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长散在核元件1反转录转座所需的ORF1p内高度保守C末端结构域的鉴定及溶液结构

Identification and solution structure of a highly conserved C-terminal domain within ORF1p required for retrotransposition of long interspersed nuclear element-1.

作者信息

Januszyk Kurt, Li Patrick Wai-Lun, Villareal Valerie, Branciforte Dan, Wu Haihong, Xie Yongming, Feigon Juli, Loo Joseph A, Martin Sandra L, Clubb Robert T

机构信息

Department of Chemistry and Biochemistry, UCLA, Los Angeles, California 90095, USA.

出版信息

J Biol Chem. 2007 Aug 24;282(34):24893-904. doi: 10.1074/jbc.M702023200. Epub 2007 Jun 14.

DOI:10.1074/jbc.M702023200
PMID:17569664
Abstract

Long interspersed nuclear element-1 (LINE-1 or L1) retrotransposons comprise a large fraction of the human and mouse genomes. The mobility of these successful elements requires the protein encoded by open reading frame-1 (ORF1p), which binds single-stranded RNA with high affinity and functions as a nucleic acid chaperone. In this report, we have used limited proteolysis, filter binding, and NMR spectroscopy to characterize the global structure of ORF1p and the three-dimensional structure of a highly conserved RNA binding domain. ORF1p contains three structured regions, a coiled-coil domain, a middle domain of unknown function, and a C-terminal domain (CTD). We show that high affinity RNA binding by ORF1p requires the CTD and residues within an amino acid protease-sensitive segment that joins the CTD to the middle domain. Insights in the mechanism of RNA binding were obtained by determining the solution structure of the CTD, which is shown to adopt a novel fold consisting of a three-stranded beta sheet that is packed against three alpha-helices. An RNA binding surface on the CTD has been localized using chemical shift perturbation experiments and is proximal to residues previously shown to be essential for retrotransposition, RNA binding, and chaperone activity. A similar structure and mechanism of RNA binding is expected for all vertebrate long interspersed nuclear element-1 elements, since residues encoding the middle, protease-sensitive segment, and CTD are highly conserved.

摘要

长散在核元件1(LINE-1或L1)逆转录转座子占人类和小鼠基因组的很大一部分。这些成功元件的移动性需要开放阅读框1(ORF1p)编码的蛋白质,该蛋白质以高亲和力结合单链RNA并作为核酸伴侣发挥作用。在本报告中,我们使用了有限蛋白酶解、滤膜结合和核磁共振光谱来表征ORF1p的整体结构以及一个高度保守的RNA结合结构域的三维结构。ORF1p包含三个结构化区域,一个卷曲螺旋结构域、一个功能未知的中间结构域和一个C末端结构域(CTD)。我们表明,ORF1p的高亲和力RNA结合需要CTD以及连接CTD与中间结构域的氨基酸蛋白酶敏感片段内的残基。通过确定CTD的溶液结构获得了对RNA结合机制的深入了解,该结构显示采用一种新颖的折叠结构,由一个三链β折叠片层堆积在三个α螺旋上组成。CTD上的RNA结合表面已通过化学位移扰动实验定位,并且靠近先前显示对逆转录转座、RNA结合和伴侣活性至关重要的残基。由于编码中间、蛋白酶敏感片段和CTD的残基高度保守,预计所有脊椎动物长散在核元件1元件都具有相似的RNA结合结构和机制。

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