萄糖和2 - 脱氧葡萄糖无效。当肝细胞用[2 - ³H,U - ¹⁴C]葡萄糖孵育时,³H/¹⁴C标记掺入糖原的情况与葡萄糖激酶的释放程度相关。由于在葡萄糖6 - 磷酸转化为果糖6 - 磷酸的过程中² - ³H丢失,底物诱导的葡萄糖激酶从Mg(2 +)依赖性结合位点向另一位点的转位可能有利于葡萄糖6 - 磷酸向糖原的分配,而不是向磷酸葡萄糖异构酶的分配。
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