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Construction and Transduction of SARS-3CL Protease Gene in Baculovirus Vector / 天津医药
Tianjin Medical Journal ; (12): 550-552,后插3, 2009.
Article de Zh | WPRIM | ID: wpr-600345
Bibliothèque responsable: WPRO
ABSTRACT
Objective: To construct severe acute respiratory syndrome (SARS)coronavirus 3CL protease gene into transforming vector prepare recombinant baculovirus and transduct it into infect insect cells to express SARS-3CL protease. Mothods: The 3cl-Teasy and pFastBac HTb bacmida were amplified. The 3cl gene was cloned into baculovirus transforming vector pFastBac HTb by enzyme-digest- and-ligase method,which was named recombinant pFB HTb-3cl. The pFB HTB-3cl was transformed into E.coli DH10Bac competent cells.The positive colonies were screened by three antibiotics and blue-white patch method. The bacmid-HTb-3cl recombinant baculovirus bacmid was obtained and purified to transfect St9 insect cells.The protease expressed in Sf9 insect cells were identified by SDS-PAGE. Results: Recombinant expression vector was obtained successfully. The 3CL protease expressed in insect cells were identified by SDS-PAGE. Conclusion: The expression of 3CL protease in insect cells provided foundation for detecting protein activities and screening inhibitor against SARS-3CL protease.
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Texte intégral: 1 Indice: WPRIM langue: Zh Texte intégral: Tianjin Medical Journal Année: 2009 Type: Article
Texte intégral: 1 Indice: WPRIM langue: Zh Texte intégral: Tianjin Medical Journal Année: 2009 Type: Article