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马立克氏病病毒DNA复制起始位点的克隆、测序及功能分析

Cloning, sequencing, and functional analysis of a Marek's disease virus origin of DNA replication.

作者信息

Camp H S, Coussens P M, Silva R F

机构信息

Department of Animal Science, Michigan State University, East Lansing 48824.

出版信息

J Virol. 1991 Nov;65(11):6320-4. doi: 10.1128/JVI.65.11.6320-6324.1991.

Abstract

Previously, we isolated a replicon from a defective Marek's disease virus (MDV), analogous to defective herpes simplex viruses (amplicons). Defective viruses contain cis-acting elements required for DNA synthesis and virus propagation such as an origin of DNA replication and a packaging-cleavage signal site. In this report, the MDV replicon was utilized to locate an origin of MDV DNA replication. A comparison of MDV replicon sequences with other herpesvirus replication origin sequences revealed a 90-bp sequence containing 72% identity to the lytic origin (oris) of herpes simplex virus type 1. This 90-bp sequence displayed no similarity to betaherpesvirus or gammaherpesvirus replication origins. The 90-bp sequence is arranged as an imperfect palindrome centered around an A+T-rich region. This sequence also contains a 9-bp motif (5'CGTTCGCAC3') highly conserved in alphaherpesvirus replication origins. To test functionality of the 90-bp putative MDV replication origin, we conducted DpnI replication assays with subclones generated from the 4-kbp MDV replicon. A 700-bp MDV replicon subfragment containing the 90-bp putative MDV replication origin sequence is capable of replicating in chicken embryo fibroblast cells cotransfected with helper virus DNA. In conclusion, we identified a functional origin of DNA replication in MDV. Similarity of MDV origin sequences to those of alphaherpesviruses supports the current contention that MDV is more closely related to alphaherpesviruses than to gammaherpesviruses.

摘要

此前,我们从一种缺陷型马立克氏病病毒(MDV)中分离出一个复制子,类似于缺陷型单纯疱疹病毒(扩增子)。缺陷病毒含有DNA合成和病毒繁殖所需的顺式作用元件,如DNA复制起点和包装切割信号位点。在本报告中,MDV复制子被用于定位MDV DNA复制的起点。将MDV复制子序列与其他疱疹病毒复制起点序列进行比较,发现一个90 bp的序列,与1型单纯疱疹病毒的裂解起点(oris)有72%的同一性。这个90 bp的序列与β疱疹病毒或γ疱疹病毒的复制起点没有相似性。90 bp的序列以一个富含A+T的区域为中心排列成一个不完全回文结构。该序列还包含一个在α疱疹病毒复制起点中高度保守的9 bp基序(5'CGTTCGCAC3')。为了测试90 bp假定的MDV复制起点的功能,我们用从4 kbp MDV复制子产生的亚克隆进行了DpnI复制分析。一个包含90 bp假定的MDV复制起点序列的700 bp MDV复制子亚片段能够在与辅助病毒DNA共转染的鸡胚成纤维细胞中复制。总之,我们在MDV中鉴定出一个功能性的DNA复制起点。MDV起点序列与α疱疹病毒起点序列的相似性支持了目前的观点,即MDV与α疱疹病毒的关系比与γ疱疹病毒的关系更密切。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0f84/250344/6d647c973e37/jvirol00054-0680-a.jpg

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