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通过ClonePix FL进行连续筛选和细胞内染色有助于分离用于单克隆抗体制备的高产细胞系。

Sequential screening by ClonePix FL and intracellular staining facilitate isolation of high producer cell lines for monoclonal antibody manufacturing.

作者信息

Roy Gargi, Miro-Quesada Guillermo, Zhuang Li, Martin Tom, Zhu Jie, Wu Herren, Marelli Marcello, Bowen Michael A

机构信息

Antibody Discovery and Protein Engineering, MedImmune LLC, One MedImmune Way, Gaithersburg, MD 20878, USA.

Bioprocess, Analytical and Manufacturing Sciences, Biopharmaceutical Development, MedImmune LLC, One MedImmune Way, Gaithersburg, MD 20878, USA.

出版信息

J Immunol Methods. 2017 Dec;451:100-110. doi: 10.1016/j.jim.2017.08.012. Epub 2017 Sep 8.

DOI:10.1016/j.jim.2017.08.012
PMID:28890364
Abstract

Screening and characterization of cell lines for stable production are critical tasks in identifying suitable recombinant cell lines for the manufacture of protein therapeutics. To aid this essential function we have developed a methodology for the selection of antibody expressing cells using fluorescence based ClonePix FL colony isolation and flow cytometry analysis following intracellular staining for immunoglobulin G (IgG). Our data show that characterization of cells by flow cytometry early in the clone selection process enables the identification of cell lines with the potential for high productivity and helps to eliminate unstable cell lines. We further demonstrate a correlation between specific productivity (qP) and intracellular heavy chain (HC) content with final productivity. The unique combination of screening using ClonePix FL and the flow cytometry approaches facilitated more efficient isolation of clonal cell lines with high productivity within a 15week timeline and which can be applied across NS0 and CHO host platforms. Furthermore, in this study we describe the critical parameters for the ClonePix FL colony based selection and the associated calculations to provide an assessment of the probability of monoclonality of the resulting cell lines.

摘要

筛选和鉴定用于稳定生产的细胞系是识别适合生产蛋白质治疗药物的重组细胞系的关键任务。为辅助这一重要功能,我们开发了一种方法,用于在对免疫球蛋白G(IgG)进行细胞内染色后,使用基于荧光的ClonePix FL集落分离和流式细胞术分析来选择表达抗体的细胞。我们的数据表明,在克隆选择过程早期通过流式细胞术对细胞进行表征,能够识别出具有高生产潜力的细胞系,并有助于淘汰不稳定的细胞系。我们进一步证明了比生产率(qP)与细胞内重链(HC)含量与最终生产率之间的相关性。使用ClonePix FL进行筛选和流式细胞术方法的独特组合,有助于在15周的时间内更有效地分离出具有高生产率的克隆细胞系,并且该方法可应用于NS0和CHO宿主平台。此外,在本研究中,我们描述了基于ClonePix FL集落选择的关键参数以及相关计算,以评估所得细胞系单克隆性的概率。

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Sequential screening by ClonePix FL and intracellular staining facilitate isolation of high producer cell lines for monoclonal antibody manufacturing.通过ClonePix FL进行连续筛选和细胞内染色有助于分离用于单克隆抗体制备的高产细胞系。
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