4.7 Article

Directed evolution of glycosyltransferase for enhanced efficiency of avermectin glucosylation

APPLIED MICROBIOLOGY AND BIOTECHNOLOGY (2021)

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Journal

APPLIED MICROBIOLOGY AND BIOTECHNOLOGY
Volume 105, Issue 11, Pages 4599-4607

Publisher

SPRINGER
DOI: 10.1007/s00253-021-11279-x

Keywords

Avermectin glucoside; Glycosyltransferase; Directed evolution; Antinematodal

Categories

Biotechnology & Applied Microbiology

Funding

  1. National Institute of Forest Science, Republic of Korea [FE0702-2016-11-2020]
  2. KRIBB Research Initiative Program, Republic of Korea [KGM2112133]
  3. National Institute of Forest Science (NIFOS), Republic of South Korea [FE0702-2016-11-2020] Funding Source: Korea Institute of Science & Technology Information (KISTI), National Science & Technology Information Service (NTIS)
  4. National Research Council of Science & Technology (NST), Republic of Korea [KGM2112133] Funding Source: Korea Institute of Science & Technology Information (KISTI), National Science & Technology Information Service (NTIS)

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In this study, the catalytic activity of the BLC enzyme on avermectin was enhanced through directed evolution. Mutants R57H, V227A, and D252V showed specific glycosylation activity for avermectin with increased efficiency, and the triple mutant R57H/V227A/D252V demonstrated the highest activity. The best mutant had improved catalytic efficiencies toward avermectin and UDP-glucose and lower free energy than the wild-type BLC, correlating with improved activity.
Avermectin, produced by Streptomyces avermitilis, is an active compound protective against nematodes, insects, and mites. However, its potential usage is limited by its low aqueous solubility. The uridine diphosphate (UDP)-glycosyltransferase (BLC) from Bacillus licheniformis synthesizes avermectin glycosides with improved water solubility and in vitro antinematodal activity. However, enzymatic glycosylation of avermectin by BLC is limited due to the low conversion rate of this reaction. Thus, improving BLC enzyme activity is necessary for mass production of avermectin glycosides for field application. In this study, the catalytic activity of BLC toward avermectin was enhanced via directed evolution. Three mutants from the BLC mutant library (R57H, V227A, and D252V) had specific glucosylation activity for avermectin 2.0-, 1.8-, and 1.5-fold higher, respectively, than wild-type BLC. Generation of combined mutations via site-directed mutagenesis led to even further enhancement of activity. The triple mutant, R57H/V227A/D252V, had the highest activity, 2.8-fold higher than that of wild-type BLC. The catalytic efficiencies (K-cat/K-m) of the best mutant (R57H/V227A/D252V) toward the substrates avermectin and UDP-glucose were improved by 2.71- and 2.29-fold, respectively, compared to those of wild-type BLC. Structural modeling analysis revealed that the free energy of the mutants was - 1.1 to - 7.1 kcal/mol lower than that of wild-type BLC, which was correlated with their improved activity.

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