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Optimisation of a simple method to transiently transfect a CHO cell line in high-throughput and at large scale

机译:优化以高通量大规模转染CHO细胞的简单方法

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摘要

Transient expression of heterologous proteins in mammalian systems is a powerful way to generate protein reagents quickly. However, it has historically suffered from poor yields in comparison to methods where the recombinant gene is stably integrated into the genome and high expressing clones isolated. Transient methods have been well described for HER-based systems. In this paper we show the use of a design of experiments (DoE) approach to quickly analyse the effect of a range of different parameters on protein expression from a CHO-based transient system. We show that this system is amenable to a very simple transfection procedure by independent direct addition of DNA and transfection reagent to the culture vessel. In addition we show that expression can be improved by reducing the temperature of the culture conditions post-transfection. The process is demonstrated to be transferrable from 3 ml cultures in deep 24-well plates through cultures in CultiFlask Bioreactors, shake flasks and up to 25 L culture in Wave Bioreactors. Data are shown to illustrate the utility of the system with a number of different classes of protein. (C) 2015 Elsevier Inc. All rights reserved.
机译:异源蛋白在哺乳动物系统中的瞬时表达是快速产生蛋白试剂的有效方法。但是,与将重组基因稳定地整合到基因组中并分离出高表达克隆的方法相比,其历来的产量很低。对于基于HER的系统,已经很好地描述了瞬态方法。在本文中,我们展示了使用实验设计(DoE)方法从基于CHO的瞬时系统快速分析一系列不同参数对蛋白质表达的影响。我们表明,通过将DNA和转染试剂独立直接添加到培养容器中,该系统适用于非常简单的转染程序。另外,我们表明可以通过降低转染后培养条件的温度来改善表达。已证明该过程可从深24孔板中的3 ml培养物通过CultiFlask生物反应器,摇瓶和Wave Bioreactor中最多25 L的培养物转移。显示了数据以说明该系统对许多不同类别的蛋白质的实用性。 (C)2015 Elsevier Inc.保留所有权利。

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