Frontiers in Molecular Biosciences (Aug 2023)

Exploring rigid-backbone protein docking in biologics discovery: a test using the DARPin scaffold

  • Francis Gaudreault,
  • Jason Baardsnes,
  • Yuliya Martynova,
  • Aurore Dachon,
  • Hervé Hogues,
  • Christopher R. Corbeil,
  • Enrico O. Purisima,
  • Mélanie Arbour,
  • Traian Sulea,
  • Traian Sulea

DOI
https://doi.org/10.3389/fmolb.2023.1253689
Journal volume & issue
Vol. 10

Abstract

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Accurate protein-protein docking remains challenging, especially for artificial biologics not coevolved naturally against their protein targets, like antibodies and other engineered scaffolds. We previously developed ProPOSE, an exhaustive docker with full atomistic details, which delivers cutting-edge performance by allowing side-chain rearrangements upon docking. However, extensive protein backbone flexibility limits its practical applicability as indicated by unbound docking tests. To explore the usefulness of ProPOSE on systems with limited backbone flexibility, here we tested the engineered scaffold DARPin, which is characterized by its relatively rigid protein backbone. A prospective screening campaign was undertaken, in which sequence-diversified DARPins were docked and ranked against a directed epitope on the target protein BCL-W. In this proof-of-concept study, only a relatively small set of 2,213 diverse DARPin interfaces were selected for docking from the huge theoretical library from mutating 18 amino-acid positions. A computational selection protocol was then applied for enrichment of binders based on normalized computed binding scores and frequency of binding modes against the predefined epitope. The top-ranked 18 designed DARPin interfaces were selected for experimental validation. Three designs exhibited binding affinities to BCL-W in the nanomolar range comparable to control interfaces adopted from known DARPin binders. This result is encouraging for future screening and engineering campaigns of DARPins and possibly other similarly rigid scaffolds against targeted protein epitopes. Method limitations are discussed and directions for future refinements are proposed.

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