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Rescue of Citrus sudden death‐associated virus in Nicotiana benthamiana plants from cloned cDNA: insights into mechanisms of expression of the three capsid proteins

机译:从克隆的cDNA中拯救本生烟草中的柑橘突然死亡相关病毒:三种衣壳蛋白表达机制的见解

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摘要

(CSDaV) is a member of the genus in the family , and has been associated with citrus sudden death (CSD) disease in Brazil. Difficulties in the purification of CSDaV from infected citrus plants have prevented progress in the investigation of the role of this virus in CSD and an understanding of its molecular biology. In this work, we have constructed a full‐length cDNA clone of CSDaV driven by the 35S promoter (35SRbz‐CSDaV). ‐mediated inoculation of 35SRbz‐CSDaV in plants enabled a fast recovery of large amounts of virions from the agroinfiltrated leaves, which allowed a better molecular characterization of CSDaV. analyses of mutant versions of 35SRbz‐CSDaV revealed the expression strategies used by CSDaV for production of the capsid proteins (CPs). We showed that CSDaV virions contain three forms of CP, each of which is generated from the same coding sequence, but by different mechanisms. The major CPp21 is a product of direct translation by leaky scanning from the second start codon in the subgenomic RNA (sgRNA), whereas the minor CPs, p25 and p23, are produced by direct translation from the first start codon in the sgRNA and by ‐proteolytic cleavage processing derived from the p25 precursor, respectively. Together, these findings contribute to advance our understanding of CSDaV genome expression strategies. In addition, the construction and characterization of the CSDaV infectious clone represent important steps towards the investigation of the role of this virus in CSD and of its use as a tool for citrus biotechnology.
机译:(CSDaV)是该家族的一员,在巴西与柑橘猝死(CSD)疾病有关。从受感染的柑橘类植物中纯化CSDaV的困难阻碍了该病毒在CSD中的作用研究及其分子生物学研究的进展。在这项工作中,我们构建了由35S启动子驱动的CSDaV的全长cDNA克隆(35SRbz-CSDaV)。介导的35SRbz-CSDaV在植物中的接种能够从农杆菌渗入的叶片中快速回收大量毒粒,从而使CSDaV具有更好的分子特征。对35SRbz-CSDaV突变体版本的分析揭示了CSDaV用于产生衣壳蛋白(CP)的表达策略。我们表明,CSDaV病毒体包含三种形式的CP,每种形式均由相同的编码序列产生,但机制不同。主要CPp21是通过从亚基因组RNA(sgRNA)的第二个起始密码子进行泄漏扫描而直接翻译的产物,而次要CPs(p25和p23)是通过从sgRNA的第一个起始密码子进行直接翻译而产生的-分别来自p25前体的蛋白水解切割过程。这些发现共同促进了我们对CSDaV基因组表达策略的理解。此外,CSDaV传染性克隆的构建和表征是研究该病毒在CSD中的作用及其作为柑橘生物技术工具的使用的重要步骤。

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