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用于生产重组蛋白的HEK293-EBNA1细胞培养

Culture of HEK293-EBNA1 Cells for Production of Recombinant Proteins.

作者信息

Tom Roseanne, Bisson Louis, Durocher Yves

出版信息

CSH Protoc. 2008 Mar 1;2008:pdb.prot4976. doi: 10.1101/pdb.prot4976.

Abstract

INTRODUCTIONFast and efficient production of recombinant proteins (r-proteins) remains a major challenge for the academic and biopharmaceutical communities. Pure r-proteins are often required in large amounts (hundreds of milligrams to gram quantities) when being developed as biotherapeutics, or in smaller quantities (milligrams) for high-throughput screening campaigns and structural or functional studies. Mammalian cells are often preferred over prokaryotic systems when expressing cDNAs of mammalian origin due to their superior capability to conduct elaborate post-translational modifications. Large-scale transfection of mammalian cells is now establishing itself as a "must-have" technology in the scientific community, as it allows the production of milligram to gram quantities of r-proteins within a few days after cDNA cloning into the appropriate expression vector. The HEK293 cell line stably expressing the Epstein-Barr virus nuclear antigen-1 (HEK293-EBNA1, or 293E) is the most commonly used cell line for large-scale transfection. When using expression vectors bearing the Epstein-Barr virus origin of replication, oriP (such as the pTT vector), a threefold improvement in r-protein yield is generally obtained over a similar non-oriP vector. This protocol describes a method for culturing HEK293-EBNA1 cells which will then be used to produce recombinant proteins.

摘要

引言

重组蛋白(r蛋白)的快速高效生产仍然是学术界和生物制药界面临的一项重大挑战。当作为生物治疗药物进行研发时,通常需要大量(数百毫克至克级)的纯r蛋白,而在高通量筛选活动以及结构或功能研究中则需要较少量(毫克级)的纯r蛋白。由于哺乳动物细胞在进行复杂的翻译后修饰方面具有卓越能力,因此在表达哺乳动物来源的cDNA时,通常比原核系统更受青睐。哺乳动物细胞的大规模转染如今已成为科学界一项“必备”技术,因为在将cDNA克隆到合适的表达载体后,它能在几天内生产出毫克至克级的r蛋白。稳定表达爱泼斯坦 - 巴尔病毒核抗原1的HEK293细胞系(HEK293 - EBNA1,或293E)是大规模转染最常用的细胞系。当使用携带爱泼斯坦 - 巴尔病毒复制起点oriP的表达载体(如pTT载体)时,与类似的非oriP载体相比,r蛋白产量通常可提高三倍。本方案描述了一种培养HEK293 - EBNA1细胞的方法,随后这些细胞将用于生产重组蛋白。

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