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葡萄糖可诱导胰腺β细胞中早期生长反应基因(Egr-1)的表达。

Glucose induces early growth response gene (Egr-1) expression in pancreatic beta cells.

作者信息

Josefsen K, Sørensen L R, Buschard K, Birkenbach M

机构信息

Bartholin Institute, Kommunehospitalet, Copenhagen, Denmark.

出版信息

Diabetologia. 1999 Feb;42(2):195-203. doi: 10.1007/s001250051139.

DOI:10.1007/s001250051139
PMID:10064100
Abstract

A copy deoxyribonucleic acid (cDNA) clone of the immediate early growth response gene, egr-1 (Krox-24, Zif268, NGFI-1), was isolated through subtractive hybridization screening to identify glucose-induced genes in pancreatic beta cells. Glucose rapidly and transiently induced egr-1 mRNA in the SV40-transformed murine beta-cell line, MIN6. Glucose also increased egr-1 mRNA expression in INS-1, betaTC3 and RINm5F beta-cell lines, although with different kinetics. Expression of the 82 kDa Egr-1 protein was induced both in MIN6 cells stimulated with glucose in vitro and in primary rat islet cells stimulated in vivo or in vitro. This response is unique to beta cells since glucose did not affect egr-1 expression in NIH-3T3 fibroblasts or glucose-sensitive hepatocytes. In beta cells egr-1 induction is specifically associated with insulin secretion, as it was not observed after stimulation with serum or insulin but was elicited by insulin secretagogues, including membrane depolarizing agents and cAMP agonists. Moreover, induction of egr-1 by glucose was inhibited by EDTA, indicating dependence on influx of extracellular Ca2+. Other immediate early response genes, c-fos and junB, were also induced following glucose stimulation with kinetics similar to egr-1, whereas c-jun and junD expression were not affected. Since the zinc-finger protein encoded by egr-1 is highly homologous to transcription factors that control expression of glucose-regulated genes in yeast, Egr-1 could mediate delayed adaptive responses of beta cells to sustained glucose stimulation through transcriptional regulation.

摘要

通过消减杂交筛选分离出立即早期生长反应基因egr-1(Krox-24、Zif268、NGFI-1)的互补脱氧核糖核酸(cDNA)克隆,以鉴定胰腺β细胞中葡萄糖诱导的基因。葡萄糖能快速短暂地诱导SV40转化的小鼠β细胞系MIN6中的egr-1信使核糖核酸(mRNA)。葡萄糖也能增加INS-1、βTC3和RINm5Fβ细胞系中egr-1 mRNA的表达,尽管动力学有所不同。82 kDa的Egr-1蛋白表达在体外受葡萄糖刺激的MIN6细胞以及体内或体外受刺激的原代大鼠胰岛细胞中均被诱导。这种反应是β细胞特有的,因为葡萄糖不影响NIH-3T3成纤维细胞或葡萄糖敏感肝细胞中的egr-1表达。在β细胞中,egr-1的诱导与胰岛素分泌特异性相关,因为在血清或胰岛素刺激后未观察到这种诱导,但胰岛素促分泌剂(包括膜去极化剂和环磷酸腺苷(cAMP)激动剂)可引发这种诱导。此外,葡萄糖对egr-1的诱导被乙二胺四乙酸(EDTA)抑制,表明其依赖细胞外钙离子的内流。其他立即早期反应基因c-fos和junB在葡萄糖刺激后也以与egr-1相似的动力学被诱导,而c-jun和junD的表达未受影响

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