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双生病毒 rep 基因突变体对 DNA 复制的反式显性抑制作用。

trans-Dominant Inhibition of Geminiviral DNA Replication by Bean Golden Mosaic Geminivirus rep Gene Mutants.

出版信息

Phytopathology. 1999 Jun;89(6):480-6. doi: 10.1094/PHYTO.1999.89.6.480.

Abstract

ABSTRACT Geminiviruses are a group of single-stranded DNA viruses that cause major losses on a number of important crops throughout the world. Bean golden mosaic virus (BGMV) is a typical bipartite, whitefly-transmitted geminivirus that causes a severe disease on beans (Phaseolus vulgaris) in the Western Hemisphere. The lack of natural resistance to geminiviruses has led to attempts to engineer resistance, particularly through the use of pathogen-derived resistance strategies. The rep gene contains several conserved domains including nucleoside triphosphate (NTP)-binding and DNA-nicking domains and is the only geminiviral gene necessary for replication. Previous analysis by our group and others has demonstrated that the NTP-binding and DNA-nicking domains are necessary for geminiviral DNA replication. The ability of the rep gene and rep gene mutants to interfere with geminiviral DNA replication, when expressed in trans, was examined using a transient assay in a tobacco suspension cell culture system. Wild-type (wt) and mutant rep genes were cloned into plasmids under the control of the cauliflower mosaic virus 35S promoter for in planta expression and coinoculated into tobacco cells with infectious clones of various geminiviruses. The wt rep gene from BGMV-GA was able to support replication of BGMV-GA DNA-B. Several different rep gene mutants, with function-abolishing mutations in the NTP-binding or DNA-nicking domains, were potent trans-dominant inhibitors of geminiviral DNA replication.

摘要

摘要 双生病毒是一类单链 DNA 病毒,它们会导致全球许多重要作物的重大损失。豆金色花叶病毒(BGMV)是一种典型的二分体、粉虱传播的双生病毒,在西半球会导致豆类(菜豆)严重发病。由于缺乏对双生病毒的天然抗性,人们试图通过利用病原体衍生的抗性策略来进行基因工程抗性改造。Rep 基因包含几个保守结构域,包括核苷三磷酸(NTP)结合和 DNA 切口结构域,是双生病毒复制所必需的唯一基因。本研究小组和其他研究小组的先前分析表明,NTP 结合和 DNA 切口结构域对于双生病毒 DNA 复制是必需的。通过在烟草悬浮细胞培养系统中的瞬时测定,研究了 Rep 基因和 Rep 基因突变体在转译时干扰双生病毒 DNA 复制的能力。wt 和突变 rep 基因被克隆到受花椰菜花叶病毒 35S 启动子控制的质粒中,用于体内表达,并与各种双生病毒的传染性克隆共接种到烟草细胞中。BGMV-GA 的 wt Rep 基因能够支持 BGMV-GA DNA-B 的复制。几个具有 NTP 结合或 DNA 切口结构域功能丧失突变的不同 Rep 基因突变体,是双生病毒 DNA 复制的有效转录显性抑制剂。

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