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This work exemplifies the advantages of using a battery of new heterofunctional epoxy supports to immobilize enzymes. We have compared the performance of a standard Sepabeads-epoxy support with other Sepabeads-epoxy supports partially modified with boronate, iminodiacetic, metal chelates, and ethylenediamine in the immobilization of the thermostable beta-galactosidase from Thermus sp. strain T2 as a model system. Immobilization yields depended on the support, ranging from 95% using Sepabeads-epoxy-chelate, Sepabeads-epoxy-amino, or Sepabeads-epoxy-boronic to 5% using Sepabeads-epoxy-IDA. Moreover, immobilization rates were also very different when using different supports. Remarkably, the immobilized beta-galactosidase derivatives showed very improved but different stabilities after favoring multipoint covalent attachment by long-term alkaline incubation, the enzyme immobilized on Sepabeads-epoxy-boronic being the most stable. This derivative had some subunits of the enzyme not covalently attached to the support (detected by SDS-PAGE). This is a problem if the biocatalysts were to be used in food technology. The optimization of the cross-linking with aldehyde-dextran permitted the full stabilization of the quaternary structure of the enzyme. The optimal derivative was very active in lactose hydrolysis even at 70 degrees C (over 1000 IU/g), maintaining its activity after long incubation times under these conditions and with no risk of product contamination with enzyme subunits.
Aldehydes, Polymers, Protein Conformation, Hydrolysis, Dextrans, Lactose, Enzymes, Immobilized, beta-Galactosidase, Enzyme Activation, Species Specificity, Enzyme Stability, Epoxy Compounds, Adsorption, Thermus, Protein Structure, Quaternary, Dimerization
Aldehydes, Polymers, Protein Conformation, Hydrolysis, Dextrans, Lactose, Enzymes, Immobilized, beta-Galactosidase, Enzyme Activation, Species Specificity, Enzyme Stability, Epoxy Compounds, Adsorption, Thermus, Protein Structure, Quaternary, Dimerization
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