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慢病毒载体的生产。

Production of lentiviral vectors.

机构信息

Généthon , Evry-Cedex, France.

New Technologies Unit, Research Division, MolMed S.p.A. , Milan, Italy.

出版信息

Mol Ther Methods Clin Dev. 2016 Apr 13;3:16017. doi: 10.1038/mtm.2016.17. eCollection 2016.

Abstract

Lentiviral vectors (LV) have seen considerably increase in use as gene therapy vectors for the treatment of acquired and inherited diseases. This review presents the state of the art of the production of these vectors with particular emphasis on their large-scale production for clinical purposes. In contrast to oncoretroviral vectors, which are produced using stable producer cell lines, clinical-grade LV are in most of the cases produced by transient transfection of 293 or 293T cells grown in cell factories. However, more recent developments, also, tend to use hollow fiber reactor, suspension culture processes, and the implementation of stable producer cell lines. As is customary for the biotech industry, rather sophisticated downstream processing protocols have been established to remove any undesirable process-derived contaminant, such as plasmid or host cell DNA or host cell proteins. This review compares published large-scale production and purification processes of LV and presents their process performances. Furthermore, developments in the domain of stable cell lines and their way to the use of production vehicles of clinical material will be presented.

摘要

慢病毒载体 (LV) 在作为治疗获得性和遗传性疾病的基因治疗载体方面的应用有了显著增加。本综述介绍了这些载体生产的最新技术,特别强调了其用于临床目的的大规模生产。与使用稳定生产细胞系生产的正逆转录病毒载体不同,临床级 LV 大多数情况下是通过在细胞工厂中生长的 293 或 293T 细胞的瞬时转染来生产的。然而,最近的发展趋势也倾向于使用中空纤维反应器、悬浮培养工艺,并实施稳定生产细胞系。与生物技术行业的惯例一样,已经建立了相当复杂的下游处理方案,以去除任何不需要的工艺衍生污染物,如质粒或宿主细胞 DNA 或宿主细胞蛋白。本综述比较了已发表的 LV 大规模生产和纯化工艺,并介绍了它们的工艺性能。此外,还将介绍稳定细胞系领域的发展及其在临床材料生产载体方面的应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a441/4830361/0a4fdadde464/mtm201617-f1.jpg

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