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作 者:李晔[1,2] 吴敬君[2] 叶逢春[2] 苏楠[2] 张翀[2] 邢新会[2]
机构地区:[1]北京电子科技职业学院,北京100029 [2]清华大学化学工程系生物化工研究所,北京100084
出 处:《生物技术通报》2013年第6期133-139,共7页Biotechnology Bulletin
基 金:国家自然科学基金重点项目(20836004);中国博士后科学基金项目(20100470140);北京电子科技职业学院院内重点课题(YZKB20-11003)
摘 要:肝素酶III(HepC)是肝素结构分析及酶法制备低分子量肝素的重要生物催化剂。为实现HepC在大肠杆菌中的可溶表达,通过PCR方法从肝素黄杆菌(Flavobacterium heparinum)的基因组中扩增得到HepC基因,采用融合蛋白方法构建了麦芽糖结合蛋白(MBP)与HepC融合的表达载体和体系,并在低温(15℃)下诱导重组大肠杆菌,显著提高了MBP-HepC重组表达的可溶性。通过摇瓶培养发酵液的HepC比酶活达到46.41 IU/mg,超过目前报道的最高水平。通过MBP与直链淀粉的亲和吸附实现了MBP-HepC的亲和分离和纯化,一步亲和纯化后蛋白的纯度即可达95%以上。该融合酶基本特性研究表明,融合肝素酶III(MBP-HepC)的最适作用pH7.3,最适作用温度为42℃-48℃。热稳定性较好,其30℃时的稳定性高于融合肝素酶I(MBP-HepA)。Heparinase III is an important enzyme for heparin structure analysis and low molecular weight heparin production.To achieve the soluble expression of HepC with high activity in recombinant E.coli,the heparinase III gene(hepC)from Flavobacterium heparinum was amplified by the PCR method,and the fusion expression vector and system of expressing fusion protein of a maltose binding protein(MBP) and HepC were constructed.The results showed that the fusion strategy by using MBP was effective to enhance solubility of the MBP-HepC when induced at low temperature of 15℃.By shake flask cultivation,the specific enzyme activity of MBP-HepC could reach about 46.41 IU/mg,which was the highest among the values reported so far.By one-step affinity purification with amylose resin,the MBP-HepC fusion protein was easily purified to more than 95% purity.The enzyme characteristic study showed that the optimum pH value of MBP-HepC was 7.3,the optimum reaction temperature was 42℃-48℃,and the thermal stability of MBP-HepC is better than Heparinase I(MBP-HepA)at 30℃.
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