AI Article Synopsis

  • A novel β-glucosidase named BbBgl was discovered from ATCC 15700 and successfully engineered to convert ginsenoside F into compound K (CK) by hydrolyzing ginsenoside Rd.
  • The enzyme was purified and showed high activity (37 U/mg protein) at optimal conditions of pH 5.0 and 35°C, with a significantly extended half-life of 180 hours.
  • BbBgl demonstrated impressive tolerance to high substrate concentrations, achieving a 96% conversion of ginsenoside Rd in 12 hours, making it promising for large-scale production of rare ginsenosides like CK.

Article Abstract

To investigate a novel β-glucosidase from ATCC 15700 (BbBgl) to produce compound K (CK) via ginsenoside F by highly selective and efficient hydrolysis of the C-3 glycoside from ginsenoside Rd, the gene was cloned and expressed in BL21. The recombinant BbBgl was purified by Ni-NTA magnetic beads to obtain an enzyme with specific activity of 37 U/mg protein using NP-Glc as substrate. The enzyme activity was optimized at pH 5.0, 35°C, 2 or 6 U/ml, and its activity was enhanced by Mn significantly. Under the optimal conditions, the half-life of the BbBgl is 180 h, much longer than the characterized β-glycosidases, and the K and V values are 2.7 mM and 39.8 µmol/mg/min for ginsenoside Rd. Moreover, the enzyme exhibits strong tolerance against high substrate concentration (up to 40 g/l ginsenoside Rd) with a molar biotransformation rate of 96% within 12 h. The good enzymatic properties and gram-scale conversion capacity of BbBgl provide an attractive method for large-scale production of rare ginsenoside CK using a single enzyme or a combination of enzymes.

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Source
http://dx.doi.org/10.4014/jmb.1808.08059DOI Listing

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