4.6 Article

Immobilized Trienzymatic System with Enhanced Stabilization for the Biotransformation of Lactose

Journal

MOLECULES
Volume 22, Issue 2, Pages -

Publisher

MDPI AG
DOI: 10.3390/molecules22020284

Keywords

beta -galactosidase; l-arabinose isomerase; d-glucose isomerase; enzyme immobilization; D-tagatose; D-fructose

Funding

  1. Programa de Desarrollo de las Ciencias Basicas (PEDECIBA-Quimica)
  2. Agencia Nacional de Investigacion e Innovacion (ANII)
  3. Comision Sectorial de Investigacion Cientifica (CAP-CSIC-UdelaR)
  4. FUNDAQUIM

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The use of ketohexose isomerases is a powerful tool in lactose whey processing, but these enzymes can be very sensitive and expensive. Development of immobilized/stabilized biocatalysts could be a further option to improve the process. In this work, -galactosidase from Bacillus circulans, l-arabinose (d-galactose) isomerase from Enterococcus faecium, and d-xylose (d-glucose) isomerase from Streptomyces rubiginosus were immobilized individually onto Eupergit C and Eupergit C 250 L. Immobilized activity yields were over 90% in all cases. With the purpose of increasing thermostability of derivatives, two post-immobilization treatments were performed: alkaline incubation to favor the formation of additional covalent linkages, and blocking of excess oxirane groups by reacting with glycine. The greatest thermostability was achieved when alkaline incubation was carried out for 24 h, producing l-arabinose isomerase-Eupergit C derivatives with a half-life of 379 h and d-xylose isomerase-Eupergit C derivatives with a half-life of 554 h at 50 degrees C. Preliminary assays using immobilized and stabilized biocatalysts sequentially to biotransform lactose at pH 7.0 and 50 degrees C demonstrated improved performances as compared with soluble enzymes. Further improvements in ketohexose productivities were achieved when the three single-immobilizates were incubated simultaneously with lactose in a mono-reactor system.

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