Expression of human interleukin-11 cDNA in E.coli

被引:0
|
作者
苗继红 [1 ]
王嘉玺 [1 ]
彭善云 [1 ]
唐佩弦 [1 ]
邹民吉 [1 ]
段聚宝 [1 ]
赵春文 [1 ]
马贤凯 [1 ]
机构
[1] Institute of Basic Medical Sciences,Beijing 100850,China
关键词
human interleukin-11 (hIL-11); E; coli; gene expression; fusion protein; inclusion body;
D O I
暂无
中图分类号
Q78 [基因工程(遗传工程)];
学科分类号
071007 ; 0836 ; 090102 ;
摘要
A 551-bp hIL-11 gene fragment that includes no nucleotide sequences encoding signalpolypeptide and the initial 8 amino acids of the mature protein was cloned into a high-level expression vectorpEx31B of E.coli.The authors identified the recombinant plasmid,designated pEx31-IL11,by restriction endonu-cleases digestion and DNA sequencing.The resulting recombinant plasmids were then used to transform E.colistrain HB101,and expression in the PL promoter system,which is temperature-regulated,was achieved.The ex-pressed fusion protein amounts to 50% of total bacterial proteins.The hIL-11 protein expressed in E.coliwas fused to the N-terminal 99 amino acids of the MS2 polymerase to form the inclusion body.Theserecombinant proteins can be purified to about 80% by extracting inclusion body with urea.OneIL-6-dependent cell line 7 TD1 was used for bioassay.The recombinant hIL-11 protein was preliminarily puri-fied and renatured to a specific activity of 10U/mg,even in the presence of an excess of a neutralizing an-ti-IL-6 antibody.
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页码:1202 / 1209
页数:8
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