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作 者:杨立宏[1] 韩丽英[1] 苏成芝[1] 高长寿[2]
机构地区:[1]第四军医大学生物化学教研室,西安710032 [2]中国科学院上海生物工程研究中心,上海200233
出 处:《生物工程学报》1996年第2期183-188,共6页Chinese Journal of Biotechnology
摘 要:利用PCR突变方法,改造了人白细胞介素-3(hIL-3)cDNA,在成熟蛋白编码顺序5'端前突变入了Xba I酶切位点和酵母类胰蛋白酶加工位点Lys-Arg的密码子。改造后的hIL-3 cDNA插入大肠杆菌-酵母穿梭质粒pVT102u/α,使其准确融合于α-交配因子前导序列之后,并置于启动子ADH1调控之下。转化入酿酒酵母宿主菌S-78筛选后,30℃培养48h。Using the PCR technique,mutated human interleukin 3(hIL-3) gene was'obtained, in which the restriction site Xba I and site of trpsin-like endoprotease were made in front of the 5' terminal encoding sequence. This gene was fused to the leader sequence of a-mating factor behind and cloned into pVT10 2u/a, a shuttle plasmid between yeast and E. coli, the fused gene can be transcripted under the coNtrol of ADH1 promoter in yeast. After fransformation of the plasmid containing the hIL-3 gene into saccharomyces cerevisiae S-78 and fermentation at 30癈 for 48 hours, it was observed that the culture supernatant was able to obviously stimulate preliferation of the hIL-3 dependent TF-1 cell line. The expressed rhIL-3 in the supernatant was more than 1. 0mg/L identified and quantified by ELISA. It was also found that the biological activity of rhIL-3 in this supernatant was about 1. 8x103u/ml after being analysised by 3H-thymidine incorproation methed using TF-1 cells.
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