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作 者:赵大鹏[1] 王晓宇[1] 刘畅[1] 戚凤春[1] 蒙冲[1] 王影[1] 王妍[1] 盛君[1] 杨煜[2] 傅学奇[2]
机构地区:[1]长春生物制品研究所,长春130062 [2]吉林大学,长春130021
出 处:《中国生物制品学杂志》2001年第3期139-142,共4页Chinese Journal of Biologicals
基 金:吉林省科技发展计划资助项目。
摘 要:目的 扩增类胰岛素生长因子I(IGF-I)210bp的DNA片段,将其克隆到PGEX-1 λT质粒,并转化到 E.coli NH522中高效表达。方法 用改进的RT-PCR法合成人肝脏cDNA,然后从该cDNA文库中扩增出IGF-I基 因。将扩增的IGF-I cDNA用 BamHI和EcoR I双酶切后,插入到同样双酶切处理的pGEX-1λT载体中,连接转化 E. coli NM522,筛选克隆,酶切鉴定后,进行了核苷酸序列分析及表达。结果 将IPTG诱导表达的菌体离心收集,经 SDS-PAGE分析,在相对分子质量34000处可见明显高表达带,表达量可占菌体蛋白总量的20%以上。免疫印迹表 明重组蛋白具有IGF-I的抗原性。结论 重组人IGF-I的成功克隆与表达,将为进一步研究人ICF-I的生物学特性 打下基础。Objective To amplify a 210bp of DNA fragment of insulin like growth factor-I (IGF-I) and clone it into plasmid pGEX- 1 λ T for high expression. Methods IGF-I gene was isolated from the human liver cDNA bank synthesized by an improved RT-PCR. The IGF-I cDNA amplified by PCR was digested by BamH I and EcoR I,and inserted into the pGEX-1λ T vector digested by the 2 kinds of enzyme,then trans-formed to E. coli NM522. The positive clones were screened out and identified by enzyme digestion and se-quencing. Results The somatic protein expressed under the induction of IPTG was collected by centrifugation and detected by SDS-PAGE. A significant band with a relative molecular weight of 34000 was observed. Thin layer scanning proved that the expressed product contained more than 20% of total somatic protein. Western blot showed the IGF-I antigenicity of expressed protein. Conclusion Recombinant human IGF-I was successfully ex-pressed in this paper. It laid a foundation of further study on the biological characteristics of human IGF-I.
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