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杆状病毒介导的转导:水疱性口炎病毒糖蛋白假型化分析

Baculovirus mediated transduction: analysis of vesicular stomatitis virus glycoprotein pseudotyping.

作者信息

Kolangath Sujit M, Basagoudanavar S H, Hosamani M, Saravanan P, Tamil Selvan R P

机构信息

ICAR-Indian Veterinary Research Institute, Hebbal, Bangalore, 560 024 India.

出版信息

Virusdisease. 2014 Dec;25(4):441-6. doi: 10.1007/s13337-014-0229-5. Epub 2014 Oct 11.

Abstract

The recombinant baculoviruses were constructed to investigate the necessity of VSV-G pseudotyping for mammalian cell transduction. The viruses were designed to express green fluorescent protein (GFP) gene under the control of cytomegalovirus promoter, with or without pseudotyping with VSV-G. VSV-G was placed under the control of polyhedrin promoter that is recognized by insect cells, allowing the formation of pseudotyped baculovirus. The study findings demonstrate that the pseudotyping of baculovirus significantly enhanced transduction efficiency compared to non-pseudotyped baculovirus, resulting in consequent distinction in the expression of GFP in mammalian cells. The results confirmed that pseudotyping is important for baculovirus mediated gene delivery. Further, when full-length VSV-G pseudotyping was compared with truncated VSV-G containing GED domain (G-stem of ectodomain in conjunction with the TM and CT domains of the glycoprotein), latter was relatively less efficient in transducing mammalian cells. This study demonstrated that pseudotyping with full-length VSV-G had better transduction efficiency in mammalian cells. However, at higher multiplicity of infection, both full-length and truncated VSV-G showed equivalent transduction. This study established the significance of pseudotyping of baculovirus with full-length VSV-G for efficient transduction of mammalian cells, utilizing the highly sensitive GFP marker system. These findings have significant implications in designing of baculovirus vector based antigen delivery for developing new generation vaccines.

摘要

构建重组杆状病毒以研究水疱性口炎病毒糖蛋白(VSV-G)假型化对哺乳动物细胞转导的必要性。这些病毒被设计为在巨细胞病毒启动子的控制下表达绿色荧光蛋白(GFP)基因,有或没有VSV-G假型化。VSV-G置于昆虫细胞识别的多角体蛋白启动子的控制下,从而允许形成假型化杆状病毒。研究结果表明,与非假型化杆状病毒相比,杆状病毒的假型化显著提高了转导效率,导致哺乳动物细胞中GFP表达出现明显差异。结果证实假型化对于杆状病毒介导的基因递送很重要。此外,当将全长VSV-G假型化与含有GED结构域(糖蛋白胞外结构域的G-茎与跨膜结构域和胞质尾结构域结合)的截短型VSV-G进行比较时,后者在转导哺乳动物细胞方面效率相对较低。这项研究表明,全长VSV-G假型化在哺乳动物细胞中具有更好的转导效率。然而,在较高的感染复数下,全长和截短型VSV-G都显示出等效的转导。这项研究利用高度敏感的GFP标记系统确立了用全长VSV-G对杆状病毒进行假型化对于高效转导哺乳动物细胞的重要性。这些发现对于设计基于杆状病毒载体的抗原递送以开发新一代疫苗具有重要意义。

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