Rouet P, Raguenez G, Tronche F, Mfou'ou V, Salier J P
INSERM Unit 78, Boisguillaume, France.
Nucleic Acids Res. 1995 Feb 11;23(3):395-404. doi: 10.1093/nar/23.3.395.
Alpha-1-microglobulin and bikunin are two plasma glycoproteins encoded by an alpha-1-microglobulin/bikunin precursor (AMBP) gene. The strict liver-specific expression of the AMBP gene is controlled by a potent enhancer made of six clustered boxes numbered 1-6 that have been reported to be proven or potential binding sites for the hepatocyte-enriched nuclear factors HNF-1, -4, -3, -1, -3, -4, respectively. In the present study, electromobility shift assays of wild-type or mutated probes demonstrated that the boxes 1-5 have a binding capacity for their cognate HNF protein. Box 5 is also a target for another, as yet unidentified, factor. A functional analysis of the wild-type or mutated enhancer, driving its homologous promoter and a reporter CAT gene in the HepG2 hepatoma cell line, demonstrated that all six boxes participate in the enhancer activity, with the primary influence of box 4 (HNF-1) and box 2 (HNF-4). A similar analysis in the HNF-free CHO cell line co-transfected with one or several HNF factors further demonstrated various interplays between boxes: box 3 (HNF-3 alpha and beta) has a negative influence over the major HNF-4 box 2 as well as a positive influence over the major HNF-1 box 4.
α1-微球蛋白和 bikunin 是由α1-微球蛋白/bikunin 前体(AMBP)基因编码的两种血浆糖蛋白。AMBP 基因严格的肝脏特异性表达受一个由六个成簇的框组成的强效增强子控制,这六个框分别编号为 1 - 6,据报道它们分别是富含肝细胞核因子 HNF - 1、- 4、- 3α、- 3β、- 1、- 4 的已证实或潜在结合位点。在本研究中,对野生型或突变型探针进行的电泳迁移率变动分析表明,框 1 - 5 对其相应的 HNF 蛋白具有结合能力。框 5 也是另一种尚未鉴定的因子的作用靶点。在 HepG2 肝癌细胞系中对驱动其同源启动子和报告基因 CAT 的野生型或突变型增强子进行功能分析表明,所有六个框都参与增强子活性,其中框 4(HNF - 1)和框 2(HNF - 4)起主要作用。在与一种或几种 HNF 因子共转染的无 HNF 的 CHO 细胞系中进行的类似分析进一步证明了各框之间的各种相互作用:框 3(HNF - 3α和β)对主要的 HNF - 4 框 2 有负面影响,而对主要的 HNF - 1 框 4 有正面影响。
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