Metal-Mediated Protein Assembly Using a Genetically Incorporated Metal-Chelating Amino Acid

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Many natural proteins function in oligomeric forms, which are critical for their sophisticated functions. The construction of protein assemblies has great potential for biosensors, enzyme catalysis, and biomedical applications. In designing protein assemblies, a critical process is to create protein-protein interaction (PPI) networks at defined sites of a target protein. Although a few methods are available for this purpose, most of them are dependent on existing PPIs of natural proteins to some extent. In this report, a metal-chelating amino acid, 2,2 '-bipyridylalanine (BPA), was genetically introduced into defined sites of a monomeric protein and used to form protein oligomers. Depending on the number of BPAs introduced into the protein and the species of metal ions (Ni2+ and Cu2+), dimers or oligomers with different oligomerization patterns were formed by complexation with a metal ion. Oligomer sizes could also be controlled by incorporating two BPAs at different locations with varied angles to the center of the protein. When three BPAs were introduced, the monomeric protein formed a large complex with Ni2+. In addition, when Cu2+ was used for complex formation with the protein containing two BPAs, a linear complex was formed. The method proposed in this report is technically simple and generally applicable to various proteins with interesting functions. Therefore, this method would be useful for the design and construction of functional protein assemblies.
Publisher
AMER CHEMICAL SOC
Issue Date
2020-12
Language
English
Article Type
Article
Citation

BIOMACROMOLECULES, v.21, no.12, pp.5021 - 5028

ISSN
1525-7797
DOI
10.1021/acs.biomac.0c01194
URI
http://hdl.handle.net/10203/280038
Appears in Collection
MSE-Journal Papers(저널논문)
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