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Production of lentiviral vectors by large-scale transient transfection of suspension cultures and affinity chromatography purification

机译:通过悬浮培养物的大规模瞬时转染和亲和层析纯化产生慢病毒载体

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摘要

The use of lentiviral vectors as gene delivery vehicles has become increasingly popular in recent years. The growing interest in these vectors has created a strong demand for large volumes of vector stocks, which entails the need for scaleable vector manufacturing procedures. In this work, we present a simple and robust process for the production of lentiviral vectors using scaleable production and purification methodologies. Lentivirus particles were produced by transient transfection of serum-free suspension-growing 293 EBNA-1 cells with four plasmids encoding the vector components using linear polyethylenimine (PEI) as transfection reagent. This process was successfully scaled-up from shake flaks to a 3-L bioreactor from which 10(10) IVP were recovered. In addition, an affinity chromatography protocol designed for purification of bioactive oncoretroviral vectors has been adapted in this work for the purification of VSV-G pseudotyped lentiviral vectors. Using heparin affinity chromatography, lentiviral particles were concentrated and purified directly from the clarified supernatants. During this step, a recovery of 53% of infective lentiviral particles was achieved while removing 94% of the impurities contained in the supernatant.
机译:近年来,慢病毒载体作为基因传递载体的使用变得越来越流行。对这些载体的日益增长的兴趣已引起对大量载体库存的强烈需求,这需要可扩展的载体生产程序。在这项工作中,我们提出了使用规模化生产和纯化方法生产慢病毒载体的简单而稳定的方法。通过使用线性聚乙烯亚胺(PEI)作为转染试剂,用编码载体成分的四个质粒瞬时转染无血清悬液生长的293 EBNA-1细胞来生产慢病毒颗粒。此过程已成功地从摇瓶扩大到3-L生物反应器,从中回收了10(10)IVP。另外,为纯化VSV-G假型慢病毒载体而设计的亲和层析方案已被设计用于纯化具有生物活性的核糖核酸病毒载体。使用肝素亲和层析,将慢病毒颗粒浓缩并直接从澄清的上清液中纯化。在此步骤中,回收了53%的感染性慢病毒颗粒,同时去除了上清液中94%的杂质。

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