Frontiers in Chemical Biology (Jul 2024)

In silico enzyme screening identifies an SDR ketoreductase from Thermus caliditerrae as an attractive biocatalyst and promising candidate for protein engineering

  • Yvett Sosa,
  • Yvett Sosa,
  • Bhav Kapur,
  • Bhav Kapur,
  • Jessica Hurtak,
  • Laura J. Kingsley,
  • Hao Wu,
  • Stefanie Gruber,
  • Herbert Nar,
  • Saad Khattabi,
  • Jesus Seco Moral,
  • Maria Fátima Lucas,
  • Caterina Martin,
  • Nikola Lončar,
  • Frederic Buono,
  • Noah Pefaur,
  • Andrew E. Nixon,
  • Jinhua J. Song

DOI
https://doi.org/10.3389/fchbi.2024.1425501
Journal volume & issue
Vol. 3

Abstract

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Introduction: Biocatalysis, particularly through engineered enzymes, presents a cost-effective, efficient, and eco-friendly approach to compound synthesis. We sought to identify ketoreductases capable of synthesizing optically pure alcohols or ketones, essential chiral building blocks for active pharmaceutical ingredients.Methods: Using BioMatchMaker®, an in silico high-throughput platform that allows the identification of wild-type enzyme sequences for a desired chemical transformation, we identified a bacterial SDR ketoreductase from Thermus caliditerrae, Tcalid SDR, that demonstrates favorable reaction efficiency and desired enantiomeric excess.Results: Here we present two crystal structures of the Tcalid SDR in an apo-form at 1.9 Å and NADP-complexed form at 1.7 Å resolution (9FE6 and 9FEB, respectively). This enzyme forms a homotetramer with each subunit containing an N-terminal Rossmann-fold domain. We use computational analysis combined with site-directed mutagenesis and enzymatic characterization to define the substrate-binding pocket. Furthermore, the enzyme retained favorable reactivity and selectivity after incubation at elevated temperature.Conclusion: The enantioselectivity combined with the thermostability of Tcalid SDR makes this enzyme an attractive engineering starting point for biocatalysis applications.

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