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脂肪细胞中氯化铝和磷脂酶C对葡萄糖载体活性的调节

Regulation of glucose carrier activity by AlCl3 and phospholipase C in fat-cells.

作者信息

Obermaier-Kusser B, Mühlbacher C, Mushack J, Rattenhuber E, Fehlmann M, Haring H U

机构信息

Institute for Diabetes Research, Munich, Federal Republic of Germany.

出版信息

Biochem J. 1988 Dec 1;256(2):515-20. doi: 10.1042/bj2560515.

Abstract

UNLABELLED

Recently it was speculated that activation of GTP-binding proteins and of phospholipase is involved in the transmission of a signal from the insulin-receptor kinase to effector systems in the cell. To confirm this hypothesis, we have tested the effect of AlCl3, which has been recently used as an experimental tool to activate GTP-binding proteins, on glucose transport in fat-cells. We found that AlCl3 has a partial insulin-like effect on glucose transport activity (3-O-methylglucose uptake, expressed as % of equilibrium value per 4 s: basal 9.6 +/- 2, AlCl3 29.6 +/- 4, insulin 74.0 +/- 3). The AlCl3 effect is totally blocked by pertussis toxin, whereas the insulin effect was not altered. The effect starts at [AlCl3] greater than 1 fM and reaches its maximum at 0.1 nM. Addition of phospholipase C (PLC; 50 munits/ml) also stimulated glucose transport (maximal 53.0 +/- 5%). Both substances acted faster than insulin itself (maximal values within 1 min for PLC, 2 min for AlCl3 and 5-10 min for insulin). Using the cytochalasin-B-binding assay to determine the effects of AlCl3 and PLC on the distribution of glucose carrier sites in subcellular fractions, we found that their glucose-transport-stimulating effect does not occur through an increase in glucose carrier sites in the plasma-membrane fraction. When PLC was combined with the phorbol ester TPA (12-O-tetradecanoylphorbol 13-acetate), which increases glucose carrier sites in the plasma membrane, an additive effect on glucose transport was found [PLC (50 munits/ml), 53.0 +/- 5%, TPA (1 nM), 17.3 +/- 2%; PLC + TPA, 68.0 +/- 3%].

IN CONCLUSION

(1) the data show that AlCl3, probably through activation of a pertussis-toxin-inhibitable G protein, and PLC are able to modulate the intrinsic glucose carrier activity; (2) as pertussis toxin did not modify the effect of insulin, it seems unlikely that the insulin signal on glucose transport involves activation of this specific G protein.

摘要

未标记

最近有人推测,GTP结合蛋白和磷脂酶的激活参与了从胰岛素受体激酶到细胞内效应系统的信号传递。为了证实这一假设,我们测试了最近被用作激活GTP结合蛋白的实验工具的AlCl3对脂肪细胞葡萄糖转运的影响。我们发现,AlCl3对葡萄糖转运活性具有部分胰岛素样作用(3-O-甲基葡萄糖摄取,以每4秒平衡值的百分比表示:基础值9.6±2,AlCl3 29.6±4,胰岛素74.0±3)。AlCl3的作用完全被百日咳毒素阻断,而胰岛素的作用未改变。该作用在[AlCl3]大于1 fM时开始,在0.1 nM时达到最大值。添加磷脂酶C(PLC;50单位/毫升)也刺激了葡萄糖转运(最大53.0±5%)。两种物质的作用都比胰岛素本身更快(PLC在1分钟内达到最大值,AlCl3在2分钟内达到最大值,胰岛素在5 - 10分钟内达到最大值)。使用细胞松弛素B结合试验来确定AlCl3和PLC对亚细胞组分中葡萄糖载体位点分布的影响,我们发现它们刺激葡萄糖转运的作用不是通过增加质膜组分中的葡萄糖载体位点来实现的。当PLC与佛波酯TPA(12-O-十四酰佛波醇13-乙酸酯)联合使用时,TPA可增加质膜中的葡萄糖载体位点,发现对葡萄糖转运有相加作用[PLC(50单位/毫升)为53.0±5%,TPA(1 nM)为17.3±2%;PLC + TPA为68.0±3%]。

结论

(1)数据表明,AlCl3可能通过激活一种可被百日咳毒素抑制的G蛋白,以及PLC能够调节内在的葡萄糖载体活性;(2)由于百日咳毒素未改变胰岛素的作用,胰岛素对葡萄糖转运的信号似乎不太可能涉及这种特定G蛋白的激活。

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