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在Sf9昆虫细胞中通过φC31介导的盒式交换实现稳定表达。

φC31 -Mediated cassette exchange in Sf9 insect cells for stable expression.

作者信息

Hu Die, Qian Jingwen, Zhang Tong, Yu Yue, Xu Zhenhe, Zhang Yuanxing, Liu Qin

机构信息

State Key Laboratory of Bioreactor Engineering, Shanghai Frontiers Science Center of Optogenetic Techniques for Cell Metabolism, East China University of Science and Technology, Shanghai, China.

Shanghai Collaborative Innovation Center for Biomanufacturing, Shanghai, China.

出版信息

Biotechnol J. 2023 Jul;18(7):e2200557. doi: 10.1002/biot.202200557. Epub 2023 Apr 28.

Abstract

Insect cells, especially Sf9 cells, are commonly used in biomanufacturing due to their advantages in high expression levels and post-translational modification. However, the development of stable expression cell lines via random integration tended to be unstable. Site-specific integration (SSI) is an alternative strategy. In this study, a φC31 -mediated cassette exchange system in Sf9 cells was established for SSI. The tagging cassette with the reporter gene egfp was randomly inserted into the cell genome. Potential platform cell lines were obtained by fluorescence-activated cell sorting (FACS) and single-cell cloning. Platform cell lines were selected by assessing the fluorescence expression, stability, and growth kinetics of cell lines. The selected platform cell lines were co-transfected with the φC31-containing plasmid and the targeting cassette. Green-fluorescence-negative clones were screened by hygromycin resistance and FACS. The resulting cell clones exhibited the expression properties of the platform cell lines. The rapid development of cell lines for the production of influenza subunit vaccines by the cassette exchange system demonstrated that the system constituted a versatile and reusable platform for the production of various recombinant proteins. Overall, the φC31-mediated cassette exchange system in Sf9 cells has the potential to facilitate and accelerate biologics development.

摘要

昆虫细胞,尤其是Sf9细胞,因其在高表达水平和翻译后修饰方面的优势而常用于生物制造。然而,通过随机整合开发稳定表达细胞系往往不稳定。位点特异性整合(SSI)是一种替代策略。在本研究中,为实现SSI在Sf9细胞中建立了一种φC31介导的盒式交换系统。将带有报告基因egfp的标签盒随机插入细胞基因组。通过荧光激活细胞分选(FACS)和单细胞克隆获得潜在的平台细胞系。通过评估细胞系的荧光表达、稳定性和生长动力学来选择平台细胞系。将所选的平台细胞系与含φC31的质粒和靶向盒共转染。通过潮霉素抗性和FACS筛选绿色荧光阴性克隆。所得细胞克隆表现出平台细胞系的表达特性。通过盒式交换系统快速开发用于生产流感亚单位疫苗的细胞系表明,该系统构成了一个用于生产各种重组蛋白的通用且可重复使用的平台。总体而言,Sf9细胞中φC31介导的盒式交换系统有潜力促进和加速生物制品的开发。

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