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Representative mammalian cell culture test materials for assessment of primary recovery technologies: A rapid method with industrial applicability

机译:评估主要回收技术的代表性哺乳动物细胞培养测试材料:具有工业实用性的快速方法

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摘要

Mammalian cell culture material is often difficult to produce accurately and reproducibly for downstream studies. This article presents a methodology for the creation of a set of cell culture test materials where key variables including cell density, cell viability, product, and the host cell protein (HCP) load can be manipulated individually. The methodology was developed using a glutamine synthetase Chinese hamster ovary cell line cultured at 5-L and 70-L scales. Cell concentration post-cell growth was manipulated using tangential flow filtration to generate a range of target cell densities of up to 100 × 106 cells/mL. A method to prepare an apoptotic cell stock to achieve target viabilities of 40–90% is also described. In addition, a range of IgG1 and HCP concentrations was achieved. The results illustrate that the proposed methodology is able to mimic different cell culture profiles by decoupling the control of the key variables. The cell culture test materials were shown to be representative of typical cell culture feed material in terms of particle size distribution and HCP population. This provides a rapid method to create the required feeds for assessing the feasibility of primary recovery technologies designed to cope with higher cell density cultures.
机译:哺乳动物细胞培养材料通常难以准确,可重复地生产用于下游研究。本文介绍了一种用于创建一组细胞培养测试材料的方法,其中可以分别操纵包括细胞密度,细胞生存力,产物和宿主细胞蛋白(HCP)负荷在内的关键变量。该方法是使用以5升和70升规模培养的谷氨酰胺合成酶中国仓鼠卵巢细胞系开发的。使用切向流过滤处理细胞生长后的细胞浓度,以产生高达100×10 6 个细胞/ mL的靶细胞密度范围。还介绍了一种制备凋亡细胞原液以实现40-90%的靶标活力的方法。另外,达到了一定范围的IgG1和HCP浓度。结果表明,所提出的方法能够通过去耦关键变量的控制来模仿不同的细胞培养谱。在粒度分布和HCP群体方面,细胞培养物测试材料显示出是典型细胞培养物进料的代表。这提供了一种快速的方法来创建所需的饲料,以评估旨在应对较高细胞密度培养的初级回收技术的可行性。

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