Morgan M S, Darrow R M, Nafz M A, Varandani P T
Biochem J. 1985 Jan 15;225(2):349-56. doi: 10.1042/bj2250349.
The effects on the uptake (cell-associated 125I) and degradation (125I-labelled products released into the medium) of 125I-insulin and bioactivity (protein, glycogen and lipid synthesis) of insulin caused by altering the cellular thiol/disulphide status in primary cultures of rat hepatocytes were studied. Incubation of hepatocyte cultures with various exogenous thiol compounds (reduced glutathione, 2-mercaptoethanol, cysteamine, dithiothreitol) resulted in increased insulin binding, but markedly decreased degradation and bioactivity. These effects could be reversed by washing or by the addition of oxidized glutathione, which alone had no effect. When cultures were exposed to certain thiol-modifying reagents (N-ethylmaleimide, p-chloromercuribenzoate, p-chloromercuribenzenesulphonate, iodoacetamide, iodoacetate), some decreases in bioactivity were evident, but the pronounced decrease in insulin degradation observed with the thiol-containing compounds was not observed with this class of compounds. None of the thiol-containing or -modifying agents tested had any significant effect on cellular ATP concentrations, indicating that the effects observed were due to perturbation of the thiol/disulphide status. Depletion of intracellular glutathione by DL-buthionine SR-sulphoximine (a specific inhibitor of glutathionine biosynthesis) decreased the syntheses of glycogen and lipid by about one-half, while having essentially no effect on protein synthesis, ATP concentrations or on the binding and degradation of insulin. The data presented here indicate that although intracellular thiol (glutathione) concentrations may be important for the maintenance of full expression of certain biological activities (glycogen and lipid synthesis), the thiol/disulphide groups on the cell surface and those immediately inside the cell membrane may be more critical in the mediation of insulin action, including the degradation and bioactivity of insulin in primary cultures of rat hepatocytes.
研究了在大鼠肝细胞原代培养物中改变细胞内硫醇/二硫键状态对¹²⁵I-胰岛素摄取(细胞结合的¹²⁵I)、降解(释放到培养基中的¹²⁵I标记产物)以及胰岛素生物活性(蛋白质、糖原和脂质合成)的影响。用各种外源性硫醇化合物(还原型谷胱甘肽、2-巯基乙醇、半胱胺、二硫苏糖醇)孵育肝细胞培养物,导致胰岛素结合增加,但降解和生物活性显著降低。通过洗涤或添加氧化型谷胱甘肽可逆转这些作用,而氧化型谷胱甘肽单独使用时无作用。当培养物暴露于某些硫醇修饰试剂(N-乙基马来酰胺、对氯汞苯甲酸、对氯汞苯磺酸盐、碘乙酰胺、碘乙酸)时,生物活性有一些降低,但未观察到含硫醇化合物所观察到的胰岛素降解明显降低。所测试的含硫醇或硫醇修饰剂均对细胞内ATP浓度无显著影响,表明所观察到的作用是由于硫醇/二硫键状态的扰动。用DL-丁硫氨酸亚砜亚胺(谷胱甘肽生物合成的特异性抑制剂)耗尽细胞内谷胱甘肽,使糖原和脂质合成减少约一半,而对蛋白质合成、ATP浓度以及胰岛素的结合和降解基本无影响。此处给出的数据表明,虽然细胞内硫醇(谷胱甘肽)浓度对于维持某些生物学活性(糖原和脂质合成)的充分表达可能很重要,但细胞表面和细胞膜内侧紧邻的硫醇/二硫键基团在介导胰岛素作用方面可能更为关键,包括大鼠肝细胞原代培养物中胰岛素的降解和生物活性。