Transient gene expression in suspension HEK-293 cells: Application to large-scale protein production

被引:93
|
作者
Baldi, L [1 ]
Muller, N [1 ]
Picasso, S [1 ]
Jacquet, R [1 ]
Girard, P [1 ]
Thanh, HP [1 ]
Derow, E [1 ]
Wurm, FM [1 ]
机构
[1] Ecole Polytech Fed Lausanne, Lab Cellular Biotechnol, LBTC, IGBB,Inst Biol Engn & Biotechnol, CH-1015 Lausanne, Switzerland
关键词
D O I
10.1021/bp049830x
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Recent advances in genomics, proteomics, and structural biology raised the general need for significant amounts of pure recombinant protein (r-protein). Because of the difficulty in obtaining in some cases proper protein folding in bacteria, several methods have been established to obtain large amounts of r-proteins by transgene expression in mammalian cells. We have developed three nonviral DNA transfer protocols for suspension-adapted HEK-293 and CHO cells: (1) a calcium phosphate based method (Ca-Pi), (2) a calcium-mediated method called Calfection, and (3) a polyethylenimine-based method (PEI). The first two methods have already been scaled up to 14 L and 100 L for HEK-293 cells in bioreactors. The third method, entirely serum-free, has been successfully applied to both suspension-adapted CHO and HEK-293 cells. We describe here the application of this technology to the transient expression in suspension cultivated HEK-293 EBNA cells of some out of more than 20 secreted r-proteins, including antibodies, dimeric proteins, and tagged proteins of various complexity. Most of the proteins were expressed from different plasmid vectors within 5 - 10 days after the availability of the DNA. Transfections were successfully performed from the small scale (1 mL in 12-well microtiter plates) to the 2 L scale. The results reported made it possible to establish an optimized cell culture and transfection protocol that minimizes batch-to-batch variations in protein expression. The work presented here proves the applicability and robustness of transient transfection technology for the expression of a variety. of recombinant proteins.
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收藏
页码:148 / 153
页数:6
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