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爱泼斯坦-巴尔病毒的串联体复制:病毒产生细胞系和新转化细胞系中末端的结构

Concatameric replication of Epstein-Barr virus: structure of the termini in virus-producer and newly transformed cell lines.

作者信息

Sato H, Takimoto T, Tanaka S, Tanaka J, Raab-Traub N

机构信息

Department of Microbiology and Immunology, School of Medicine, University of North Carolina, Chapel Hill 27599-7295.

出版信息

J Virol. 1990 Nov;64(11):5295-300. doi: 10.1128/JVI.64.11.5295-5300.1990.

Abstract

The linear form of Epstein-Barr virus (EBV) DNA has homologous direct tandem repeats of approximately 500 bp at each terminus (TR). After infection, EBV DNA circularizes via the TR to form the intracellular episomal DNA. To analyze the mechanism of the synthesis of linear DNA through possible replicative intermediates, the terminal fragments were identified in the total intracellular DNA and the covalently closed circular DNA from a productively infected cell line after induction of replication or after treatment with an inhibitor of viral DNA synthesis. These studies indicate that some of the fused terminal fragments detected in the total intracellular DNA are replication-dependent forms which are selectively excluded from the covalently closed circular fraction and are eliminated after treatment with acyclovir. The EBV terminal restriction enzyme fragments were identified in three producer cell lines, each with a characteristic number of TR in the intracellular episomal DNA. Identification of the termini in cell lines established with the three virus strains revealed that the newly transformed cell lines had a greater number of TR than did the template DNA in the producer cell line. The increase in the number of TR in progeny episomes indicates that linear DNA is produced from concatameric replicative intermediates rather than from amplified catenated circular intermediates.

摘要

爱泼斯坦-巴尔病毒(EBV)DNA的线性形式在每个末端(TR)具有约500 bp的同源直接串联重复序列。感染后,EBV DNA通过TR环化形成细胞内游离型DNA。为了通过可能的复制中间体分析线性DNA的合成机制,在诱导复制后或用病毒DNA合成抑制剂处理后,从高效感染的细胞系的总细胞内DNA和共价闭合环状DNA中鉴定末端片段。这些研究表明,在总细胞内DNA中检测到的一些融合末端片段是复制依赖性形式,它们被选择性地排除在共价闭合环状部分之外,并在用阿昔洛韦处理后被消除。在三个产生细胞系中鉴定了EBV末端限制酶片段,每个细胞系在细胞内游离型DNA中具有特征性数量的TR。在用三种病毒株建立的细胞系中对末端的鉴定表明,新转化的细胞系比产生细胞系中的模板DNA具有更多的TR。子代游离型中TR数量的增加表明线性DNA是由串联复制中间体产生的,而不是由扩增的连环环状中间体产生的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ac43/248575/0a95fab9d9ca/jvirol00066-0075-a.jpg

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