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工程改造并鉴定表达复制酶基因荧光报告蛋白的禽类冠状病毒突变株。

Engineering and Characterization of Avian Coronavirus Mutants Expressing Fluorescent Reporter Proteins from the Replicase Gene.

机构信息

Institut für Virologie, Freie Universität Berlin, Berlin, Germany.

National Veterinary Product Engineering Research Center, Jiangsu Academy of Agricultural Sciences, Nanjing, Jiangsu, China.

出版信息

J Virol. 2022 Jul 27;96(14):e0065322. doi: 10.1128/jvi.00653-22. Epub 2022 Jul 5.

Abstract

Infectious bronchitis virus (IBV) is an avian coronavirus that causes infectious bronchitis, an acute and highly contagious respiratory disease of chickens. IBV evolution under the pressure of comprehensive and widespread vaccination requires surveillance for vaccine resistance, as well as periodic vaccine updates. Reverse genetics systems are very valuable tools in virology, as they facilitate rapid genetic manipulation of viral genomes, thereby advancing basic and applied research. We report here the construction of an infectious clone of IBV strain Beaudette as a bacterial artificial chromosome (BAC). The engineered full-length IBV clone allowed the rescue of an infectious virus that was phenotypically indistinguishable from the parental virus. We used the infectious IBV clone and examined whether an enhanced green fluorescent protein (EGFP) can be produced by the replicase gene ORF1 and autocatalytically released from the replicase polyprotein through cleavage by the main coronavirus protease. We show that IBV tolerates insertion of the EGFP ORF at the 3' end of the replicase gene, between the sequences encoding nsp13 and nsp16 (helicase, RNA exonuclease, RNA endonuclease, and RNA methyltransferase). We further show that EGFP is efficiently cleaved from the replicase polyprotein and can be localized in double-membrane vesicles along with viral RNA polymerase and double-stranded RNA, an intermediate of IBV genome replication. One of the engineered reporter EGFP viruses were genetically stable during passage in cultured cells. We demonstrate that the reporter EGFP viruses can be used to study virus replication in host cells and for antiviral drug discovery and development of diagnostic assays. Reverse genetics systems based on bacterial artificial chromosomes (BACs) are the most valuable systems in coronavirus research. Here, we describe the establishment of a reverse genetics system for the avian coronavirus strain Beaudette, the most intensively studied strain. We cloned a copy of the avian coronavirus genome into a BAC vector and recovered infectious virus in permissive cells. We used the new system to construct reporter viruses that produce enhanced green fluorescent protein (EGFP). The EGFP coding sequence was inserted into 11 known cleavage sites of the major coronavirus protease in the replicase gene ORF1. Avian coronavirus tolerated the insertion of the EGFP coding sequence at three sites. The engineered reporter viruses replicated with parental efficiency in cultured cells and were sufficiently genetically stable. The new system facilitates functional genomics of the avian coronavirus genome but can also be used for the development of novel vaccines and anticoronaviral drugs.

摘要

传染性支气管炎病毒(IBV)是一种禽冠状病毒,可引起传染性支气管炎,这是一种急性且高度传染性的鸡呼吸道疾病。在全面广泛接种疫苗的压力下,IBV 的进化需要对疫苗抗性进行监测,同时还需要定期更新疫苗。反向遗传学系统是病毒学中非常有价值的工具,因为它们可以促进病毒基因组的快速遗传操作,从而推进基础和应用研究。我们在此报告构建了传染性支气管炎病毒 Beaudette 株的细菌人工染色体(BAC)感染性克隆。该工程全长 IBV 克隆允许拯救出表型与亲本病毒无法区分的传染性病毒。我们使用传染性 IBV 克隆并检查增强型绿色荧光蛋白(EGFP)是否可以由复制酶基因 ORF1 产生,并通过主要冠状病毒蛋白酶的切割从复制酶多蛋白中自动释放。我们表明,IBV 可以容忍 EGFP ORF 在复制酶基因的 3'末端插入,在编码 nsp13 和 nsp16(解旋酶、RNA 外切酶、RNA 内切酶和 RNA 甲基转移酶)的序列之间。我们进一步表明,EGFP 可以从复制酶多蛋白中有效切割,并可以与病毒 RNA 聚合酶和双链 RNA 一起定位于双膜囊泡中,这是 IBV 基因组复制的中间产物。在细胞培养中传代时,一种工程报告 EGFP 病毒具有遗传稳定性。我们证明,报告 EGFP 病毒可用于研究宿主细胞中的病毒复制以及抗病毒药物的发现和诊断测定的开发。基于细菌人工染色体(BAC)的反向遗传学系统是冠状病毒研究中最有价值的系统。在这里,我们描述了建立用于禽冠状病毒 Beaudette 株的反向遗传学系统的过程,该株是研究最深入的株。我们将禽冠状病毒基因组的一个副本克隆到 BAC 载体中,并在允许的细胞中恢复了传染性病毒。我们使用新系统构建了产生增强型绿色荧光蛋白(EGFP)的报告病毒。EGFP 编码序列插入到复制酶基因 ORF1 中的主要冠状病毒蛋白酶的 11 个已知切割位点之一。禽冠状病毒可耐受 EGFP 编码序列在三个位点的插入。工程报告病毒在细胞培养物中以与亲本相同的效率复制,并且遗传稳定性足够高。新系统促进了禽冠状病毒基因组的功能基因组学研究,但也可用于开发新型疫苗和抗冠状病毒药物。

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