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用于生产热休克蛋白糖蛋白96的MethA肿瘤细胞悬浮培养过程:转瓶中的工艺优化

Suspension culture process of MethA tumor cell for the production of heat-shock protein glycoprotein 96: process optimization in spinner flasks.

作者信息

Tang Ya-Jie, Li Hong-Mei, Hamel Jean-François P

机构信息

Department of Chemical Engineering, Massachusetts Institute of Technology, 77 Massachusetts Avenue, Cambridge, Massachusetts 02139, USA.

出版信息

Biotechnol Prog. 2007 Nov-Dec;23(6):1363-77. doi: 10.1021/bp0702774. Epub 2007 Oct 18.

Abstract

Heat-shock proteins (HSPs) act like "chaperones", making sure that the cell's proteins are in the right shape and in the right place at the right time. Heat-shock protein glycoprotein 96 (gp96) is a member of the HSP90 protein family, which chaperones a number of molecules in protein folding and transportation. Heat-shock protein gp96 serves as a natural adjuvant for chaperoning antigenic peptides into the immune surveillance pathways. Currently, heat-shock protein gp96 was only isolated from murine and human tissues and cell lines. An animal cell suspension culture process for the production of heat-shock protein gp96 by MethA tumor cell was developed for the first time in spinner flasks. Effects of culture medium and condition were studied to enhance the MethA tumor cell density and the production and productivity of heat-shock protein gp96. Initial glucose concentration had a significant effect on the heat-shock protein gp96 accumulation, and an initial glucose level of 7.0 g/L was desirable for MethA tumor cell growth and heat-shock protein gp96 production and productivity. Cultures at an initial glutamine concentration of 3 and 6 mM were nutritionally limited by glutamine. At an initial glutamine concentration of 6 mM, the maximal viable cell density of 19.90 x 10(5) cells/mL and the maximal heat-shock protein gp96 production of 4.95 mg/L was obtained. The initial concentration of RPMI 1640 and serum greatly affected the MethA tumor cell culture process. Specifically cultures with lower initial concentration of RPMI 1640 resulted in lower viable cell density and lower heat-shock protein gp96 production. At an initial serum concentration of 8%, the maximal viable cell density of 19.18 x 10(5) cells/mL and the maximal heat-shock protein gp96 production of 5.67 mg/L was obtained. The spin rate significantly affected the cell culture process in spinner flasks, and a spin rate of 150 rpm was desirable for MethA tumor cell growth and heat-shock protein gp96 production and productivity. Not only the cell density but also the production and productivity of heat-shock protein gp96 attained in this work are the highest reported in the culture of MethA tumor cell. This work offers an effective approach for producing heat-shock protein glycoprotein 96 from the cell culture process. The fundamental information obtained in this study may be useful for the efficient production of heat-shock protein by animal cell suspension culture on a large scale.

摘要

热休克蛋白(HSPs)就像“伴侣蛋白”,确保细胞中的蛋白质在正确的时间处于正确的形状和位置。热休克蛋白糖蛋白96(gp96)是HSP90蛋白家族的成员,它在蛋白质折叠和运输过程中辅助多种分子。热休克蛋白gp96作为一种天然佐剂,将抗原肽带入免疫监视途径。目前,热休克蛋白gp96仅从小鼠和人类组织及细胞系中分离得到。首次在转瓶中开发了一种利用MethA肿瘤细胞生产热休克蛋白gp96的动物细胞悬浮培养工艺。研究了培养基和培养条件对提高MethA肿瘤细胞密度以及热休克蛋白gp96产量和产率的影响。初始葡萄糖浓度对热休克蛋白gp96的积累有显著影响,对于MethA肿瘤细胞生长以及热休克蛋白gp96的产量和产率而言,初始葡萄糖水平为7.0 g/L是理想的。初始谷氨酰胺浓度为3 mM和6 mM的培养物在营养上受到谷氨酰胺的限制。在初始谷氨酰胺浓度为6 mM时,获得了最大活细胞密度19.90×10⁵个细胞/mL和最大热休克蛋白gp96产量4.95 mg/L。RPMI 1640和血清的初始浓度极大地影响了MethA肿瘤细胞的培养过程。具体而言,RPMI 1640初始浓度较低的培养物导致活细胞密度较低以及热休克蛋白gp96产量较低。在初始血清浓度为8%时,获得了最大活细胞密度19.18×10⁵个细胞/mL和最大热休克蛋白gp96产量5.67 mg/L。转速显著影响转瓶中的细胞培养过程,对于MethA肿瘤细胞生长以及热休克蛋白gp96的产量和产率而言,150 rpm的转速是理想的。在这项工作中获得的不仅是细胞密度,还有热休克蛋白gp96的产量和产率,都是MethA肿瘤细胞培养中报道的最高值。这项工作为从细胞培养过程中生产热休克蛋白糖蛋白96提供了一种有效方法。本研究中获得的基础信息可能有助于通过动物细胞悬浮培养大规模高效生产热休克蛋白。

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