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作 者:王建勋[1,2] 陈松森[1,2] 狄旭[1,2] 宋卫华
机构地区:[1]中国医学科学院基础医学研究所 [2]中国协和医科大学基础医学院
出 处:《中国生物化学与分子生物学报》1999年第3期398-402,共5页Chinese Journal of Biochemistry and Molecular Biology
摘 要:利用RT-PCR方法成功地从PI(PMA,Ionomycin)、PHA活化的人T细胞中扩增出hIL-17编码区cDNA(468bp),克隆测序证实得到该基因.用特殊设计的引物扩增hIL-17成熟肽编码区(414bp),接入表达载体pET30a质粒中.pET30a-mhIL-17在大肠杆菌BL21(DE3)中获得高效表达,目的蛋白占总菌体蛋白50%左右.经凝胶过滤和阴离子交换层析两步分离纯化和复性,得到单体型rmhIL-17,纯度达98%以上,N端16个氨基酸序列分析,结果与文献报道一致.SDS-PAGE法测定分子量为16kD,薄层丙烯酰胺凝胶等电聚焦分析该蛋白等电点为pH8.8~8.9,3HTdR参入法测定rmhIL-17单体的体外活性,实验结果表明rmhIL-17对PHA活化人的PBMC细胞具有抑制作用。Human interleukin 17(hIL 17) cDNA(468 bp) was successfully amplified from human T cells activated by PI(PMA,Ionomycin)and PHA with RT PCR method.The results of cloning and sequencing proved this cDNA was the hIL 17 gene full length coding sequence.The cDNA(414 bp) coding mature hIL 17 was amplified with special designed primers.The cDNA fragments were cloned into expression vectors:pET30a.The pET30a mhIL 17 could highly express in E.coli BL21 (DE3),the recombinant hIL 17 was about 50% of total proteins.Monomer recombinant mhIL 17(98% pure) could be obtained with two steps of purification:gel filtration and ion exchange chromatography and renaturation.N terminal sequencing of rmhIL 17 showed the first 16 amino acids were the same as the sequence reported.Molecular weight and pI of rmhIL 17 were 16 kD and pH 8 8~8 9,measured with SDS PAGE and IEF respectively. In vitro activity assay found monomer rmhIL 17 could suppress the activation of human PBMC by PHA.It suggested that monomer rmhIL 17 had the similar activity with soluble IL 17 receptor.
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