A De Novo-Designed Type 3 Copper Protein Tunes Catechol Substrate Recognition and Reactivity

被引:16
|
作者
Pirro, Fabio [1 ]
La Gatta, Salvatore [1 ]
Arrigoni, Federica [2 ]
Famulari, Antonino [3 ,4 ]
Maglio, Ornella [1 ,5 ]
Del Vecchio, Pompea [1 ]
Chiesa, Mario [3 ]
De Gioia, Luca [2 ]
Bertini, Luca [2 ]
Chino, Marco [1 ]
Nastri, Flavia [1 ]
Lombardi, Angela [1 ]
机构
[1] Univ Naples Federico II, Dept Chem Sci, Via Cintia, I-80126 Naples, Italy
[2] Univ Milano Bicocca, Dept Biotechnol & Biosci, Piazza Sci 2, I-20126 Milan, Italy
[3] Univ Torino, Dept Chem, Via Giuria 9, I-10125 Turin, Italy
[4] Univ Zaragoza, Dept Condensed Matter Phys, Calle Pedro Cerbuna 12, Zaragoza 50009, Spain
[5] Natl Res Council CNR, Inst Biostruct & Bioimaging IBB, Via Pietro Castellino 111, I-80131 Naples, Italy
关键词
Artificial Metalloenzymes; Phenol Oxidases; Protein Design; Substrate Selectivity; T3 di-Copper Site; DE-NOVO; ARTIFICIAL METALLOENZYMES; ACTIVE-SITES; OXIDASE; METALLOPROTEINS; TYROSINASE; COMPLEXES; EVOLUTION; CATALYSIS; RESONANCE;
D O I
10.1002/anie.202211552
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
De novo metalloprotein design is a remarkable approach to shape protein scaffolds toward specific functions. Here, we report the design and characterization of Due Rame 1 (DR1), a de novo designed protein housing a di-copper site and mimicking the Type 3 (T3) copper-containing polyphenol oxidases (PPOs). To achieve this goal, we hierarchically designed the first and the second di-metal coordination spheres to engineer the di-copper site into a simple four-helix bundle scaffold. Spectroscopic, thermodynamic, and functional characterization revealed that DR1 recapitulates the T3 copper site, supporting different copper redox states, and being active in the O-2-dependent oxidation of catechols to o-quinones. Careful design of the residues lining the substrate access site endows DR1 with substrate recognition, as revealed by Hammet analysis and computational studies on substituted catechols. This study represents a premier example in the construction of a functional T3 copper site into a designed four-helix bundle protein.
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页数:10
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