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在表达丙酮酸羧化酶的 HEK-293 细胞中增强糖蛋白的产生。

Enhanced glycoprotein production in HEK-293 cells expressing pyruvate carboxylase.

机构信息

Département de Génie Chimique, École Polytechnique de Montréal, C.P. 6079, Succ. Centre-ville, Montréal, Québec, Canada.

出版信息

Metab Eng. 2011 Sep;13(5):499-507. doi: 10.1016/j.ymben.2011.05.004. Epub 2011 May 23.

Abstract

There is an imperative need for expression systems allowing the efficient and robust manufacturing of high quality glycoproteins. In the present work, HEK-293 cells stably expressing interferon-α2b were further engineered with the insertion of the yeast pyruvate carboxylase 2 gene. In batch cultures, marked reductions in lactate and ammonia production were observed compared to the parental cell clone. Although the maximum specific growth rate remained unchanged, the altered metabolism led to a 2-fold increase in maximum cell density and 33% increase in the integral of viable cell concentration and interferon production yield. The underlying metabolic changes were further investigated using various (13)C-labeled substrates and measuring the resulting lactate mass isotopomer distributions. Simultaneous metabolite and isotopomer balancing allowed the accurate determination of key intracellular fluxes. Such detailed and quantitative knowledge about the central carbon metabolism of the cells is instrumental to further support the development of high-yield fed-batch processes.

摘要

非常需要能够高效且稳健地生产高质量糖蛋白的表达系统。在本研究中,进一步对稳定表达干扰素-α2b 的 HEK-293 细胞进行工程改造,插入酵母丙酮酸羧化酶 2 基因。与亲本细胞克隆相比,在分批培养中观察到乳酸盐和氨的产生明显减少。尽管最大比生长速率保持不变,但改变的代谢导致最大细胞密度增加了 2 倍,活细胞浓度和干扰素产量的积分增加了 33%。使用各种 (13)C 标记的底物进一步研究了潜在的代谢变化,并测量了所得乳酸盐质量同位素分布。同时的代谢物和同位素平衡允许准确确定关键的细胞内通量。这种关于细胞中心碳代谢的详细和定量的知识对于进一步支持高产补料分批过程的发展至关重要。

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