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Preparation and application of epoxyachitosan/alginate support in the immobilization of microbial lipases by covalent attachment
The aim of this work was the preparation and application of highly hydrophobic epoxyachitosan/alginate as a support to immobilize microbial lipases from Thermomyces lanuginosus commercially available as Lipolase registered (TLL1) and Lipex registered 100L (TLL2) and Pseudomonas fluorescens (PFL). Th...
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Published in: | Reactive & functional polymers 2013-01, Vol.73 (1), p.160-167 |
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Main Authors: | , , , , |
Format: | Article |
Language: | English |
Subjects: | |
Online Access: | Get full text |
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Summary: | The aim of this work was the preparation and application of highly hydrophobic epoxyachitosan/alginate as a support to immobilize microbial lipases from Thermomyces lanuginosus commercially available as Lipolase registered (TLL1) and Lipex registered 100L (TLL2) and Pseudomonas fluorescens (PFL). The catalytic properties of the biocatalysts were assayed in olive oil hydrolysis and butyl butyrate synthesis. The results indicated that 12 h was enough for TLL1 to be immobilized on the support. Covalent attachment of TLL1 turned biocatalysts highly active and around 6-fold more stable than free lipase. Based on the results, a time of incubation of 24 h was selected for further studies about the maximum immobilized protein amount and butyl butyrate synthesis. Maximum protein loading immobilized was found to be 25.4 mg g-1 support for TLL1, followed by TLL2 (20.5 mg g-1) and PFL (15.5 mg g-1) offering 80 mg protein g-1 support. The immobilization of TLL1 and TLL2 resulted in highly active biocatalysts (around 1300 IU g-1 gel), almost fivefold higher than PFL (272.4 IU g-1 gel). In butyl butyrate synthesis, PFL showed similar activity to TLL1 and TLL2 derivatives, up to 60 mmol L-1. The biocatalysts displayed high activity after five successive cycles, retaining around 95% of the initial activity. |
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ISSN: | 1381-5148 |