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Producing Recombinant Adeno-Associated Virus in Foster Cells: Overcoming Production Limitations Using a Baculovirus–Insect Cell Expression Strategy

机译:在寄养细胞中生产重组腺相关病毒:使用杆状病毒-昆虫细胞表达策略克服生产限制

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摘要

Establishing pharmacological parameters, such as efficacy, routes of administration, and toxicity, for recombinant adeno-associated virus (rAAV) vectors is a prerequisite for gaining acceptance for clinical applications. In fact, even a therapeutic window, that is, the dose range between therapeutic efficacy and toxicity, has yet to be determined for rAAV in vivo. Multiphase clinical trials investigating the safety and efficacy of recombinant AAV-based therapeutics will require unprecedented vector production capacity to meet the needs of preclinical toxicology studies, and the progressive clinical protocol phases of safety/dose escalation (phase I), efficacy (phase II), and high-enrollment, multicenter evaluations (phase III). Methods of rAAV production capable of supporting such trials must be scalable, robust, and efficient. We have taken advantage of the ease of scalability of nonadherent cell culture techniques coupled with the inherent efficiency of viral infection to develop an rAAV production method based on recombinant baculovirus-mediated expression of AAV components in insect-derived suspension cells.
机译:建立重组腺相关病毒(rAAV)载体的药理参数,例如功效,给药途径和毒性,是获得临床应用认可的先决条件。实际上,甚至还没有确定体内rAAV的治疗窗,即治疗功效和毒性之间的剂量范围。研究基于重组AAV的疗法的安全性和有效性的多阶段临床试验将需要空前的载体生产能力,以满足临床前毒理学研究的需要,以及安全性/剂量递增(I期),有效性(II期)的渐进临床方案阶段,以及高入学率的多中心评估(第三阶段)。能够支持此类试验的rAAV生产方法必须是可扩展的,强大的和有效的。我们已经利用了非粘附细胞培养技术的可扩展性,以及病毒感染的固有效率,来开发基于重组杆状病毒介导的昆虫来源的悬浮细胞中AAV成分表达的rAAV生产方法。

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