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作 者:黄天明[1] 黄绍明[2] 莫发荣[1] 何少健[1] 周素芳[3] 邓琼英[2] 李松峰[2] 黄敏丽[4] 李山[5] 薛慧琴[1] 梁皓[4] 范容[1] 闫磊[1] 谢小薰[1] 罗国容[1]
机构地区:[1]广西医科大学组织胚胎学教研室,南宁530021 [2]广西医科大学解剖学教研室 [3]广西医科大学生化教研室 [4]广西医科大学第一附属医院眼科 [5]广西医科大学第一附属医院检验科
出 处:《广西医科大学学报》2006年第3期345-348,共4页Journal of Guangxi Medical University
基 金:国家自然科学基金资助课题(No.30460037);高校博士点专项基金资助项目(No.20050598006);广西自然科学基金资助项目(No.0542068)
摘 要:目的:研究肝癌相关抗原kinectin基因片断的体外重组表达方法,为该抗原的生产奠定基础。方法:用PCR法扩增肝癌相关抗原kinectin的基因片断,将目的基因插入表达载体pMAL-C2上麦芽糖结合蛋白(MBP)基因下游的多克隆位点,转化DH5α菌。通过蓝白斑筛选、PCR鉴定、内切酶鉴定及DNA测序筛出正确的重组子,并用其转化TB1菌。用IPTG对重组的TB1工程菌进行诱导表达,SDS-PAGE电泳鉴定。结果:kinectin基因片断正确插入pMAL-C2载体的多克隆位点,用IPTG对工程菌进行诱导,可见目的蛋白条带出现。结论:pMAL-C2载体可用于对肝癌相关抗原kinectin的体外基因重组表达。Objective:To study the method to recombine and express the gene segment of HCC-associated antigen-kinectin in vitro, which will provide a basis for the production of this antigen. Methods: The gene segment of kinectin was amplified by PCR, and then inserted into the vector pMAL-C2 at the downstream of the gene encoding the MBP protein. The recombinant vector was transfected into E. coli DH5α. The blue-white selection assay, PCR, incision enzyme assay and DNA sequencing were performed to find out the right recombinant clone. The right clone was transfected into the expression host (E. coli TB1), then the engineering bacteria was induced by IPTG. The induction products were analyzed through the SDSPAGE electrophoresis. Result: The gene segment of kinectin have been successfully inserted into the vector pMAL-C2 at the multiple clone site, and the interest protein was expressed when the engineering bacteria was induced by IPTG. Conclusion: The expression vector pMAL-C2 can be used to recombine and express the gene segment of kinectin in vitro.
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