Kardassis D, Sacharidou E, Zannis V I
Division of Basic Sciences, Section of Biochemistry, Department Of Medicine, University Of Crete and Institute Of Molecular Biology and Biotechnology, Heraklion, Crete, Greece.
J Biol Chem. 1998 Jul 10;273(28):17810-6. doi: 10.1074/jbc.273.28.17810.
The regulatory elements CIIC (-159/-116) and CIIB (-102/-81) of the apolipoprotein CII (apoCII) promoter have distinct specificities for orphan nuclear receptors (Vorgia, P., Zannis, V. I., and Kardassis, D. (1998) J. Biol. Chem. 273, 4188-4199). In this communication we investigated the contribution of ligand-dependent and orphan nuclear receptors on the transcriptional regulation of the human apoCII gene. It was found that element CIIC in addition to ARP-1 and EAR-2 binds RXRalpha/T3Rbeta heterodimers strongly, whereas element CIIB binds hepatic nuclear factor 4 (HNF-4) exclusively. Binding is abolished by mutations that alter the HRE binding motifs. Transient cotransfection experiments showed that in the presence of T3, RXRalpha/T3Rbeta heterodimers transactivated the -205/+18 apoCII promoter 1.6- and 11-fold in HepG2 and COS-1 respectively. No transactivation was observed in the presence of 9-cis-retinoic acid. Transactivation requires the regulatory element CIIC, suggesting that this element contains a thyroid hormone response element. HNF-4 did not affect the apoCII promoter activity in HepG2 cells. However, mutations in the HNF-4 binding site on element CIIB and inhibition of HNF-4 synthesis in HepG2 cells by antisense HNF-4 constructs decreased the apoCII promoter activity to 25-40% of the control, indicating that HNF-4 is a positive regulator of the apoCII gene. ARP-1 repressed the -205/+18 but not the -104/+18 apoCII promoter activity in HepG2 cells, indicating that the repression depends on the regulatory element CIIC. In contrast, combination of ARP-1 and HNF-4 transactivated different apoCII promoter segments as well as a minimal adenovirus major late promoter driven by the regulatory element CIIB. Mutagenesis or deletion of elements CIIB or CIIC established that the observed transactivation requires DNA binding of one of the two factors and may result from HNF-4-ARP-1 interactions that elicit the transactivation functions of HNF-4. The combined data indicate that RXRalpha/T3Rbeta in the presence of T3 and HNF-4 can upregulate the apoCII promoter activity by binding to the regulatory elements CIIC and CIIB, respectively. In addition, ARP-1 can either have inhibitory or stimulatory effects on the apoCII promoter activity via different mechanisms.
载脂蛋白CII(apoCII)启动子的调控元件CIIC(-159 / -116)和CIIB(-102 / -81)对孤儿核受体具有不同的特异性(Vorgia,P.,Zannis,V. I.,和Kardassis,D.(1998)J. Biol. Chem. 273,4188 - 4199)。在本通讯中,我们研究了配体依赖性和孤儿核受体对人apoCII基因转录调控的作用。发现元件CIIC除了与ARP - 1和EAR - 2结合外,还能强烈结合RXRα/T3Rβ异二聚体,而元件CIIB仅结合肝细胞核因子4(HNF - 4)。改变HRE结合基序的突变会消除这种结合。瞬时共转染实验表明,在存在T3的情况下,RXRα/T3Rβ异二聚体在HepG2和COS - 1细胞中分别使-205 / +18 apoCII启动子激活1.6倍和11倍。在存在9 - 顺式视黄酸的情况下未观察到激活作用。激活需要调控元件CIIC,这表明该元件含有甲状腺激素反应元件。HNF - 4不影响HepG2细胞中apoCII启动子的活性。然而,元件CIIB上HNF - 4结合位点的突变以及反义HNF - 4构建体对HepG2细胞中HNF - 4合成的抑制作用使apoCII启动子活性降至对照的25 - 40%,表明HNF - 4是apoCII基因的正调控因子。ARP - 1抑制HepG2细胞中-205 / +18但不抑制-104 / +18 apoCII启动子的活性,这表明这种抑制作用取决于调控元件CIIC。相反,ARP - 1和HNF - 4的组合激活了不同的apoCII启动子片段以及由调控元件CIIB驱动的最小腺病毒主要晚期启动子。对元件CIIB或CIIC进行诱变或缺失表明,观察到的激活需要这两种因子之一与DNA结合,并且可能是由引发HNF - 4转录激活功能的HNF - 4 - ARP - 1相互作用导致的。综合数据表明,在存在T3的情况下,RXRα/T3Rβ和HNF - 4可分别通过与调控元件CIIC和CIIB结合来上调apoCII启动子的活性。此外,ARP - 1可通过不同机制对apoCII启动子活性产生抑制或刺激作用。
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