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人眼角膜缘上皮细胞和成纤维细胞中 GLUT1 活性的差异调节。

Differential regulation of GLUT1 activity in human corneal limbal epithelial cells and fibroblasts.

机构信息

Department of Chemistry and Biochemistry, Calvin College, 3201 Burton SE, Grand Rapids, MI 49546, USA.

出版信息

Biochimie. 2013 Feb;95(2):258-63. doi: 10.1016/j.biochi.2012.09.022. Epub 2012 Sep 23.

Abstract

The corneal epithelial tissue is a layer of rapidly growing cells that are highly glycolytic and express GLUT1 as the major glucose transporter. It has been shown that GLUT1 in L929 fibroblast cells and other cell lines can be acutely activated by a variety agents. However, the acute regulation of glucose uptake in corneal cells has not been systematically investigated. Therefore, we examined glucose uptake in an immortalized human corneal-limbal epithelial (HCLE) cell line and compared it to glucose uptake in L929 fibroblast cells, a cell line where glucose uptake has been well characterized. We report that the expression of GLUT1 in HCLE cells is 6.6-fold higher than in L929 fibroblast cells, but the HCLE cells have a 25-fold higher basal rate of glucose uptake. Treatment with agents that interfere with mitochondrial metabolism, such as sodium azide and berberine, activate glucose uptake in L929 cells over 3-fold, but have no effect on glucose uptake HCLE cells. Also, agents known to react with thiols, such cinnamaldehyde, phenylarsine oxide and nitroxyl stimulate glucose uptake in L929 cells 3-4-fold, but actually inhibit glucose uptake in HCLE cells. These data suggest that in the fast growing HCLE cells, GLUT1 is expressed at a higher concentration and is already highly activated at basal conditions. These data support a model for the acute activation of GLUT1 that suggests that the activity of GLUT1 is enhanced by the formation of an internal disulfide bond within GLUT1 itself.

摘要

角膜上皮组织是一层快速生长的细胞,具有高度的糖酵解作用,并表达 GLUT1 作为主要的葡萄糖转运蛋白。已经表明,L929 成纤维细胞和其他细胞系中的 GLUT1 可以被各种试剂急性激活。然而,角膜细胞中葡萄糖摄取的急性调节尚未得到系统研究。因此,我们检查了永生人角膜缘上皮 (HCLE)细胞系中的葡萄糖摄取,并将其与葡萄糖摄取进行了比较L929 成纤维细胞,一种葡萄糖摄取特征良好的细胞系。我们报告说,GLUT1 在 HCLE 细胞中的表达是 L929 成纤维细胞的 6.6 倍,但 HCLE 细胞的基础葡萄糖摄取率高 25 倍。用干扰线粒体代谢的试剂处理,如叠氮化钠和小檗碱,使 L929 细胞的葡萄糖摄取增加 3 倍以上,但对 HCLE 细胞的葡萄糖摄取没有影响。此外,已知与硫醇反应的试剂,如肉桂醛、苯胂氧化物和亚硝酸盐,使 L929 细胞的葡萄糖摄取增加 3-4 倍,但实际上抑制 HCLE 细胞的葡萄糖摄取。这些数据表明,在快速生长的 HCLE 细胞中,GLUT1 以更高的浓度表达,并在基础条件下已经高度激活。这些数据支持 GLUT1 急性激活的模型,表明 GLUT1 的活性通过 GLUT1 自身内部二硫键的形成而增强。

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