Literature DB >> 29784819

Xenoprotein engineering via synthetic libraries.

Zachary P Gates1, Alexander A Vinogradov2, Anthony J Quartararo2, Anupam Bandyopadhyay2, Zi-Ning Choo2, Ethan D Evans2, Kathryn H Halloran2, Alexander J Mijalis2, Surin K Mong2, Mark D Simon2, Eric A Standley2, Evan D Styduhar2, Sarah Z Tasker2, Faycal Touti2, Jessica M Weber2, Jessica L Wilson2, Timothy F Jamison2, Bradley L Pentelute1.   

Abstract

Chemical methods have enabled the total synthesis of protein molecules of ever-increasing size and complexity. However, methods to engineer synthetic proteins comprising noncanonical amino acids have not kept pace, even though this capability would be a distinct advantage of the total synthesis approach to protein science. In this work, we report a platform for protein engineering based on the screening of synthetic one-bead one-compound protein libraries. Screening throughput approaching that of cell surface display was achieved by a combination of magnetic bead enrichment, flow cytometry analysis of on-bead screens, and high-throughput MS/MS-based sequencing of identified active compounds. Direct screening of a synthetic protein library by these methods resulted in the de novo discovery of mirror-image miniprotein-based binders to a ∼150-kDa protein target, a task that would be difficult or impossible by other means.

Keywords:  D-protein; flow cytometry; mirror-image miniprotein; protein engineering; xenoprotein

Mesh:

Substances:

Year:  2018        PMID: 29784819      PMCID: PMC6003312          DOI: 10.1073/pnas.1722633115

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  94 in total

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