Characterisation of ascocorynin biosynthesis in the purple jellydisc fungus Ascocoryne sarcoides

Carsten Wieder; Roberta Peres da Silva; Jessica Witts; Christof Martin Jäger; Elena Geib; Matthias Brock

doi:10.1186/s40694-022-00138-7

Fungal Biology and Biotechnology (Apr 2022)

Characterisation of ascocorynin biosynthesis in the purple jellydisc fungus Ascocoryne sarcoides

Carsten Wieder,
Roberta Peres da Silva,
Jessica Witts,
Christof Martin Jäger,
Elena Geib,
Matthias Brock

Affiliations

Carsten Wieder: Fungal Biology Group, School of Life Sciences, University of Nottingham
Roberta Peres da Silva: Fungal Biology Group, School of Life Sciences, University of Nottingham
Jessica Witts: Fungal Biology Group, School of Life Sciences, University of Nottingham
Christof Martin Jäger: Sustainable Process Technologies Research Group, Faculty of Engineering, University of Nottingham
Elena Geib: Fungal Biology Group, School of Life Sciences, University of Nottingham
Matthias Brock: Fungal Biology Group, School of Life Sciences, University of Nottingham

DOI: https://doi.org/10.1186/s40694-022-00138-7
Journal volume & issue: Vol. 9, no. 1
pp. 1 – 15

Abstract

Read online

Abstract Background Non-ribosomal peptide synthetase-like (NRPS-like) enzymes are highly enriched in fungal genomes and can be discriminated into reducing and non-reducing enzymes. Non-reducing NRPS-like enzymes possess a C-terminal thioesterase domain that catalyses the condensation of two identical aromatic α-keto acids under the formation of enzyme-specific substrate-interconnecting core structures such as terphenylquinones, furanones, butyrolactones or dioxolanones. Ascocoryne sarcoides produces large quantities of ascocorynin, which structurally resembles a terphenylquinone produced from the condensation of p-hydroxyphenylpyruvate and phenylpyruvate. Since the parallel use of two different substrates by a non-reducing NRPS-like enzyme appeared as highly unusual, we investigated the biosynthesis of ascocorynin in A. sarcoides. Results Here, we searched the genome of A. sarcoides for genes coding for non-reducing NRPS-like enzymes. A single candidate gene was identified that was termed acyN. Heterologous gene expression confirmed that AcyN is involved in ascocorynin production but only produces the non-hydroxylated precursor polyporic acid. Although acyN is embedded in an ascocorynin biosynthesis gene cluster, a gene encoding a monooxygenase required for the hydroxylation of polyporic acid was not present. Expression analyses of all monooxygenase-encoding genes from A. sarcoides identified a single candidate that showed the same expression pattern as acyN. Accordingly, heterologous co-expression of acyN and the monooxygenase gene resulted in the production of ascocorynin. Structural modelling of the monooxygenase suggests that the hydrophobic substrate polyporic acid enters the monooxygenase from a membrane facing entry site and is converted into the more hydrophilic product ascocorynin, which prevents its re-entry for a second round of hydroxylation. Conclusion This study characterises the first naturally occurring polyporic acid synthetase from an ascomycete. It confirms the high substrate and product specificity of this non-reducing NRPS-like enzyme and highlights the requirement of a monooxygenase to produce the terphenylquinone ascocorynin.

Published in Fungal Biology and Biotechnology

ISSN: 2054-3085 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Technology: Chemical technology: Biotechnology
Website: https://fungalbiolbiotech.biomedcentral.com

About the journal

Abstract

Keywords