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Combined use of versatile peroxidase and aryl alcohol oxidase of Pleurotus eryngii to decolorize melanin on the skin

Authors
Park, Kyung HyeLim, HeawonBaik, JinaNho, Youn-HwaKim, MisunKang, SeunghyunKang, Taek Jin
Issue Date
Oct-2024
Publisher
Elsevier Applied Science
Keywords
Versatile peroxidase; Aryl alcohol oxidase; Enzymatic melanin decolorization
Citation
Process Biochemistry, v.145, pp 221 - 228
Pages
8
Indexed
SCIE
SCOPUS
Journal Title
Process Biochemistry
Volume
145
Start Page
221
End Page
228
URI
https://scholarworks.dongguk.edu/handle/sw.dongguk/22689
DOI
10.1016/j.procbio.2024.06.035
ISSN
1359-5113
1873-3298
Abstract
Melanin plays an important role in protecting skin cells from harmful UV radiation, but its uneven pigmentation in the skin sometimes demands cosmetic resolution. As a safe and effective way of evening the skin tone, enzymatic decolorization of melanin at the stratum corneum has been proposed. In this regard, the use of lignin peroxidase, in the presence of hydrogen peroxide and veratryl alcohol, an electron mediator, has been explored. Here, we first show that versatile peroxidase (VP) and aryl alcohol oxidase (AAO) purified from the Pleurotus eryngii liquid culture can be used to decolorize melanin without exogenous hydrogen peroxide. This resembles the oxidative degradation pathway of lignin in nature; AAO generates hydrogen peroxide from veratryl alcohol, and VP utilizes generated hydrogen peroxide while using veratryl alcohol as a mediator. We further explored the use of POX_Pe, the crude peroxidase preparation of the Pleurotus eryngii liquid culture, for melanin decolorization because of its better stability. Using POX_Pe and veratryl alcohol, over 60 % of melanin decolorization was obtained in 1 h in the absence of exogenous hydrogen peroxide addition. Furthermore, POX_Pe could decolorize melanin in a 3D human pigmented epidermis model, demonstrating its possible applications in cosmetics.
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