Journal
ACS CATALYSIS
Volume 10, Issue 1, Pages 891-+Publisher
AMER CHEMICAL SOC
DOI: 10.1021/acscatal.9b05080
Keywords
protein design; peroxidase; substrate binding site; X-ray crystallography; EPR; molecular docking
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Funding
- National Natural Science Foundation of China [21977042]
- Special Scientific Research Funds for Central Nonprofit Institutes, Yellow Sea Fisheries Research Institute, Chinese Academy of Fishery Sciences [20603022016011]
- Financial Fund of the ministry of Agriculture and Rural Affairs, China (NFZX2018)
- Human Provincial Innovation Foundation for Postgraduate [CX20190729]
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Functional enzyme design has made tremendous progress, but designer enzymes with activities comparable to those of natural enzymes are still limited. In this study, we rationally engineered a functional peroxidase with a catalytic binding site of guaiacol in a model protein, myoglobin (Mb), by replacing Phe46 with a serine (F46S mutation), together with a distal Tyr in the heme pocket (F43Y mutation). The double mutant F43Y/F46S Mb exhibited an overall catalytic efficiency that exceeds most natural peroxidases and is similar to the most efficient horseradish peroxidase. The catalytic substrate binding site was further confirmed by X-ray crystallography, EPR spectroscopy, and inhibition studies, as well as molecular docking simulations. Remarkably, this study reports an artificial peroxidase with an engineered catalytic binding site whose structure was solved both in the absence and presence of the substrate.
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