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多重数字 mRNA 表达分析系统——在重组中国仓鼠卵巢细胞分批培养过程中,UPR 特异性基因表达变化的 mRNA 丰度和响应的全系统变化。

Multiplexed Digital mRNA Expression Analysis Profiles System-Wide Changes in mRNA Abundance and Responsiveness of UPR-Specific Gene Expression Changes During Batch Culture of Recombinant Chinese Hamster Ovary Cells.

机构信息

Programa Institucional de Fomento a la Investigación, Desarrollo e Innovación, Univ. Tecnológica Metropolitana, Ignacio Valdivieso 2409, San Joaquín, P.O. Box, 8940577, Santiago, Chile.

The University of Manchester, Faculty of Life Sciences, Manchester Institute of Biotechnology, M1 7DN, Manchester, United Kingdom.

出版信息

Biotechnol J. 2018 Mar;13(3):e1700429. doi: 10.1002/biot.201700429. Epub 2018 Feb 2.

DOI:10.1002/biot.201700429
PMID:29323465
Abstract

The unfolded protein response (UPR) signaling pathway is viewed as critical for setting the effectiveness of recombinant protein expression in CHO cells. In this study, Nanostring nCounter technology is used to study expression of a group of genes associated with cellular processes linked to UPR activation under ER stress and the changing environment of a batch culture. Time course induction of ER stress, using tunicamycin (TM), shows a group of genes such as Chop, Trb3, Sqstm1, Grp78, and Herpud1 respond rapidly to TM inhibition of N-glycosylation, while others such as Atf5, Odz4, and Birc5 exhibits a delayed response. In batch culture, expression of "classical" UPR markers only increases when cells enter decline phase. In addition to providing a detailed analysis of the expression of process-relevant UPR markers during batch culture and in response to imposed chemical stress, we also highlighted six genes (Herpud1, Odz4, Sqstm1, Trb3, Syvn1, and Birc5) associated with the perception of ER stress responses in recombinant CHO cells. Herpud1 (involved in ER-associated degradation) exhibits a rapid (primary) response to stress and its relationship (and that of the other five genes) to the overall cellular UPR may identify novel targets to modulate recombinant protein production in CHO cells.

摘要

未折叠蛋白反应(UPR)信号通路被认为对设定 CHO 细胞中重组蛋白表达的有效性至关重要。在这项研究中,Nanostring nCounter 技术用于研究一组与 UPR 激活相关的基因表达,这些基因与内质网应激和批培养不断变化的环境有关。使用衣霉素(TM)对 ER 应激进行时间过程诱导,表明一组基因(如 Chop、Trb3、Sqstm1、Grp78 和 Herpud1)对 TM 抑制 N-糖基化的反应迅速,而其他基因(如 Atf5、Odz4 和 Birc5)则表现出延迟反应。在批培养中,只有当细胞进入衰退阶段时,“经典”UPR 标志物的表达才会增加。除了提供批培养过程中与内质网应激相关的 UPR 标志物表达的详细分析以及对施加的化学应激的反应外,我们还强调了与重组 CHO 细胞中内质网应激反应感知相关的六个基因(Herpud1、Odz4、Sqstm1、Trb3、Syvn1 和 Birc5)。Herpud1(参与内质网相关降解)对应激表现出快速(主要)反应,其与其他五个基因的关系(以及其他五个基因的关系)与细胞整体 UPR 可能确定调节 CHO 细胞中重组蛋白生产的新靶点。

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