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dc.contributor.authorWu, Yue-Jinen_US
dc.contributor.authorCheng, Chih-Yuen_US
dc.contributor.authorLi, Yaw-Kuenen_US
dc.date.accessioned2014-12-08T15:09:04Z-
dc.date.available2014-12-08T15:09:04Z-
dc.date.issued2009-08-01en_US
dc.identifier.issn0009-4536en_US
dc.identifier.urihttp://hdl.handle.net/11536/6904-
dc.description.abstractThe gene of Serratia marcescens chitinase A (chiA) was cloned by PCR. The complete gene was constructed into a pRSET vector and expressed in Escherichia coli. The recombinant enzyme was purified to > 90% homogeneity by hydrophobic interaction chromatography followed by ion-exchange separation. Measured with an electrospray-ionization mass spectrometer, the molecular mass of the protein was 58,607 Da, consistent with a theoretical calculation of the deduced protein without the signal peptide. The recombinant enzyme was characterized and tested for the preparation of chitobiose. In general, the recombinant Chtinase A exhibited an exo-type catalytic activity toward colloidal chitin and released both N-acetylglucosamine and N,N-diacetyl chitobiose as products. After extensive testing, we produced N,N-diacetyl chitobiose as the predominant product when the enzymatic reaction was performed in sodium acetate buffer at pH 5.5; under such conditions, an enzymatic process is established for the production of the disaccharide on a 100-g scale.en_US
dc.language.isoen_USen_US
dc.subjectSerratia marcescensen_US
dc.subjectChitinase Aen_US
dc.subjectColloidal chitinen_US
dc.subjectN,N-Diacetyl chitobioseen_US
dc.titleCloning and Expression of Chitinase A from Serratia marcescens for Large-scale Preparation of N,N-Diacetyl Chitobioseen_US
dc.typeArticleen_US
dc.identifier.journalJOURNAL OF THE CHINESE CHEMICAL SOCIETYen_US
dc.citation.volume56en_US
dc.citation.issue4en_US
dc.citation.spage688en_US
dc.citation.epage695en_US
dc.contributor.department應用化學系zh_TW
dc.contributor.departmentDepartment of Applied Chemistryen_US
dc.identifier.wosnumberWOS:000269961800005-
dc.citation.woscount3-
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