直接液滴数字PCR法定量大肠杆菌宿主残留DNA

Jeremy Anderson, M. Hussain
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引用次数: 1

摘要

用大肠杆菌生产的注射用药物必须进行宿主残留DNA (hr DNA)杂质检测,以保证药物的纯度和安全性。由于允许的hr较低,因此需要高灵敏度的方法。液滴数字PCR (ddPCR)是一种新方法,它将反应分割成约20,000纳米升大小的液滴,每个液滴作为单个PCR反应。终点PCR完成后,对液滴进行荧光分析,并将其分为阳性或阴性,并使用泊松统计量对DNA进行定量。在这里,我们描述了直接大肠杆菌hr DNA ddPCR方法的发展,其中药物直接添加到ddPCR反应中。我们发现,ddPCR方法具有可接受的精密度和较高的准确度,适用于不同的生物药物,与qPCR相比,对药物基质具有更高的耐受性。该方法不需要DNA提取或标准曲线来定量未知样品中的hr DNA。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A Direct Droplet Digital PCR Method for E. coli Host Residual DNA Quantification
Injectable drugs manufactured in E. coli must be tested for host residual DNA (hr DNA) impurity in ensuring drug purity and safety. Because of low allowable hr DNA as impurity, highly sensitive methods are needed. Droplet digital PCR (ddPCR) is a new method where the reaction is partitioned into about 20,000 nanoliter-sized droplets and each droplet acts as individual PCR reaction. After completion of end-point PCR, droplets are analyzed for fluorescence and categorized as positive or negative and DNA quantified using Poisson statistics. Here we describe development of a direct E. coli hr DNA dd PCR method where the drug is directly added to the ddPCR reaction. We show that the ddPCR method has acceptable precision and high accuracy, works with different biologic drugs, and compared to qPCR shows higher tolerance of drug matrices. The method does not require DNA extraction or standard curves for quantification of hr DNA in unknown samples.
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