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Construction of an infectious clone of Zika virus stably expressing an EGFP marker in a eukaryotic expression system

机译:在真核表达系统中稳定地表达EGFP标记的Zika病毒的传染性克隆的构建

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摘要

Zika virus is becoming one of the most widely transmitted arboviruses in the world. Development of antiviral inhibitor and vaccine requires an experimental system that allows rapid monitoring of the virus infection. This is achievable with a reverse genetic system. In this study, we constructed an infectious clone for Zika virus that stably expressing EGFP. A PCR-mediated recombination approach was used to assemble the full-length Zika virus genome containing the CMV promoter, intron, EGFP, hepatitis delta virus ribozyme, and SV40 terminator sequence for cloning into the pBAC11 vector to produce recombinant pBAC-ZIKA-EGFP. ZIKA-EGFP virus?was rescued by transfection of pBAC-ZIKA-EGFP into 293T cells. The characterization of ZIKA-EGFP virus was determined by qPCR, plaque assay, CCK-8, and Western blot. Rescued ZIKA-EGFP virus exhibited stable replication for at least five generations in tissue culture. ZIKA-EGFP can effectively infect C6/36, SH-SY5Y and Vero cells, and cause cytopathic effects on SH-SY5Y and Vero cells. The inhibition of ZIKA-EGFP by NF-κB inhibitor, caffeic acid phenethyl ester was observed by fluorescence microscopy. Our results suggested that Zika virus infectious clone with an EGFP marker retained it infectivity as wide-type Zika virus which could be used for drugs screening.
机译:Zika病毒正在成为世界上最广泛传播的野生术之一。抗病毒抑制剂和疫苗的发展需要一种实验系统,可以快速监测病毒感染。这是通过反向遗传系统实现的。在这项研究中,我们构建了一种稳定表达EGFP的Zika病毒的传染性克隆。使用PCR介导的重组方法来组装含有CMV启动子,内含子,EGFP,肝炎δ病毒核酶和SV40终止子序列的全长Zika病毒基因组,用于克隆到PBAC11载体中以产生重组PBAC-ZIKA-EGFP。 Zika-EGFP病毒?通过将PBAC-ZIKA-EGFP转染到293T细胞中来拯救。 Zika-EGFP病毒的表征由QPCR,斑块测定,CCK-8和Western印迹测定。获救的Zika-EGFP病毒在组织培养中表现出至少五代的稳定复制。 Zika-EGFP可以有效地感染C6 / 36,SH-SY5Y和VERO细胞,并对SH-SY5Y和VERO细胞引起细胞病变作用。通过NF-κB抑制剂抑制Zika-EGFP,通过荧光显微镜观察咖啡酸苯乙基酯。我们的结果表明,Zika病毒传染性克隆与EGFP标记物保留了IT感染性,作为宽型Zika病毒,可用于药物筛选。

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