Hsieh D J, Camiolo S M, Yates J L
Department of Human Genetics, Roswell Park Cancer Institute, Buffalo, NY 14263.
EMBO J. 1993 Dec 15;12(13):4933-44. doi: 10.1002/j.1460-2075.1993.tb06187.x.
Replication of the circular, 170 kb genome of Epstein-Barr virus (EBV) during latent infection is performed by the cellular replication machinery under cell-cycle control. A single viral protein, EBNA1, directs the cellular replication apparatus to initiate replication within the genetically defined replication origin, oriP, at a cluster of four EBNA1 binding sites, referred to here as the physical origin of bidirectional replication, or OBR. A second cluster of EBNA1 binding sites within oriP, the 30 bp repeats, serves an essential role as a replication enhancer and also provides a distinct episome maintenance function that is unrelated to replication. We examined the functional elements of oriP for binding by EBNA1 and possibly other proteins in proliferating Raji cells by generating in vivo footprints using two reagents, dimethylsulfate (DMS) and KMnO4. We also employed deoxyribonuclease I (DNase I) with permeabilized cells. The in vivo and permeabilized cell footprints at the EBNA1 binding sites, particularly those obtained using DMS, gave strong evidence that all of these sites are bound by EBNA1 in asynchronously dividing cells. No consistent evidence was found to suggest binding by other proteins at any other sites within the functional regions of oriP. Thymines at symmetrical positions of the OBR within oriP were oxidized when cells were treated with permanganate, suggestive of bends or other distortions of DNA structure at these positions; binding of EBNA1 in vitro to total DNA from Raji cells induced reactivity to permanganate at identical positions. The simplest interpretation of the results, which were obtained using asynchronously dividing cells, is that EBNA1 binds to its sites at oriP and holds the OBR in a distorted conformation throughout most of the cell cycle, implying that replication is initiated by a cellular mechanism and is not limited by an availability of EBNA1 for binding to oriP.
在潜伏感染期间,爱泼斯坦-巴尔病毒(EBV)170 kb的环状基因组的复制由处于细胞周期控制下的细胞复制机制完成。单个病毒蛋白EBNA1引导细胞复制装置在基因定义的复制起点oriP内起始复制,oriP位于四个EBNA1结合位点的簇处,此处称为双向复制的物理起点,即OBR。oriP内的第二簇EBNA1结合位点,即30 bp重复序列,作为复制增强子发挥重要作用,并且还提供与复制无关的独特附加体维持功能。我们通过使用两种试剂硫酸二甲酯(DMS)和高锰酸钾在体内产生足迹,研究了oriP的功能元件与增殖的Raji细胞中EBNA1以及可能的其他蛋白质的结合情况。我们还对透化细胞使用了脱氧核糖核酸酶I(DNase I)。EBNA1结合位点处的体内和透化细胞足迹,特别是使用DMS获得的足迹,有力地证明了所有这些位点在异步分裂细胞中都被EBNA1结合。没有发现一致的证据表明在oriP功能区域内的任何其他位点有其他蛋白质结合。当用高锰酸盐处理细胞时,oriP内OBR对称位置的胸腺嘧啶被氧化,表明这些位置的DNA结构存在弯曲或其他扭曲;EBNA1在体外与Raji细胞的总DNA结合会在相同位置诱导对高锰酸盐的反应性。使用异步分裂细胞获得的结果的最简单解释是,EBNA1在oriP处与其位点结合,并在细胞周期的大部分时间内将OBR保持在扭曲的构象中,这意味着复制是由细胞机制启动的,并且不受EBNA1与oriP结合可用性的限制。
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