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Omniligase-1-Mediated Phage-Peptide Library Modification and Insulin Engineering.

Authors :
Zhang YW
Lin NP
Guo X
Szabo-Fresnais N
Ortoleva PJ
Chou DH
Source :
ACS chemical biology [ACS Chem Biol] 2024 Feb 16; Vol. 19 (2), pp. 506-515. Date of Electronic Publication: 2024 Jan 24.
Publication Year :
2024

Abstract

Chemical and enzymatic modifications of peptide-displayed libraries have been successfully employed to expand the phage display library. However, the requirement of specific epitopes and scaffolds has limited the scope of protein engineering using phage display. In this study, we present a novel approach utilizing omniligase-1-mediated selective and specific ligation on the phage pIII protein, offering a high conversion rate and compatibility with commercially available phage libraries. We applied this method to perform high-throughput engineering of insulin analogues with randomized B chain C-terminal regions. Insulin analogues with different B chain C-terminal segments were selected and exhibited biological activity equivalent to that of human insulin. Molecular dynamics studies of insulin analogues revealed a novel interaction between the insulin B27 residue and insulin receptor L1 domain. In summary, our findings highlight the potential of omniligase-1-mediated phage display in the development and screening of disulfide-rich peptides and proteins. This approach holds promise for the creation of novel insulin analogues with enhanced therapeutic properties and exhibits potential for the development of other therapeutic compounds.

Details

Language :
English
ISSN :
1554-8937
Volume :
19
Issue :
2
Database :
MEDLINE
Journal :
ACS chemical biology
Publication Type :
Academic Journal
Accession number :
38266161
Full Text :
https://doi.org/10.1021/acschembio.3c00685