Plasmid DNA Manufacturing for Indirect and Direct Clinical Applications

质粒 良好制造规范 遗传增强 DNA 碱裂解 基因 生物 溶解 计算生物学 dna疫苗 生物技术 分子生物学 遗传学 监管事务
作者
Marco Schmeer,Tatjana Buchholz,Martin Schleef
出处
期刊:Human Gene Therapy [Mary Ann Liebert]
卷期号:28 (10): 856-861 被引量:47
标识
DOI:10.1089/hum.2017.159
摘要

Plasmid DNA is currently gaining increasing importance for clinical research applications in gene therapy and genetic vaccination. For direct gene transfer into humans, good manufacturing practice (GMP)-grade plasmid DNA is mandatory. The same holds true if the drug substance contains a genetically modified cell, for example chimeric antigen receptor (CAR) T cells, where these cells as well as the contained plasmids are used. According to the responsible regulatory agencies, they have to be produced under full GMP. On the other hand, for GMP production of, for example, mRNA or viral vectors (lentiviral vectors, adeno-associated virus vectors, etc.), in many cases, High Quality Grade plasmid DNA is accepted as a starting material. The manufacturing process passes through different production steps. To ensure the right conditions are used for the plasmid, a pilot run must be conducted at the beginning. In this step, a followed upscaling with respect to reproducibility and influences on product quality is performed. Subsequently, a cell bank of the transformed productions strain is established and characterized. This cell bank is used for the cultivation process. After cell harvesting and lysis, several chromatography steps are conducted to receive a pure plasmid product. Depending on the respective required quality grade, the plasmid product is subject to several quality controls. The last step consists of formulation and filling of the product.
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