Hatzivassiliou E, Cardot P, Zannis V I, Mitsialis S A
Department of Medicine, Boston University School of Medicine, 700 Albany Street, CABR-W509, Boston, Massachusetts 02118, USA.
Biochemistry. 1997 Jul 29;36(30):9221-31. doi: 10.1021/bi963145k.
We have analyzed the functional domains of the Drosophila orphan receptor Ultraspiracle (usp), a homologue of the vertebrate retinoic X receptor alpha, as well as the ability of heterodimers between usp and the thyroid hormone receptor beta (T3Rbeta) to transactivate the human apolipoprotein A-II (apoA-II) promoter. DNA binding assays demonstrated that heterodimers of usp and the human T3Rbeta can bind to the hormone response element (HRE) of the regulatory element AIIJ (-734 to -716) of the human apoA-II promoter. Cotransfection experiments have shown that the combination of usp and T3Rbeta can transactivate the human apoA-II promoter in COS-1 cells 7-8-fold in the presence of thyroid hormone (T3). The observed transactivation was not affected by the deletion of the amino-terminal residues 1-85 of usp, which represent a putative transactivation domain, suggesting that the function of usp is to recruit T3Rbeta. Furthermore, a mutant usp, with impaired DNA binding properties, can form heterodimers with T3Rbeta in vitro but has reduced ability to transactivate the human apoA-II promoter. A minimal thymidine kinase (tk) promoter driven by four AIIJ regulatory elements is repressed to 20% of its original activity by T3Rbeta and the repression is relieved by usp/T3Rbeta heterodimers. Deletion analysis demonstrated that factors bound to the regulatory elements AIIJ, AIIAB, and AIIH participate in the usp/T3Rbeta-mediated transactivation of the human apoA-II promoter. Similarly to element AIIJ, element AIIAB binds usp/T3Rbeta heterodimers, whereas element AIIH binds a COS-1 nuclear activity that is supershifted with anti-hepatic nuclear factor 1 antibodies. The findings suggest that optimal transactivation of the apoA-II promoter by usp/T3Rbeta heterodimers requires complex interactions between these heterodimers and factors bound to other regulatory elements. The observed transcriptional activation through heterodimer formation between nuclear receptors from species as divergent in the evolutionary scale as insects and mammals indicates that the functional domains of these proteins have been highly conserved.
我们分析了果蝇孤儿受体超气门蛋白(usp)的功能结构域,它是脊椎动物视黄酸X受体α的同源物,还研究了usp与甲状腺激素受体β(T3Rβ)之间的异二聚体激活人载脂蛋白A-II(apoA-II)启动子的能力。DNA结合试验表明,usp与人T3Rβ的异二聚体能够结合人apoA-II启动子调控元件AIIJ(-734至-716)的激素反应元件(HRE)。共转染实验表明,在甲状腺激素(T3)存在的情况下,usp和T3Rβ的组合能够在COS-1细胞中激活人apoA-II启动子7至8倍。观察到的激活不受usp氨基末端1至85位残基缺失的影响,这些残基代表一个假定的激活结构域,这表明usp的功能是招募T3Rβ。此外,一个DNA结合特性受损的突变体usp在体外能够与T3Rβ形成异二聚体,但激活人apoA-II启动子的能力降低。由四个AIIJ调控元件驱动的最小胸苷激酶(tk)启动子被T3Rβ抑制至其原始活性的20%,而usp/T3Rβ异二聚体可缓解这种抑制。缺失分析表明,与调控元件AIIJ、AIIAB和AIIH结合的因子参与了usp/T3Rβ介导的人apoA-II启动子的激活。与元件AIIJ类似,元件AIIAB结合usp/T3Rβ异二聚体,而元件AIIH结合一种COS-1核活性,该活性可被抗肝细胞核因子1抗体超迁移。这些发现表明,usp/T3Rβ异二聚体对apoA-II启动子的最佳激活需要这些异二聚体与结合在其他调控元件上的因子之间的复杂相互作用。通过昆虫和哺乳动物等在进化尺度上差异巨大的物种的核受体之间形成异二聚体所观察到的转录激活表明,这些蛋白质的功能结构域高度保守。
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