Analysis of Subcellular Localization and Pathogenicity of Plum Bark Necrosis Stem-Pitting Associated Virus Protein P6

Pub Date : 2023-01-01 DOI:10.32604/phyton.2023.028237
Yuanyuan Li, Jinze Mu, Qingliang Li, Huabing Liu, Xuefeng Yuan, Deya Wang
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Abstract

Infection of plum bark necrosis stem pitting associated virus (PBNSPaV) has been reported in many prunus species in several countries, causing signi�cant economic losses. The very small proteins encoded by plant viruses are often overlooked due to their short sequences and uncertain signi�cance. However, numerous studies have indicated that they might play important roles in the pathogenesis of virus infection. The role of small hydrophobic protein P6, encoded by the open reading frame 2 of PBNSPaV, has not been well explored. In this study, we ampli�ed the P6 fragment from a PBNSPaV isolate by RT-PCR using speci�c primers and found that it is 174 bp long and encodes a protein of approximately 6.3 kD with a transmembrane domain. Subcellular localization analysis of P6 proteins in tobacco leaves showed that P6 localizes in cytomembrane and nuclear membrane. To further clarify the pathogenicity of P6 proteins, a PVX-P6 expression vector was constructed by inserting the p6 fragment into a potato virus X (PVX)-based vector and transformed into Agrobacterium tumefaciens GV3101. In�ltration of N. benthamiana with the PVX vector-transformed A. tumefaciens led to slight mosaic symptoms at 14 days of post-inoculation. Meanwhile, in�ltration with the PVX-P6 vector-transformed A. tumefaciens resulted in no signi�cant symptoms. These results demonstrated that heterologous expression of P6 in N. benthamiana could not enhance the pathogenicity of PVX. Our study indicates that p6 may not be a potential pathogenic factor associate with the causing of symptoms, and mode of action of PBNSPaV-P6 protein remain to be further studied.
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李树树皮坏死茎蚀相关病毒蛋白P6亚细胞定位及致病性分析
李树树皮坏死茎蚀相关病毒(PBNSPaV)在一些国家的许多李树品种中都有报道,造成了重大的经济损失。植物病毒所编码的非常小的蛋白质由于序列短、意义不确定而经常被忽视。然而,大量研究表明,它们可能在病毒感染的发病机制中发挥重要作用。PBNSPaV开放阅读框2编码的小疏水蛋白P6的作用尚未得到很好的探索。在这项研究中,我们利用特异性引物,用RT-PCR扩增了PBNSPaV分离物的P6片段,发现它长174 bp,编码一个约6.3 kD的蛋白,具有跨膜结构域。烟草叶片P6蛋白亚细胞定位分析表明,P6蛋白定位于细胞膜和核膜。为了进一步明确P6蛋白的致病性,将P6片段插入马铃薯病毒X (PVX)载体,构建PVX-P6表达载体,并转化为农杆菌GV3101。接种后14天,用PVX载体转化的瘤胃拟南芽胞杆菌浸渍本拟南芽胞杆菌可引起轻微的花叶症状。与此同时,PVX-P6载体转化的瘤化假单胞菌未引起明显症状。这些结果表明,P6在benthamiana中的异源表达不能增强PVX的致病性。我们的研究提示p6可能不是引起症状的潜在致病因素,PBNSPaV-P6蛋白的作用方式有待进一步研究。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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