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菜豆金色花叶双生病毒复制相关蛋白(AC1)中假定的NTP结合结构域的突变分析

Mutational analysis of a putative NTP-binding domain in the replication-associated protein (AC1) of bean golden mosaic geminivirus.

作者信息

Hanson S F, Hoogstraten R A, Ahlquist P, Gilbertson R L, Russell D R, Maxwell D P

机构信息

Department of Plant Pathology, University of Wisconsin-Madison 53706, USA.

出版信息

Virology. 1995 Aug 1;211(1):1-9. doi: 10.1006/viro.1995.1373.

Abstract

Bean golden mosaic virus (BGMV) is a whitefly-transmitted, ssDNA geminivirus with a bipartite genome. AC1 is the only ORF required for geminiviral replication. A putative NTP-binding motif, EGX4GKTX32DD, was present in the derived amino acid sequence of the replication-associated protein from the AC1 ORF for 13 geminiviruses including BGMV-GA (Guatemalan isolate, amino acids 221-263). We analyzed the phenotypes of mutations within this domain using a rapid and sensitive PCR-based assay for geminiviral replication developed for these studies. Replication in tobacco cells (NT-1 suspension cells) and infection of beans were abolished when codons were changed from K228 to H or D262 to R within the putative NTP-binding site. A temperature-sensitive replication phenotype was conferred by changing E221 to R within the putative NTP-binding domain. Replication was unaffected by changing a nonconserved codon near the putative NTP-binding domain from 1190 to R. Our results demonstrate that the putative NTP-binding domain is required for geminiviral replication. The role of NTP hydrolysis and the possible value of these mutants in a trans-dominant interference scheme for virus-derived resistance are discussed.

摘要

菜豆金色花叶病毒(BGMV)是一种由粉虱传播的单链DNA双生病毒,具有双分体基因组。AC1是双生病毒复制所需的唯一开放阅读框。在包括BGMV - GA(危地马拉分离株,氨基酸221 - 263)在内的13种双生病毒的AC1开放阅读框的复制相关蛋白的推导氨基酸序列中,存在一个推定的NTP结合基序EGX4GKTX32DD。我们使用为这些研究开发的一种基于PCR的快速灵敏的双生病毒复制检测方法,分析了该结构域内突变的表型。当推定的NTP结合位点内的密码子从K228变为H或D262变为R时,烟草细胞(NT - 1悬浮细胞)中的复制和菜豆的感染被消除。通过将推定的NTP结合结构域内的E221变为R赋予了温度敏感的复制表型。将推定的NTP结合结构域附近的一个非保守密码子从1190变为R对复制没有影响。我们的结果表明,推定的NTP结合结构域是双生病毒复制所必需的。讨论了NTP水解的作用以及这些突变体在病毒衍生抗性的反式显性干扰策略中的可能价值。

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