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Programming interchangeable and reversible heterooligomeric protein self-assembly using a bifunctional ligand
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- Authors
- Issue Date
- 2024-02
- Publisher
- Royal Society of Chemistry
- Citation
- Chemical Science, Vol.15 No.8, pp.2975-2983
- Abstract
- Protein design for self-assembly allows us to explore the emergence of protein-protein interfaces through various chemical interactions. Heterooligomers, unlike homooligomers, inherently offer a comprehensive range of structural and functional variations. Besides, the macromolecular repertoire and their applications would significantly expand if protein components could be easily interchangeable. This study demonstrates that a rationally designed bifunctional linker containing an enzyme inhibitor and maleimide can guide the formation of diverse protein heterooligomers in an easily applicable and exchangeable manner without extensive sequence optimizations. As proof of concept, we selected four structurally and functionally unrelated proteins, carbonic anhydrase, aldolase, acetyltransferase, and encapsulin, as building block proteins. The combinations of two proteins with the bifunctional linker yielded four two-component heterooligomers with discrete sizes, shapes, and enzyme activities. Besides, the overall size and formation kinetics of the heterooligomers alter upon adding metal chelators, acidic buffer components, and reducing agents, showing the reversibility and tunability in the protein self-assembly. Given that the functional groups of both the linker and protein components are readily interchangeable, our work broadens the scope of protein-assembled architectures and their potential applications as functional biomaterials. This study illustrates that a carefully designed bifunctional linker can steer the construction of various protein heterooligomers without extensive sequence optimizations, expanding the structural and functional diversity of protein architectures.
- ISSN
- 2041-6520
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