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Bifurcate evolution of quinone synthetases in basidiomycetes
by
Gressler, Markus
, Stallforth, Pierre
, Raztsou, Ihar
, Arndt, Hans-Dieter
, Hoffmeister, Dirk
, Lawrinowitz, Stefanie
, Seibold, Paula Sophie
in
Adenylation
/ Amino acids
/ Applied Microbiology
/ Atromentin
/ Basidiomycota
/ Biofilms
/ Bioinformatics
/ Biological products
/ Biomedical and Life Sciences
/ Biosynthesis
/ Biotechnology
/ Consortia
/ Dioxygenase
/ Enzymes
/ Evolution
/ Genomes
/ Hapalopilus
/ Life Sciences
/ Ligases
/ Liquid chromatography
/ Mass spectrometry
/ Mass spectroscopy
/ Microbial Genetics and Genomics
/ Microbiology
/ Microorganisms
/ Mushrooms
/ Mycology
/ Natural products
/ Phylogenetics
/ Phylogeny
/ Pigments
/ Plant Pathology
/ Polyporic acid
/ Proteins
/ Quinone
/ Quinone synthetase
/ Quinones
/ Scientific imaging
/ Substrate specificity
/ Substrates
2023
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Bifurcate evolution of quinone synthetases in basidiomycetes
by
Gressler, Markus
, Stallforth, Pierre
, Raztsou, Ihar
, Arndt, Hans-Dieter
, Hoffmeister, Dirk
, Lawrinowitz, Stefanie
, Seibold, Paula Sophie
in
Adenylation
/ Amino acids
/ Applied Microbiology
/ Atromentin
/ Basidiomycota
/ Biofilms
/ Bioinformatics
/ Biological products
/ Biomedical and Life Sciences
/ Biosynthesis
/ Biotechnology
/ Consortia
/ Dioxygenase
/ Enzymes
/ Evolution
/ Genomes
/ Hapalopilus
/ Life Sciences
/ Ligases
/ Liquid chromatography
/ Mass spectrometry
/ Mass spectroscopy
/ Microbial Genetics and Genomics
/ Microbiology
/ Microorganisms
/ Mushrooms
/ Mycology
/ Natural products
/ Phylogenetics
/ Phylogeny
/ Pigments
/ Plant Pathology
/ Polyporic acid
/ Proteins
/ Quinone
/ Quinone synthetase
/ Quinones
/ Scientific imaging
/ Substrate specificity
/ Substrates
2023
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Bifurcate evolution of quinone synthetases in basidiomycetes
by
Gressler, Markus
, Stallforth, Pierre
, Raztsou, Ihar
, Arndt, Hans-Dieter
, Hoffmeister, Dirk
, Lawrinowitz, Stefanie
, Seibold, Paula Sophie
in
Adenylation
/ Amino acids
/ Applied Microbiology
/ Atromentin
/ Basidiomycota
/ Biofilms
/ Bioinformatics
/ Biological products
/ Biomedical and Life Sciences
/ Biosynthesis
/ Biotechnology
/ Consortia
/ Dioxygenase
/ Enzymes
/ Evolution
/ Genomes
/ Hapalopilus
/ Life Sciences
/ Ligases
/ Liquid chromatography
/ Mass spectrometry
/ Mass spectroscopy
/ Microbial Genetics and Genomics
/ Microbiology
/ Microorganisms
/ Mushrooms
/ Mycology
/ Natural products
/ Phylogenetics
/ Phylogeny
/ Pigments
/ Plant Pathology
/ Polyporic acid
/ Proteins
/ Quinone
/ Quinone synthetase
/ Quinones
/ Scientific imaging
/ Substrate specificity
/ Substrates
2023
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Bifurcate evolution of quinone synthetases in basidiomycetes
Journal Article
Bifurcate evolution of quinone synthetases in basidiomycetes
2023
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Overview
Background
The terphenylquinones represent an ecologically remarkable class of basidiomycete natural products as they serve as central precursors of pigments and compounds that impact on microbial consortia by modulating bacterial biofilms and motility. This study addressed the phylogenetic origin of the quinone synthetases that assemble the key terphenylquinones polyporic acid and atromentin.
Results
The activity of the
Hapalopilus rutilans
synthetases HapA1, HapA2 and of
Psilocybe cubensis
PpaA1 were reconstituted in Aspergilli. Liquid chromatography and mass spectrometry of the culture extracts identified all three enzymes as polyporic acid synthetases. PpaA1 is unique in that it features a C-terminal, yet catalytically inactive dioxygenase domain. Combined with bioinformatics to reconstruct the phylogeny, our results demonstrate that basidiomycete polyporic acid and atromentin synthetases evolved independently, although they share an identical catalytic mechanism and release structurally very closely related products. A targeted amino acid replacement in the substrate binding pocket of the adenylation domains resulted in bifunctional synthetases producing both polyporic acid and atromentin.
Conclusions
Our results imply that quinone synthetases evolved twice independently in basidiomycetes, depending on the aromatic α-keto acid substrate. Furthermore, key amino acid residues for substrate specificity were identified and changed which led to a relaxed substrate profile. Therefore, our work lays the foundation for future targeted enzyme engineering.
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