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Identification of the Limitations on Recombinant Gene Expression in CHO Cell Lines With Varying Luciferase Production Rates

机译:萤光素酶生产率不同的CHO细胞株中重组基因表达的限制的鉴定。

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Mammalian cell lines are currently employed as one of the main cellular factories for the expression of recombinant protein-based drugs. The establishment of high-producing cell lines typically begins with a heterogeneous starter population of cells, from which the highest producing cells are selected via empirical approaches. This approach is time consuming, and is likely to encounter natural upper limits imposed by the inherent biology of the cell lines in question. In an attempt to understand both the nature of the variability in populations of cells transfected with recombinant protein encoding DNA and the natural mechanisms of productivity limitation, we developed protocols for the detailed investigation of gene expression pathways in such cell lines. This novel approach was then applied to a set of clonal CHOK1 cell lines producing recombinant luciferase with varying productivities. Our results show that the initial limitation in these cell lines is at the transcriptional level, however in the highest producing cell line post-translational mechanisms affecting both protein turnover and protein folding become severely limiting. The implications for the development of strategies to engineer cells for enhanced recombinant protein production levels are discussed.
机译:哺乳动物细胞系目前被用作表达基于重组蛋白的药物的主要细胞工厂之一。高产细胞系的建立通常从异质起始细胞群体开始,通过经验方法从中选择最高产细胞。这种方法很耗时,并且很可能会遇到有关细胞系固有生物学所施加的自然上限。为了理解被编码DNA的重组蛋白转染的细胞群体的变异性和生产力限制的天然机制,我们开发了用于详细研究此类细胞系中基因表达途径的方案。然后将该新方法应用于产生具有不同生产率的重组荧光素酶的一组克隆CHEK1细胞系。我们的结果表明,这些细胞系的初始限制是在转录水平上,但是在产量最高的细胞系中,影响蛋白质更新和蛋白质折叠的翻译后机制变得十分严格。讨论了开发用于工程化细胞以提高重组蛋白生产水平的策略的意义。

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