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鹦鹉呼肠孤病毒 4 的反向遗传学研究揭示了糖蛋白基因的独特剪接,影响病毒的传播。

Reverse genetics of parrot bornavirus 4 reveals a unique splicing of the glycoprotein gene that affects viral propagation.

机构信息

Laboratory of RNA Viruses, Department of Virus Research, Institute for Life and Medical Sciences (LiMe), Kyoto University , Kyoto, Japan.

Laboratory of Microbiology, School of Veterinary Medicine, Azabu University , Kanagawa, Japan.

出版信息

J Virol. 2023 Aug 31;97(8):e0050923. doi: 10.1128/jvi.00509-23. Epub 2023 Aug 14.

Abstract

Viruses can utilize host splicing machinery to enable the expression of multiple genes from a limited-sized genome. Orthobornaviruses use alternative splicing to regulate the expression level of viral proteins and achieve efficient viral replication in the nucleus. Although more than 20 orthobornaviruses have been identified belonging to eight different viral species, virus-specific splicing has not been demonstrated. Here, we demonstrate that the glycoprotein (G) transcript of parrot bornavirus 4 (PaBV-4; species ), a highly virulent virus in psittacines, undergoes mRNA splicing and expresses a soluble isoform termed sGP. Interestingly, the splicing donor for sGP is not conserved in other orthobornaviruses, including those belonging to the same orthobornavirus species, suggesting that this splicing has evolved as a PaBV-4-specific event. We have also shown that exogenous expression of sGP does not affect PaBV-4 replication or virion infectivity. In this study, to investigate the role of sGP in viral replication, we established a reverse genetics system for PaBV-4 by using avian cell lines and generated a recombinant virus lacking the spliced mRNA for sGP. Using the recombinant viruses, we show that the replication of the sGP-deficient virus is significantly slower than that of the wild-type virus and that the exogenous expression of sGP cannot restore its propagation efficiency. These results suggest that autologous or controlled expression of sGP by splicing may be important for PaBV-4 propagation. The reverse genetics system for avian bornaviruses developed here will be a powerful tool for understanding the replication strategies and pathogenesis of avian orthobornaviruses. IMPORTANCE Parrot bornavirus 4 (PaBV-4) is the dominant cause of proventricular dilatation disease, a severe gastrointestinal and central nervous system disease among avian bornaviruses. In this study, we discovered that PaBV-4 expresses a soluble isoform of glycoprotein (G), called sGP, through alternative splicing of the G mRNA, which is unique to this virus. To understand the role of sGP in viral replication, we generated recombinant PaBV-4 lacking the newly identified splicing donor site for sGP using a reverse genetics system and found that its propagation was significantly slower than that of the wild-type virus, suggesting that sGP plays an essential role in PaBV-4 infection. Our results provide important insights not only into the replication strategy but also into the pathogenesis of PaBV-4, which is the most prevalent bornavirus in captive psittacines worldwide.

摘要

病毒可以利用宿主剪接机制来实现从有限大小的基因组中表达多个基因。正粘病毒通过选择性剪接来调节病毒蛋白的表达水平,从而在细胞核中实现高效的病毒复制。尽管已经鉴定出超过 20 种正粘病毒,属于八个不同的病毒种,但尚未证明病毒特异性剪接的存在。在这里,我们证明了鹦鹉博尔纳病毒 4(PaBV-4;种)的糖蛋白(G)转录本发生 mRNA 剪接,并表达一种称为 sGP 的可溶性同工型。有趣的是,sGP 的剪接供体在其他正粘病毒中并不保守,包括属于同一正粘病毒种的病毒,这表明这种剪接是 PaBV-4 特有的事件。我们还表明,sGP 的外源性表达不会影响 PaBV-4 的复制或病毒粒子的感染力。在这项研究中,为了研究 sGP 在病毒复制中的作用,我们使用禽细胞系建立了 PaBV-4 的反向遗传学系统,并生成了一种缺乏剪接的 sGP 信使 RNA 的重组病毒。使用重组病毒,我们表明,sGP 缺失病毒的复制速度明显慢于野生型病毒,并且 sGP 的外源性表达不能恢复其繁殖效率。这些结果表明,sGP 的自体或受控剪接表达可能对 PaBV-4 的繁殖很重要。这里开发的禽正粘病毒反向遗传学系统将成为理解禽正粘病毒复制策略和发病机制的有力工具。重要性鹦鹉博尔纳病毒 4(PaBV-4)是导致前胃扩张病的主要原因,该病是一种严重的胃肠道和中枢神经系统疾病,在禽正粘病毒中普遍存在。在这项研究中,我们发现 PaBV-4 通过 G mRNA 的选择性剪接表达一种可溶性糖蛋白(G)同工型,称为 sGP,这是该病毒特有的。为了了解 sGP 在病毒复制中的作用,我们使用反向遗传学系统生成了缺乏新鉴定的 sGP 剪接供体位点的重组 PaBV-4,并发现其繁殖速度明显慢于野生型病毒,表明 sGP 在 PaBV-4 感染中发挥重要作用。我们的研究结果不仅为病毒复制策略提供了重要的见解,也为 PaBV-4 的发病机制提供了重要的见解,因为 PaBV-4 是全世界圈养鹦鹉中最普遍的博尔纳病毒。

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