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在轻度酸性pH条件下生产基于逆转录病毒的载体。

Production of Retrovirus-Based Vectors in Mildly Acidic pH Conditions.

作者信息

Holic Nathalie, Fenard David

机构信息

Généthon, 91002, Evry, France.

INSERM, UMR_S951, Généthon, 1bis, rue de l'Internationale-BP60, 91002, Evry, France.

出版信息

Methods Mol Biol. 2016;1448:41-8. doi: 10.1007/978-1-4939-3753-0_3.

Abstract

Gene transfer vectors based on retroviridae are increasingly becoming a tool of choice for biomedical research and for the development of biotherapies in rare diseases or cancers. To meet the challenges of preclinical and clinical production, different steps of the production process of self-inactivating γ-retroviral (RVs) and lentiviral vectors (LVs) have been improved (e.g., transfection, media optimization, cell culture conditions). However, the increasing need for mass production of such vectors is still a challenge and could hamper their availability for therapeutic use. Recently, we observed that the use of a neutral pH during vector production is not optimal. The use of mildly acidic pH conditions (pH 6) can increase by two- to threefold the production of RVs and LVs pseudotyped with the vesicular stomatitis virus G (VSV-G) or gibbon ape leukemia virus (GALV) glycoproteins. Here, we describe the production protocol in mildly acidic pH conditions of GALVTR- and VSV-G-pseudotyped LVs using the transient transfection of HEK293T cells and the production protocol of GALV-pseudotyped RVs produced from a murine producer cell line. These protocols should help to achieve higher titers of vectors, thereby facilitating experimental research and therapeutic applications.

摘要

基于逆转录病毒科的基因转移载体正日益成为生物医学研究以及罕见病或癌症生物疗法开发的首选工具。为应对临床前和临床生产的挑战,自失活γ-逆转录病毒(RVs)和慢病毒载体(LVs)生产过程的不同步骤已得到改进(例如,转染、培养基优化、细胞培养条件)。然而,大规模生产此类载体的需求不断增加仍是一项挑战,可能会阻碍其用于治疗用途。最近,我们观察到在载体生产过程中使用中性pH并非最佳选择。使用轻度酸性pH条件(pH 6)可使以水疱性口炎病毒G(VSV-G)或长臂猿白血病病毒(GALV)糖蛋白假型化的RVs和LVs的产量提高两到三倍。在此,我们描述了使用HEK293T细胞瞬时转染在轻度酸性pH条件下生产GALVTR和VSV-G假型化LVs的方案,以及从小鼠生产细胞系生产GALV假型化RVs的方案。这些方案应有助于实现更高的载体滴度,从而促进实验研究和治疗应用。

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