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作 者:张家忠[1] 李小燕[2] 向田[2] 章晓联[2]
机构地区:[1]襄樊职业技术学院医学院,湖北襄樊441021 [2]武汉大学免疫系,湖北武汉443000
出 处:《襄樊职业技术学院学报》2007年第2期23-26,共4页Journal of Xiangfan Vocational and Technical College
摘 要:目的构建L-ficolin突变体的原核表达载体,为研究L-ficolin的糖结合位点奠定基础。方法设计L-ficolin突变体基因上、下游引物,分别引入EcoRⅠ和XhoⅠ酶切位点。以插入L—ficolin M2(Val144Phe)和M6(Glu 307Asp)点突变的完整编码区基因的质粒pCDNA3-L-ficolin为模板,通过PCR扩增获得突变体的基因片段,将其克隆入原核表达载体pGEX—KG.然后通过酶切和序列测定对其进行鉴定;将此表达载体转化入表达菌BL21(DE3)pLvSs诱导表达。并采用SDS—PAGE对表达产物进行鉴定。结果经酶切及序列分析表明.成功地构建了重组原核表达载体pGEX-KG—L—ficolin—M2、pGEX-KG-L-ficolin—M6,SDS—PAGE显示目的蛋白大量表达。结论L—ficolin突变体融合蛋白可以在大肠杆菌中大量表达。为研究L-ficolin的糖结合位点打下基础。Object To construct a recombinant prokaryotic plasmid of L-ficolin mutant that can express L-ficolin mutant GST-protein. Method The L-ficolin mutant gene derived from the plasmid pCDNA3-L-ficolin by polymerase chain reaction (PCR) was cloned into the prokaryotic expression vector pGEX-KG. The recombinant expression plasmids were transformed into BL21 (DE3) pLySs and expressed. The expression products were analyzed by SDS-PAGE. Result L-ficolin mutant gene was rightly inserted into the vector by restruction enzyme analysis and sequence analysis. The proteins were expressed at high level respectively according to the SDSPAGE results. Conclusinon: The prokaryotic expression vector with L-ficolin mutant gene was efficiently expressed in BL21 (DE3) pLySs bacteria. sites. The result would contribute to further studies of L-ficolin Sugar binding sites.
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