Iynedjian P B, Marie S, Wang H, Gjinovci A, Nazaryan K
Division of Clinical Biochemistry and Diabetes Research, University of Geneva School of Medicine, 1211 Geneva, Switzerland.
J Biol Chem. 1996 Nov 15;271(46):29113-20. doi: 10.1074/jbc.271.46.29113.
Glucokinase gene regions that are important for liver specific expression of the enzyme have been functionally identified using transient transfection of rat hepatocytes. Maximal luciferase activity was elicited by a reporter plasmid with 3.4 kilobase pairs of genomic DNA flanking the liver glucokinase promoter. Deletion of a gene fragment between -1000 and -600 with respect to the start of transcription resulted in a 60% decrease in luciferase activity. Further reduction, close to background level, occurred upon deletion of a 90-base pair sequence between -123 and -34. Reporter plasmids with the liver glucokinase promoter and any length of flanking sequence were minimally active in INS-1 insulinoma cells, and conversely reporters with the beta-cell-specific promoter were ineffective in primary hepatocytes. In FTO-2B hepatoma cells, a differentiated line expressing many liver-specific traits but not the endogenous glucokinase gene, the promoter proximal region between -123 and -34 markedly stimulated the expression of transfected plasmids above background. However, addition of the flanking region up to -1000 inhibited luciferase expression. The gene fragment from -1003 to -707 was shown to be a bona fide, hepatocyte-specific enhancer by the following criteria: 1) it stimulated reporter expression by more than 10- and 5-fold when inserted directly upstream of the glucokinase TATA box or complete promoter, respectively, regardless of orientation; 2) it stimulated gene expression from the heterologous SV 40 promoter 4-fold; 3) it was also effective from a downstream position; and 4) in contrast to the enhancer effect in primary hepatocytes, the sequence acted as a silencer in FTO-2B cells and was neutral in INS-1 cells. Both the promoter proximal and the enhancer regions were marked by DNase I hypersensitive sites in the chromatin of primary hepatocytes but not hepatoma or insulinoma cells. Seven footprinted elements termed A through G were mapped in the enhancer by the in vitro DNase I protection assay. Elements A-C may bind liver enriched factors, because they were not protected by spleen nuclear extract. In hepatocyte transfection, the downstream half of the enhancer containing elements A-C was about half as effective as the complete enhancer in stimulating glucokinase promoter activity. Site-directed mutagenesis of element A virtually abrogated the activity of the half-enhancer, whereas mutation of element C had a more moderate effect. The sequence between -732 and -578 upstream of the liver start of transcription in the human glucokinase gene displays 79% sequence identity with the downstream half of the rat enhancer. The human gene fragment ligated to the minimal rat liver glucokinase promoter was shown to work as an enhancer in the hepatocyte transfection system.
利用大鼠肝细胞的瞬时转染技术,已在功能上鉴定出对该酶肝脏特异性表达至关重要的葡萄糖激酶基因区域。一个带有3.4千碱基对肝脏葡萄糖激酶启动子侧翼基因组DNA的报告质粒引发了最大的荧光素酶活性。相对于转录起始点,缺失-1000至-600之间的基因片段导致荧光素酶活性降低60%。进一步缺失-123至-34之间90个碱基对的序列后活性进一步降低,接近背景水平。带有肝脏葡萄糖激酶启动子和任何长度侧翼序列的报告质粒在INS -1胰岛素瘤细胞中活性极低,相反,带有β细胞特异性启动子的报告质粒在原代肝细胞中无效。在FTO -2B肝癌细胞中,该细胞系表达许多肝脏特异性特征但不表达内源性葡萄糖激酶基因,启动子近端区域-123至-34之间显著刺激转染质粒的表达高于背景水平。然而,添加直至-1000的侧翼区域会抑制荧光素酶表达。-1003至-707的基因片段被证明是一个真正的肝细胞特异性增强子,依据以下标准:1)当分别直接插入葡萄糖激酶TATA盒或完整启动子上游时,无论方向如何,它分别刺激报告基因表达超过10倍和5倍;2)它刺激来自异源SV40启动子的基因表达4倍;3)从下游位置也有效;4)与在原代肝细胞中的增强子效应相反,该序列在FTO -2B细胞中起沉默子作用,在INS -1细胞中呈中性。启动子近端区域和增强子区域在原代肝细胞染色质中均有DNase I超敏位点标记,但在肝癌或胰岛素瘤细胞中没有。通过体外DNase I保护试验在增强子中定位了七个足迹元件,称为A至G。元件A - C可能结合肝脏富集因子,因为它们未被脾核提取物保护。在肝细胞转染中,包含元件A - C的增强子下游一半在刺激葡萄糖激酶启动子活性方面约为完整增强子的一半效果。元件A的定点诱变几乎消除了半增强子活性,但元件C的突变影响较温和。人类葡萄糖激酶基因转录起始点上游-732至-578之间的序列与大鼠增强子下游一半具有79% 的序列同一性。连接到最小大鼠肝脏葡萄糖激酶启动子的人类基因片段在肝细胞转染系统中显示出作为增强子的作用。
