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    HUANG Zhiª²li, LUO Liª²xin, LING Junª²jian, YANG Ruª²di, LIANG Shiª²zhong

    The College of Food Engineering and Biotechnology, South China University of Technology,Guangzhou,Guangdong 510640

    Abstract In this study, the nattokinase(NK) gene was amplified by PCR with bacillus subtilis genomic DNA as the template and cloned into PUC19 vector. After analyzed by restriction enzyme and PCR, the NK gene was cloned into the expression vector and expressed in E. coli. It was shown that the expression products have the fibrinolytic activity determined by CLT and the expression protein accounted for 12% of the total cell protein by SDSª²PAGE.The optimum cultivating and inducing times were determined as 6 h and 5 h respectively.

    Key words nattokinase;gene cloning;gene expression

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