Roberts L R, Nichols L A, Holland L J
Department of Physiology, University of Missouri School of Medicine, Columbia 65212.
Biochemistry. 1993 Nov 2;32(43):11627-37. doi: 10.1021/bi00094a020.
The blood-clotting protein fibrinogen is composed of three subunits, designated A alpha, B beta, and gamma, which are encoded by a family of related genes. As part of the acute-phase response, expression of the fibrinogen genes is coordinately regulated in the liver by glucocorticoids. To understand the factors underlying this hormonal response, we have examined control of transcription from fibrinogen gene fragments transfected into hepatocytes from the frog Xenopus laevis. This analysis is the first in any species to define transcriptional regulatory elements for the fibrinogen genes by transfection into primary liver cells, rather than liver-derived cell lines. A transfection vector was constructed containing the Xenopus B beta gene transcription start site and 1293 bp of the 5' flanking sequence linked to the firefly luciferase gene. When this construct was transfected into primary liver parenchymal cells, luciferase expression was induced approximately 14-fold by glucocorticoids, an increase similar to the transcriptional stimulation of the endogenous B beta subunit gene. DNA fragments with as little as 284 bases of upstream sequence retained full hormone responsiveness. This region contains a sequence resembling the canonical glucocorticoid response element (GRE) at bases -148 to -162. Deletions or specific point mutations eliminating this putative GRE led to complete loss of glucocorticoid inducibility. Physical association of the steroid hormone receptor with this functional GRE was demonstrated with a truncated form of the rat glucocorticoid receptor containing the DNA-binding domain. A second possible GRE at positions -526 to -540 was not hormone-responsive, in either the presence or the absence of the more proximal GRE. The regulatory region also has a sequence similar to the binding site for a liver-specific transcription factor, hepatocyte nuclear factor 1 (HNF-1), at positions -120 to -132. Specific point mutations in the HNF-1-binding site, in a construct containing a wild-type GRE, reduced promoter activity by a factor of 10, while stimulation by glucocorticoids was retained. Binding studies confirmed specific interaction between this site and the transcription factor HNF-1 alpha from mouse. Thus, we have identified a GRE sufficient to account for full glucocorticoid inducibility and an HNF-1 site close to the promoter that are major determinants of transcriptional control of the Xenopus fibrinogen B beta subunit gene in cells from normal liver tissue.
凝血蛋白纤维蛋白原由三个亚基组成,分别命名为Aα、Bβ和γ,它们由一组相关基因编码。作为急性期反应的一部分,纤维蛋白原基因的表达在肝脏中受到糖皮质激素的协同调节。为了了解这种激素反应的潜在因素,我们研究了转染到非洲爪蟾肝细胞中的纤维蛋白原基因片段的转录调控。这种分析是首次在任何物种中通过转染原代肝细胞而非肝源性细胞系来确定纤维蛋白原基因的转录调控元件。构建了一个转染载体,其中包含非洲爪蟾Bβ基因转录起始位点和与萤火虫荧光素酶基因相连的1293 bp的5'侧翼序列。当这个构建体转染到原代肝实质细胞中时,荧光素酶表达受到糖皮质激素的诱导,增加了约14倍,这一增加与内源性Bβ亚基基因的转录刺激相似。上游序列仅有284个碱基的DNA片段仍保留了完整的激素反应性。该区域在碱基-148至-162处包含一个类似于典型糖皮质激素反应元件(GRE)的序列。消除这个假定的GRE的缺失或特定点突变导致糖皮质激素诱导性完全丧失。用含有DNA结合结构域的大鼠糖皮质激素受体的截短形式证明了类固醇激素受体与这个功能性GRE的物理结合。在-526至-540位置的第二个可能的GRE在存在或不存在更近端的GRE的情况下均无激素反应性。调控区域在-120至-132位置还有一个与肝特异性转录因子肝细胞核因子1(HNF-1)结合位点相似的序列。在含有野生型GRE的构建体中,HNF-1结合位点的特定点突变使启动子活性降低了10倍,同时保留了糖皮质激素的刺激作用。结合研究证实了该位点与小鼠转录因子HNF-1α之间的特异性相互作用。因此,我们确定了一个足以解释完全糖皮质激素诱导性的GRE和一个靠近启动子的HNF-1位点,它们是正常肝组织细胞中非洲爪蟾纤维蛋白原Bβ亚基基因转录调控的主要决定因素。
