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在表达假定病毒复制酶修饰成分的植物中对马铃薯X病毒感染具有极强抗性。

Extreme resistance to potato virus X infection in plants expressing a modified component of the putative viral replicase.

作者信息

Longstaff M, Brigneti G, Boccard F, Chapman S, Baulcombe D

机构信息

Sainsbury Laboratory, Norwich Research Park, UK.

出版信息

EMBO J. 1993 Feb;12(2):379-86. doi: 10.1002/j.1460-2075.1993.tb05669.x.

DOI:10.1002/j.1460-2075.1993.tb05669.x
PMID:8440232
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC413220/
Abstract

Three types of mutation were introduced into the sequence encoding the GDD motif of the putative replicase component of potato virus X (PVX). All three mutations rendered the viral genome completely noninfectious when inoculated into Nicotiana clevelandii or into protoplasts of Nicotiana tabacum (cv. Samsun NN). In order to test whether these negative mutations could inactivate the viral genome in trans, the mutant genes were expressed in transformed N.tabacum (cv. Samsun NN) under control of the 35S RNA promoter of cauliflower mosaic virus and the transformed lines were inoculated with PVX. In 10 lines tested in which the GDD motif was expressed as GAD or GED there was no effect on susceptibility to PVX. In two of four lines transformed to express the ADD form of the conserved motif, the F1 and F2 progeny plants were highly resistant to infection by PVX, although only to strains closely related to the source of the transgene. The resistance was associated with suppression of PVX accumulation in the inoculated and systemic leaves and in protoplasts of the transformed plants, although some low level viral RNA production was observed in the inoculated but not the systemic leaves when the inoculum was as high as 100 or 250 micrograms/ml PVX RNA. These results suggest for a plant virus, as reported previously for Q beta phage, that virus resistance may be engineered by expression of dominant negative mutant forms of viral genes in transformed cells.

摘要

将三种类型的突变引入到马铃薯X病毒(PVX)假定复制酶组分的GDD基序编码序列中。当接种到克利夫兰烟草或烟草(品种Samsun NN)原生质体中时,所有这三种突变均使病毒基因组完全无感染性。为了测试这些负向突变是否能在反式作用中使病毒基因组失活,将突变基因在花椰菜花叶病毒35S RNA启动子的控制下在转化的烟草(品种Samsun NN)中表达,并将转化株系接种PVX。在测试的10个株系中,其中GDD基序表达为GAD或GED,对PVX的易感性没有影响。在四个转化以表达保守基序ADD形式的株系中的两个中,F1和F2后代植株对PVX感染具有高度抗性,尽管仅对与转基因来源密切相关的毒株有抗性。抗性与PVX在接种叶和系统叶以及转化植物原生质体中的积累受到抑制有关,尽管当接种物中PVX RNA高达100或250微克/毫升时,在接种叶而非系统叶中观察到一些低水平的病毒RNA产生。这些结果表明,对于一种植物病毒,如先前对Qβ噬菌体所报道的那样,病毒抗性可以通过在转化细胞中表达病毒基因的显性负突变形式来构建。

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