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胰岛素对离体大鼠膈肌葡萄糖转运作用的潜在机制。细胞内转运单位向质膜的明显易位。

Potential mechanism of insulin action on glucose transport in the isolated rat diaphragm. Apparent translocation of intracellular transport units to the plasma membrane.

作者信息

Wardzala L J, Jeanrenaud B

出版信息

J Biol Chem. 1981 Jul 25;256(14):7090-3.

PMID:6265437
Abstract

[3H]Cytochalasin B binding and its competitive inhibition by D-glucose have been used to quantitate the number of functional glucose transport units in plasma and microsomal membranes prepared from intact rat diaphragm. In a series of three experiments, plasma membranes prepared from diaphragms which have not been incubated with insulin bind approximately 16 pmol of cytochalasin B/mg of membrane protein to the D-glucose-inhibitable binding site. If 280 nM (40,000 microunits/ml) insulin is present during the incubation, cytochalasin B binding to the plasma membranes is increased approximately 2-fold without alteration in the dissociation constant of this site. Membranes in the microsomal fraction prepared from diaphragms which have been incubated for 30 min in the absence of insulin contain 21 pmol of D-glucose-inhibitable cytochalasin B binding sites/mg of membrane protein. However, in the presence of insulin during the incubation period, the number of these sites in the microsomal fraction is decreased to 12 pmol/mg of membrane protein. These results suggest that insulin stimulates glucose transport in the isolated rat diaphragm primarily through a translocation of functional glucose transport units from an intracellular membrane pool to the plasma membrane. These results are similar to the results observed in rat adipose cells (Cushman, S. W., and Wardzala, L. J. (1980) J. Biol. Chem. 255, 4758-4762) and suggest that this mechanism of insulin-stimulated glucose transport activity may be general to other cell types.

摘要

[3H]细胞松弛素B结合及其被D-葡萄糖的竞争性抑制已被用于定量从完整大鼠膈肌制备的质膜和微粒体膜中功能性葡萄糖转运单位的数量。在一系列三个实验中,从未与胰岛素孵育的膈肌制备的质膜,在D-葡萄糖可抑制的结合位点上,每毫克膜蛋白结合约16皮摩尔细胞松弛素B。如果在孵育期间存在280 nM(40,000微单位/毫升)胰岛素,细胞松弛素B与质膜的结合增加约2倍,而该位点的解离常数没有改变。在无胰岛素的情况下孵育30分钟的膈肌制备的微粒体部分中的膜,每毫克膜蛋白含有21皮摩尔D-葡萄糖可抑制的细胞松弛素B结合位点。然而,在孵育期间存在胰岛素的情况下,微粒体部分中这些位点的数量减少到每毫克膜蛋白12皮摩尔。这些结果表明,胰岛素主要通过功能性葡萄糖转运单位从细胞内膜池向质膜的易位来刺激分离的大鼠膈肌中的葡萄糖转运。这些结果与在大鼠脂肪细胞中观察到的结果相似(库什曼,S.W.,和瓦尔扎拉,L.J.(1980年)《生物化学杂志》255,4758 - 4762),并表明这种胰岛素刺激的葡萄糖转运活性机制可能对其他细胞类型也普遍适用。

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