Protocol for a high titer of BaEV-Rless pseudotyped lentiviral vector: Focus on syncytium formation and detachment

生物 效价 转染 病毒学 合胞体 细胞培养 分子生物学 病毒 宽容 遗传增强 病毒复制 基因 遗传学
作者
Kazuhiro Noguchi,Yasuhiro Ikawa,Mika Takenaka,Yuta Sakai,Toshihiro Fujiki,Rie Kuroda,Matthew N. Chappell,Valentina Ghiaccio,Stefano Rivella,Taizo Wada
出处
期刊:Journal of Virological Methods [Elsevier]
卷期号:314: 114689-114689
标识
DOI:10.1016/j.jviromet.2023.114689
摘要

The development of hematopoietic stem cell (HSCs) gene therapy for DNA repair disorders, such as Fanconi anemia and Bloom syndrome, is challenging because of the induction of HSCs apoptosis by cytokine stimulation. Although the Baboon envelope pseudotyped lentiviral vector (BaEV-Rless-LV) has been reported as a non-stimulatory gene transfer tool, the virus titer of BaEV-Rless-LV is too low for use in clinical applications. Transfected 293 T cells with helper plasmids, including the BaEV-Rless plasmid, showed morphological changes, such as syncytium formation and detachment. To establish a novel protocol for producing a high titer of BaEV-Rless-LV, we optimized three aspects of a basic virus production protocol by focusing on modifying culture conditions and the use of reagents: the virus titer increased 3-fold when the amount of BaEV-Rless plasmid was increased 1.2-fold; the highest titer was obtained when the viral supernatant was harvested at 48-h post-transfection, despite complete syncytium formation and detachment of the 293 T cells; and the use of poly-L-lysine-coated culture plates to enhance the adhesion and proliferation of 293 T cells and prevent detachment doubled the titer. Collectively, our novel protocol resulted in a 10-fold titer increase compared to the basic protocol and may be useful in clinical applications for treating DNA repair disorders.
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