Substrate specificity mapping of fungal CAZy AA3_2 oxidoreductases

Hongbo Zhao; Johanna Karppi; Owen Mototsune; Daria Poshina; Jenny Svartström; Thi Truc Minh Nguyen; Tri Minh Vo; Adrian Tsang; Emma Master; Maija Tenkanen

doi:10.1186/s13068-024-02491-8

Substrate specificity mapping of fungal CAZy AA3_2 oxidoreductases

Biotechnol Biofuels Bioprod. 2024 Mar 27;17(1):47. doi: 10.1186/s13068-024-02491-8.

Authors

Hongbo Zhao¹, Johanna Karppi², Owen Mototsune³, Daria Poshina⁴, Jenny Svartström⁴, Thi Truc Minh Nguyen⁵, Tri Minh Vo⁵, Adrian Tsang⁵, Emma Master^{3

2}, Maija Tenkanen⁴

Affiliations

¹ Department of Food and Nutrition, University of Helsinki, Helsinki, Finland. hongbo.zhao@helsinki.fi.
² Department of Bioproducts and Biosystems, Aalto University, Espoo, Finland.
³ Department of Chemical Engineering and Applied Chemistry, University of Toronto, Toronto, ON, Canada.
⁴ Department of Food and Nutrition, University of Helsinki, Helsinki, Finland.
⁵ Centre for Structural and Functional Genomics, Concordia University, 7141 Sherbrooke Street West, Montreal, QC, H4B 1R6, Canada.

Abstract

Background: Oxidative enzymes targeting lignocellulosic substrates are presently classified into various auxiliary activity (AA) families within the carbohydrate-active enzyme (CAZy) database. Among these, the fungal AA3 glucose-methanol-choline (GMC) oxidoreductases with varying auxiliary activities are attractive sustainable biocatalysts and important for biological function. CAZy AA3 enzymes are further subdivided into four subfamilies, with the large AA3_2 subfamily displaying diverse substrate specificities. However, limited numbers of enzymes in the AA3_2 subfamily are currently biochemically characterized, which limits the homology-based mining of new AA3_2 oxidoreductases. Importantly, novel enzyme activities may be discovered from the uncharacterized parts of this large subfamily.

Results: In this study, phylogenetic analyses employing a sequence similarity network (SSN) and maximum likelihood trees were used to cluster AA3_2 sequences. A total of 27 AA3_2 proteins representing different clusters were selected for recombinant production. Among them, seven new AA3_2 oxidoreductases were successfully produced, purified, and characterized. These enzymes included two glucose dehydrogenases (TaGdhA and McGdhA), one glucose oxidase (ApGoxA), one aryl alcohol oxidase (PsAaoA), two aryl alcohol dehydrogenases (AsAadhA and AsAadhB), and one novel oligosaccharide (gentiobiose) dehydrogenase (KiOdhA). Notably, two dehydrogenases (TaGdhA and KiOdhA) were found with the ability to utilize phenoxy radicals as an electron acceptor. Interestingly, phenoxy radicals were found to compete with molecular oxygen in aerobic environments when serving as an electron acceptor for two oxidases (ApGoxA and PsAaoA), which sheds light on their versatility. Furthermore, the molecular determinants governing their diverse enzymatic functions were discussed based on the homology model generated by AlphaFold.

Conclusions: The phylogenetic analyses and biochemical characterization of AA3_2s provide valuable guidance for future investigation of AA3_2 sequences and proteins. A clear correlation between enzymatic function and SSN clustering was observed. The discovery and biochemical characterization of these new AA3_2 oxidoreductases brings exciting prospects for biotechnological applications and broadens our understanding of their biological functions.

Keywords: CAZy family AA3_2; Gentiobiose; Oxidoreductase; Phenoxy radical; Sequence similarity network.

Abstract

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