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A qPCR Method for AAV Genome Titer with ddPCR-Level of Accuracy and Precision

机译:具有DDPCR级别精度和精度的AAV基因组滴度的QPCR方法

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摘要

Recombinant adeno-associated virus (rAAV) is one of the main vectors used in gene therapy. An accurate genome titer is not only critical for clinical dosing, but also a prerequisite for many analytical assays for AAV product characterization. AAV genome titer is traditionally determined by qPCR; however, assay precision is not optimal despite extensive efforts. More recently, droplet digital PCR (ddPCR) emerged as a powerful alternative that offers excellent accuracy and precision. However, currently ddPCR is not as widely available as qPCR and operates at a lower throughput and a higher cost. In this paper, we introduce an improved qPCR method with two major optimizations: (1) using an AAV reference material as qPCR standard instead of plasmid DNA and (2) implementing a “digestion-free” method by adding 5% Tween 20 to standard and sample preparations. The new method has been extensively tested with AAV of different serotypes, purification status, and transgenes encapsidated and was found to be highly accurate, precise, and robust. This significantly improved and simplified assay can be easily adopted by researchers in the gene therapy field and further automated for high-throughput applications.
机译:重组腺相关病毒(RAAV)是基因治疗中使用的主要载体之一。准确的基因组滴度不仅对临床给药至关重要,而且对AAV产品表征的许多分析测定的先决条件。 AAV基因组滴度传统上由QPCR确定;然而,尽管广泛的努力,Assay精度并不是最佳的。最近,Droplet Digital PCR(DDPCR)作为一种强大的替代方案,提供了出色的准确性和精度。然而,目前DDPCR并不像QPCR一样广泛使用,并以较低的吞吐量和更高的成本运行。在本文中,我们介绍了一种改进的QPCR方法,具有两种主要优化:(1)使用AAV参考材料作为QPCR标准而不是质粒DNA和(2)通过加入5%Tween 20来实现“消化”方法和样品制剂。新方法已被广泛测试的AAV不同的血清型,净化状态和封装的转基因,并被发现是高度准确的,精确和鲁棒的。基因治疗领域的研究人员可以轻易采用这种显着改善和简化的测定,并进一步自动化高通量应用。

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