Accurate Determination of Plasmid Copy Number of Flow-Sorted Cells using Droplet Digital PCR

质粒 单元格排序 化学 流式细胞术 绿色荧光蛋白 分子生物学 恶臭假单胞菌 数字聚合酶链反应 人口 DNA 基因 生物 聚合酶链反应 生物化学 社会学 人口学
作者
Michael Jahn,Carsten Vorpahl,Dominique Türkowsky,Martin Lindmeyer,Bruno Bühler,Hauke Harms,Susann Müller
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:86 (12): 5969-5976 被引量:44
标识
DOI:10.1021/ac501118v
摘要

Many biotechnological processes rely on the expression of a plasmid-based target gene. A constant and sufficient number of plasmids per cell is desired for efficient protein production. To date, only a few methods for the determination of plasmid copy number (PCN) are available, and most of them average the PCN of total populations disregarding heterogeneous distributions. Here, we utilize the highly precise quantification of DNA molecules by droplet digital PCR (ddPCR) and combine it with cell sorting using flow cytometry. A duplex PCR assay was set up requiring only 1000 sorted cells for precise determination of PCN. The robustness of this method was proven by thorough optimization of cell sorting, cell disruption, and PCR conditions. When non plasmid-harboring cells of Pseudomonas putida KT2440 were spiked with different dilutions of the expression plasmid pA-EGFP_B, a PCN from 1 to 64 could be accurately detected. As a proof of principle, induced cultures of P. putida KT2440 producing an EGFP-fused model protein by means of the plasmid pA-EGFP_B were investigated by flow cytometry and showed two distinct subpopulations, fluorescent and nonfluorescent cells. These two subpopulations were sorted for PCN determination with ddPCR. A remarkably diverging plasmid distribution was found within the population, with nonfluorescent cells showing a much lower PCN (≤1) than fluorescent cells (PCN of up to 5) under standard conditions.
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