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Immobilization of Mucor javanicus lipase on effectively functionalized silica nanoparticles
Authors:Moon Il Kim   Hyun Ok Ham   Seong-Dae Oh   Hyun Gyu Park   Ho Nam Chang  Seong-Ho Choi
Affiliation:

aDepartment of Chemical and Biomolecular Engineering, Korea Advanced Institute of Science and Technology, Daejeon 305-701, Republic of Korea

bDepartment of Chemistry, Hannam University, 133 Ojeong-dong, Daeduck-gu, Daejeon, Republic of Korea

Abstract:Mucor javanicus lipase was effectively immobilized on silica nanoparticles which were prepared by Stöber method. Glycidyl methacrylate (GMA), which bears a reactive epoxide group, was incorporated onto the surface of the nanoparticles and the epoxide groups were directly used for multipoint coupling of the enzyme. We also introduced amine residues by coupling ethylene diamine (EDA) to the epoxide group of GMA. M. javanicus lipase was covalently immobilized onto the amine-activated silica nanoparticles by using glutaraldehyde (GA) or 1,4 phenylene diisothiocyanate (NCS) as a coupling agent. The lipase loading capacities of the EDA-GA and EDA-NCS nanoparticles (81.3 and 60.9 mg g−1, respectively) were much higher than that of the unmodified GMA nanoparticles (18.9 mg g−1). The relative hydrolytic activities in an aqueous medium of the lipases immobilized on EDA-GA and EDA-NCS attached silica nanoparticles (115% and 107%, respectively) were significantly high and almost in the same range with the free enzyme. This may be due to the improvement of the enzyme–substrate interaction by avoiding the potential aggregation of free lipase molecules. The immobilized lipases were also more resistant to temperature inactivation than the free form. This work demonstrates that the size-controlled silica nanoparticles can be efficiently employed as host materials for enzyme immobilization leading to high activity and stability of the immobilized enzymes.
Keywords:Mucor javanicus lipase   Silica nanoparticles   Covalent attachment   High activity   Stability
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