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18个氨基酸的U1A自身调节结构域内的决定因素,这些因素可解除协同RNA结合、多聚腺苷酸化抑制和同二聚化之间的偶联。

Determinants within an 18-amino-acid U1A autoregulatory domain that uncouple cooperative RNA binding, inhibition of polyadenylation, and homodimerization.

作者信息

Guan Fei, Palacios Daphne, Hussein Reem I, Gunderson Samuel I

机构信息

Rutgers University, Piscataway, New Jersey 08854, USA.

出版信息

Mol Cell Biol. 2003 May;23(9):3163-72. doi: 10.1128/MCB.23.9.3163-3172.2003.

Abstract

The human U1 snRNP-specific U1A protein autoregulates its own production by binding to and inhibiting the polyadenylation of its own pre-mRNA. Previous work demonstrated that a short sequence of U1A protein is essential for autoregulation and contains three distinct activities, which are (i) cooperative binding of two U1A proteins to a 50-nucleotide region of U1A pre-mRNA called polyadenylation-inhibitory element RNA, (ii) formation of a novel homodimerization surface, and (iii) inhibition of polyadenylation by inhibition of poly(A) polymerase (PAP). In this study, we purified and analyzed 11 substitution mutant proteins, each having one or two residues in this region mutated. In 5 of the 11 mutant proteins, we found that particular amino acids associate with one activity but not another, indicating that they can be uncoupled. Surprisingly, in three mutant proteins, these activities were improved upon, suggesting that U1A autoregulation is selected for suboptimal inhibitory efficiency. The effects of these mutations on autoregulatory activity in vivo were also determined. Only U1A and U170K are known to regulate nuclear polyadenylation by PAP inhibition; thus, these results will aid in determining how widespread this type of regulation is. Our molecular dissection of the consequences of conformational changes within an RNP complex presents a powerful example to those studying more complicated pre-mRNA-regulatory systems.

摘要

人类U1 snRNP特异性的U1A蛋白通过结合并抑制其自身前体mRNA的多聚腺苷酸化来自动调节自身的产生。先前的研究表明,U1A蛋白的一段短序列对于自动调节至关重要,并且包含三种不同的活性,即:(i)两个U1A蛋白协同结合到U1A前体mRNA的一个50个核苷酸区域,该区域称为多聚腺苷酸化抑制元件RNA;(ii)形成一个新的同二聚化表面;(iii)通过抑制多聚腺苷酸聚合酶(PAP)来抑制多聚腺苷酸化。在本研究中,我们纯化并分析了11种替代突变蛋白,每种蛋白在该区域有一个或两个残基发生突变。在11种突变蛋白中的5种中,我们发现特定氨基酸与一种活性相关而与另一种活性无关,这表明它们可以被解偶联。令人惊讶的是,在三种突变蛋白中,这些活性得到了改善,这表明U1A自动调节选择了次优的抑制效率。还确定了这些突变对体内自动调节活性的影响。已知只有U1A和U170K通过抑制PAP来调节核多聚腺苷酸化;因此,这些结果将有助于确定这种调节类型的广泛程度。我们对核糖核蛋白复合物内构象变化后果的分子剖析为研究更复杂的前体mRNA调节系统的人员提供了一个有力的例子。

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