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转基因或植物表达载体介导的李痘病毒重组

Transgenic or plant expression vector-mediated recombination of Plum Pox Virus.

作者信息

Varrelmann M, Palkovics L, Maiss E

机构信息

Institute of Plant Diseases and Plant Protection, University of Hannover, 30419 Hanover, Germany.

出版信息

J Virol. 2000 Aug;74(16):7462-9. doi: 10.1128/jvi.74.16.7462-7469.2000.

Abstract

Different mutants of an infectious full-length clone (p35PPV-NAT) of Plum pox virus (PPV) were constructed: three mutants with mutations of the assembly motifs RQ and DF in the coat protein gene (CP) and two CP chimeras with exchanges in the CP core region of Zucchini yellow mosaic virus and Potato virus Y. The assembly mutants were restricted to single infected cells, whereas the PPV chimeras were able to produce systemic infections in Nicotiana benthamiana plants. After passages in different transgenic N. benthamiana plants expressing the PPV CP gene with a complete (plant line 4.30.45.) or partially deleted 3'-nontranslated region (3'-NTR) (plant line 17.27. 4.), characterization of the viral progeny of all mutants revealed restoration of wild-type virus by recombination with the transgenic CP RNA only in the presence of the complete 3'-NTR (4.30.45.). Reconstitution of wild-type virus was also observed following cobombardment of different assembly-defective p35PPV-NAT together with a movement-defective plant expression vector of Potato virus X expressing the intact PPV-NAT CP gene transiently in nontransgenic N. benthamiana plants. Finally, a chimeric recombinant virus was detected after cobombardment of defective p35PPV-NAT with a plant expression vector-derived CP gene from the sour cherry isolate of PPV (PPV-SoC). This chimeric virus has been established by a double recombination event between the CP-defective PPV mutant and the intact PPV-SoC CP gene. These results demonstrate that viral sequences can be tested for recombination events without the necessity for producing transgenic plants.

摘要

构建了李痘病毒(PPV)感染性全长克隆(p35PPV-NAT)的不同突变体:三个在外壳蛋白基因(CP)中具有组装基序RQ和DF突变的突变体,以及两个在西葫芦黄花叶病毒和马铃薯Y病毒CP核心区域进行交换的CP嵌合体。组装突变体局限于单个感染细胞,而PPV嵌合体能够在本氏烟草植株中产生系统感染。在不同的表达具有完整(株系4.30.45)或部分缺失3'-非翻译区(3'-NTR)(株系17.27.4)的PPV CP基因的转基因本氏烟草植株中传代后,对所有突变体病毒后代的表征显示,仅在存在完整3'-NTR(4.30.45)的情况下,通过与转基因CP RNA重组才能恢复野生型病毒。在非转基因本氏烟草植株中,将不同的组装缺陷型p35PPV-NAT与瞬时表达完整PPV-NAT CP基因的马铃薯X病毒运动缺陷型植物表达载体共轰击后,也观察到了野生型病毒的重建。最后,在用来自酸樱桃分离株PPV(PPV-SoC)的植物表达载体衍生的CP基因对缺陷型p35PPV-NAT进行共轰击后,检测到了一种嵌合重组病毒。这种嵌合病毒是由CP缺陷型PPV突变体与完整的PPV-SoC CP基因之间的双重组事件形成的。这些结果表明,无需生产转基因植物即可检测病毒序列的重组事件。

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