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1. Understanding the biosynthesis, metabolic regulation, and anti-phytopathogen activity of 3,7-dihydroxytropolone in Pseudomonas spp.

Author

Alaster D. Moffat, Lars Höing, Javier Santos-Aberturas, Tim Markwalder, Jacob G. Malone, Robin Teufel, and Andrew W. Truman

Subjects
natural antimicrobial products, biosynthesis, Pseudomonas, specialized metabolism, biosynthetic gene cluster, Microbiology, QR1-502
Abstract

ABSTRACT The genus Pseudomonas is a prolific source of specialized metabolites with significant biological activities, including siderophores, antibiotics, and plant hormones. These molecules play pivotal roles in environmental interactions, influencing pathogenicity, inhibiting microorganisms, responding to nutrient limitation and abiotic challenges, and regulating plant growth. These properties mean that pseudomonads are suitable candidates as biological control agents against plant pathogens. Multiple transposon-based screens have identified a Pseudomonas biosynthetic gene cluster (BGC) associated with potent antibacterial and antifungal activities, which produces 7-hydroxytropolone (7-HT). In this study, we show that this BGC also makes 3,7-dihydroxytropolone (3,7-dHT), which has strong antimicrobial activity toward Streptomyces scabies, a potato pathogen. Through metabolomics and reporter assays, we unveil the involvement of cluster-situated genes in generating phenylacetyl-coenzyme A, a key precursor for tropolone biosynthesis via the phenylacetic acid catabolon. The clustering of these phenylacetic acid genes within tropolone BGCs is unusual in other Gram-negative bacteria. Our findings support the interception of phenylacetic acid catabolism via an enoyl-CoA dehydratase encoded in the BGC, as well as highlighting an essential role for a conserved thioesterase in biosynthesis. Biochemical assays were used to show that this thioesterase functions after a dehydrogenation–epoxidation step catalyzed by a flavoprotein. We use this information to identify diverse uncharacterized BGCs that encode proteins with homology to flavoproteins and thioesterases involved in tropolone biosynthesis. This study provides insights into tropolone biosynthesis in Pseudomonas, laying the foundation for further investigations into the ecological role of tropolone production.IMPORTANCEPseudomonas bacteria produce various potent chemicals that influence interactions in nature, such as metal-binding molecules, antibiotics, or plant hormones. This ability to synthesize bioactive molecules means that Pseudomonas bacteria may be useful as biological control agents to protect plants from agricultural pathogens, as well as a source of antibiotic candidates. We have identified a plant-associated Pseudomonas strain that can produce 3,7-dihydroxytropolone, which has broad biological activity and can inhibit the growth of Streptomyces scabies, a bacterium that causes potato scab. Following the identification of this molecule, we used a combination of genetic, chemical, and biochemical experiments to identify key steps in the production of tropolones in Pseudomonas species. Understanding this biosynthetic process led to the discovery of an array of diverse pathways that we predict will produce new tropolone-like molecules. This work should also help us shed light on the natural function of antibiotics in nature.

Published
2024
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2. Mass Spectrometric Analysis of Cucurbitacins and Dihydrocucurbitacins from the Tuber of Citrullus naudinianus

Author

Moritz Benka, Kristof Görlitz, Michael C. Schöttgen, Simon Lagies, Daniel A. Mohl, Michel Kather, Iwanette Du Preez-Bruwer, Davis Mumbengegwi, Robin Teufel, Stefanie Kowarschik, Roman Huber, Dietmar A. Plattner, and Bernd Kammerer

Subjects
Citrullus naudinianus, cucurbitacins, 23,24-dihydrocucurbitacins, HPLC, MS, MS/MS, Microbiology, QR1-502
Abstract

The vast pool of structurally and functionally distinct secondary metabolites (i.e., natural products (NPs)) is constantly being expanded, a process also driven by the rapid progress in the development of analytical techniques. Such NPs often show potent biological activities and are therefore prime candidates for drug development and medical applications. The ethyl acetate extract of the tuber of Citrullus naudinianus (C. naudinianus), an African melon with edible fruits and seeds, shows in vitro immunomodulatory activity presumably elicited by cucurbitacins that are known major constituents of this plant. Further potentially immunomodulatory cucurbitacins or cucurbitacin derivatives were assumed to be in the tuber. Given the typically high content of cucurbitacins with similar physicochemical features but often distinct bioactivities, an efficient and reliable separation process is a prerequisite for their detailed characterization and assessment in terms of bioactivity. We therefore developed a detection method to screen and differentiate cucurbitacins via high-performance liquid chromatography/quadrupole-time-of-flight tandem mass spectrometry (HPLC-QTOF-MS/MS). In order to confirm the identification, the fragmentation patterns of two cucurbitacins and one 23,24-dihydrocucurbitacin were also investigated. Six characteristic fragments were identified and three of them were employed for the identification of cucurbitacins and 23,24-dihydrocucurbitacins in the extract. As a result, in addition to eight previously reported cucurbitacins from this plant four distinct 23,24-dihydrocucurbitacins (B, D, E, and I) were putatively identified and newly found in the ethyl acetate extract of the tuber of C. naudinianus. The established methodology enables rapid and efficient LC-MS-based analysis and identification of cucurbitacins and 23,24-dihydrocucurbitacins in plant extracts.

Published
2023
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3. Enzymatic spiroketal formation via oxidative rearrangement of pentangular polyketides

Author

Britta Frensch, Thorsten Lechtenberg, Michel Kather, Zeynep Yunt, Martin Betschart, Bernd Kammerer, Steffen Lüdeke, Michael Müller, Jörn Piel, and Robin Teufel

Subjects
Science
Abstract

Rubromycin family of natural products belongs to aromatic polyketides with diverse bioactivities, but details of their biosynthesis are limited. Here, the authors report the complete in vitro reconstitution of enzymatic formation of the spiroketal moiety of rubromycin polyketides, driven by flavin-dependent enzymes, and characterize reaction intermediates.

Published
2021
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5. An acetyltransferase controls the metabolic flux in rubromycin polyketide biosynthesis by direct modulation of redox tailoring enzymes

Author

Marina Toplak, Adelheid Nagel, Britta Frensch, Thorsten Lechtenberg, and Robin Teufel

Subjects
General Chemistry
Abstract

The often complex control of bacterial natural product biosynthesis typically involves global and pathway-specific transcriptional regulators of gene expression, which often limits the yield of bioactive compounds under laboratory conditions. However, little is known about regulation mechanisms on the enzymatic level. Here, we report a novel regulatory principle for natural products involving a dedicated acetyltransferase, which modifies a redox-tailoring enzyme and thereby enables pathway furcation and alternating pharmacophore assembly in rubromycin polyketide biosynthesis. The rubromycins such as griseorhodin (

Published
2022

6. Ungewöhnliche Flavoenzyme steuern die Bildung von Troponen in Bakterien

Author

Marina Toplak, Lars Höing, and Robin Teufel

Subjects
Molecular Biology, Biotechnology
Abstract

Bacterial tropone natural products play important roles in symbiotic interactions, e. g., as protective antibiotics or toxins. Remarkably, their biosynthesis relies on an interweaving of primary and secondary metabolism. Accordingly, the sequestration of a shunt product from aromatic catabolism by a non-canonical flavoenzyme leads to an advanced biosynthetic intermediate. The enzyme hereby operates as a novel dioxygenase that activates O2 for CoA thioester bond cleavage and ring epoxidation.

Published
2022

7. Catalytic Control of Spiroketal Formation in Rubromycin Polyketide Biosynthesis

Author

Jörn Piel, Robin Teufel, Raspudin Saleem-Batcha, and Marina Toplak

Subjects
Stereochemistry, polyketide synthase, Flavoprotein, Catalysis, antibiotics, Mixed Function Oxygenases, chemistry.chemical_compound, Polyketide, lenticulone, Protein Domains, Biosynthesis, Catalytic Domain, Polyketide synthase, Moiety, Quinone Reductases, redox tailoring, ATP synthase, biology, Quinones, General Chemistry, General Medicine, Monooxygenase, Kinetics, chemistry, Mutation, Biocatalysis, Flavin-Adenine Dinucleotide, Mutagenesis, Site-Directed, biology.protein, collinone, Pharmacophore, Oxidation-Reduction, NADP, Ethers, Protein Binding
Abstract

The medically important bacterial aromatic polyketide natural products typically feature a planar, polycyclic core structure. An exception is found for the rubromycins, whose backbones are disrupted by a bisbenzannulated [5,6]-spiroketal pharmacophore that was recently shown to be assembled by flavin-dependent enzymes. In particular, a flavoprotein monooxygenase proved critical for the drastic oxidative rearrangement of a pentangular precursor and the installment of an intermediate [6,6]-spiroketal moiety. Here we provide structural and mechanistic insights into the control of catalysis by this spiroketal synthase, which fulfills several important functions as reductase, monooxygenase, and presumably oxidase. The enzyme hereby tightly controls the redox state of the substrate to counteract shunt product formation, while also steering the cleavage of three carbon-carbon bonds. Our work illustrates an exceptional strategy for the biosynthesis of stable chroman spiroketals., Angewandte Chemie. International Edition, 60 (52), ISSN:1433-7851, ISSN:1521-3773, ISSN:0570-0833

Published
2021

8. Bacterial Tropone Natural Products and Derivatives: Overview of their Biosynthesis, Bioactivities, Ecological Role and Biotechnological Potential

Author

Ying Duan, Melanie Petzold, Robin Teufel, and Raspudin Saleem-Batcha

Subjects
Antifungal Agents, natural products, roseobacticides, Reviews, Antineoplastic Agents, Review, Tropodithietic acid, Phenylacetic acid, 010402 general chemistry, 01 natural sciences, Biochemistry, Tropolone, tropodithietic acid, chemistry.chemical_compound, Biosynthesis, Neoplasms, Animals, Humans, Molecular Biology, chemistry.chemical_classification, Biological Products, Bacteria, 010405 organic chemistry, Ecology, Organic Chemistry, Fungi, Marine invertebrates, symbiosis, Anti-Bacterial Agents, 0104 chemical sciences, Quorum sensing, Enzyme, chemistry, Molecular Medicine, %22">Fish , tropolones, Tropone, Biotechnology
Abstract

Tropone natural products are non‐benzene aromatic compounds of significant ecological and pharmaceutical interest. Herein, we highlight current knowledge on bacterial tropones and their derivatives such as tropolones, tropodithietic acid, and roseobacticides. Their unusual biosynthesis depends on a universal CoA‐bound precursor featuring a seven‐membered carbon ring as backbone, which is generated by a side reaction of the phenylacetic acid catabolic pathway. Enzymes encoded by separate gene clusters then further modify this key intermediate by oxidation, CoA‐release, or incorporation of sulfur among other reactions. Tropones play important roles in the terrestrial and marine environment where they act as antibiotics, algaecides, or quorum sensing signals, while their bacterial producers are often involved in symbiotic interactions with plants and marine invertebrates (e. g., algae, corals, sponges, or mollusks). Because of their potent bioactivities and of slowly developing bacterial resistance, tropones and their derivatives hold great promise for biomedical or biotechnological applications, for instance as antibiotics in (shell)fish aquaculture., Accidents will happen: The biosynthesis of bacterial tropone natural products depends on an unusual intertwining of primary and secondary metabolism. Remarkably, a shunt product arising from a “metabolic accident” of an aromatic catabolic pathway serves as universal precursor for tropone natural products.

Published
2020

9. Oxidative Carbon Backbone Rearrangement in Rishirilide Biosynthesis

Author

Robin Teufel, David L. Zechel, Olga Tsypik, Britta Frensch, Thomas Paululat, Andreas Bechthold, and Roman Makitrynskyy

Subjects
Anthracenes, Stereochemistry, Epoxide, Anthraquinones, General Chemistry, Flavin group, 010402 general chemistry, 01 natural sciences, Biochemistry, Redox, Carbon, Streptomyces, Catalysis, Biosynthetic Pathways, 0104 chemical sciences, chemistry.chemical_compound, Polyketide, Colloid and Surface Chemistry, Bacterial Proteins, chemistry, Biosynthesis, Intramolecular force, Moiety, Aldol condensation, Oxidation-Reduction
Abstract

The structural diversity of type II polyketides is largely generated by tailoring enzymes. In rishirilide biosynthesis by Streptomyces bottropensis, 13C-labeling studies previously implied extraordinary carbon backbone and side-chain rearrangements. In this work, we employ gene deletion experiments and in vitro enzyme studies to identify key biosynthetic intermediates and expose intricate redox tailoring steps for the formation of rishirilides A, B, and D and lupinacidin A. First, the flavin-dependent RslO5 reductively ring-opens the epoxide moiety of an advanced polycyclic intermediate to form an alcohol. Flavin monooxygenase RslO9 then oxidatively rearranges the carbon backbone, presumably via lactone-forming Baeyer-Villiger oxidation and subsequent intramolecular aldol condensation. While RslO9 can further convert the rearranged intermediate to rishirilide D and lupinacidin A, an additional ketoreductase RslO8 is required for formation of the main products rishirilide A and rishirilide B. This work provides insight into the structural diversification of aromatic polyketide natural products via unusual redox tailoring reactions that appear to defy biosynthetic logic.

Published
2020

10. Aminoperoxide adducts expand the catalytic repertoire of flavin monooxygenases

Author

Jacob N. Sanders, Robin Teufel, Raspudin Saleem-Batcha, Arne Matthews, Frederick Stull, and K. N. Houk

Subjects
Dinitrocresols, Nitrogen, Stereochemistry, Flavoprotein, Flavin group, Crystallography, X-Ray, Peroxide, Chemical synthesis, Catalysis, 03 medical and health sciences, chemistry.chemical_compound, Structural motif, Molecular Biology, Phylogeny, 030304 developmental biology, 0303 health sciences, biology, Escherichia coli Proteins, 030302 biochemistry & molecular biology, Cell Biology, Monooxygenase, Peroxides, Oxygen, chemistry, Biocatalysis, Oxygenases, biology.protein
Abstract

One of the hallmark reactions catalyzed by flavin-dependent enzymes is the incorporation of an oxygen atom derived from dioxygen into organic substrates. For many decades, these flavin monooxygenases were assumed to use exclusively the flavin-C4a-(hydro)peroxide as their oxygen-transferring intermediate. We demonstrate that flavoenzymes may instead employ a flavin-N5-peroxide as a soft α-nucleophile for catalysis, which enables chemistry not accessible to canonical monooxygenases. This includes, for example, the redox-neutral cleavage of carbon-hetero bonds or the dehalogenation of inert environmental pollutants via atypical oxygenations. We furthermore identify a shared structural motif for dioxygen activation and N5-functionalization, suggesting a conserved pathway that may be operative in numerous characterized and uncharacterized flavoenzymes from diverse organisms. Our findings show that overlooked flavin-N5-oxygen adducts are more widespread and may facilitate versatile chemistry, thus upending the notion that flavin monooxygenases exclusively function as nature's equivalents to organic peroxides in synthetic chemistry.

Published
2020

11. Bacterial Dehydrogenases Facilitate Oxidative Inactivation and Bioremediation of Chloramphenicol

Author

Lei Zhang, Marina Toplak, Raspudin Saleem‐Batcha, Lars Höing, Roman Jakob, Nico Jehmlich, Martin von Bergen, Timm Maier, and Robin Teufel

Subjects
Organic Chemistry, Molecular Medicine, Molecular Biology, Biochemistry
Abstract

Antimicrobial resistance represents a major threat to human health and knowledge of the underlying mechanisms is therefore vital. Here, we report the discovery and characterization of oxidoreductases that inactivate the broad-spectrum antibiotic chloramphenicol via dual oxidation of the C3-hydroxyl group. Accordingly, chloramphenicol oxidation either depends on standalone glucose-methanol-choline (GMC)-type flavoenzymes, or on additional aldehyde dehydrogenases that boost overall turnover. These enzymes also enable the inactivation of the chloramphenicol analogues thiamphenicol and azidamfenicol, but not of the C3-fluorinated florfenicol. Notably, distinct isofunctional enzymes can be found in Gram-positive (e. g., Streptomyces sp.) and Gram-negative (e. g., Sphingobium sp.) bacteria, which presumably evolved their selectivity for chloramphenicol independently based on phylogenetic analyses. Mechanistic and structural studies provide further insights into the catalytic mechanisms of these biotechnologically interesting enzymes, which, in sum, are both a curse and a blessing by contributing to the spread of antibiotic resistance as well as to the bioremediation of chloramphenicol.

Published
2022
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12. Three Rings to Rule Them All: How Versatile Flavoenzymes Orchestrate the Structural Diversification of Natural Products

Author

Marina Toplak and Robin Teufel

Subjects
Biological Products, Bacteria, Bacterial Proteins, Flavoproteins, Flavins, Polyketides, Perspective, Biochemistry, Oxidation-Reduction, Biosynthetic Pathways, Substrate Specificity
Abstract

The structural diversification of natural products is instrumental to their versatile bioactivities. In this context, redox tailoring enzymes are commonly involved in the modification and functionalization of advanced pathway intermediates en route to the mature natural products. In recent years, flavoprotein monooxygenases have been shown to mediate numerous redox tailoring reactions that include not only (aromatic) hydroxylation, Baeyer–Villiger oxidation, or epoxidation reactions but also oxygenations that are coupled to extensive remodeling of the carbon backbone, which are often central to the installment of the respective pharmacophores. In this Perspective, we will highlight recent developments and discoveries in the field of flavoenzyme catalysis in bacterial natural product biosynthesis and illustrate how the flavin cofactor can be fine-tuned to enable chemo-, regio-, and stereospecific oxygenations via distinct flavin-C4a-peroxide and flavin-N5-(per)oxide species. Open questions remain, e.g., regarding the breadth of chemical reactions enabled particularly by the newly discovered flavin-N5-oxygen adducts and the role of the protein environment in steering such cascade-like reactions. Outstanding cases involving different flavin oxygenating species will be exemplified by the tailoring of bacterial aromatic polyketides, including enterocin, rubromycins, rishirilides, mithramycin, anthracyclins, chartreusin, jadomycin, and xantholipin. In addition, the biosynthesis of tropone natural products, including tropolone and tropodithietic acid, will be presented, which features a recently described prototypical flavoprotein dioxygenase that may combine flavin-N5-peroxide and flavin-N5-oxide chemistry. Finally, structural and mechanistic features of selected enzymes will be discussed as well as hurdles for their application in the formation of natural product derivatives via bioengineering.

Published
2021

13. Bacterial flavoprotein monooxygenase YxeK salvages toxic S-(2-succino)-adducts via oxygenolytic C-S bond cleavage

Author

Holly R. Ellis, Bernd Kammerer, Simon Lagies, Arne Matthews, Julia Schönfelder, Frederick Stull, Erik Schleicher, and Robin Teufel

Subjects
Stereochemistry, Sulfur metabolism, Flavoprotein, Bacillus subtilis, Biochemistry, Mixed Function Oxygenases, Substrate Specificity, Fumarates, Oxidoreductase, Flavins, Operon, Cysteine, Sulfhydryl Compounds, Molecular Biology, Bond cleavage, chemistry.chemical_classification, biology, Flavoproteins, Chemistry, Mutagenesis, Acetylation, Cell Biology, Monooxygenase, biology.organism_classification, Kinetics, Models, Chemical, biology.protein, Mutagenesis, Site-Directed
Abstract

Thiol-containing nucleophiles such as cysteine react spontaneously with the citric acid cycle intermediate fumarate to form S-(2-succino)-adducts. In Bacillus subtilis, a salvaging pathway encoded by the yxe operon has recently been identified for the detoxification and exploitation of these compounds as sulfur sources. This route involves acetylation of S-(2-succino)cysteine to N-acetyl-2-succinocysteine, which is presumably converted to oxaloacetate and N-acetylcysteine, before a final deacetylation step affords cysteine. The critical oxidative cleavage of the C-S bond of N-acetyl-S-(2-succino)cysteine was proposed to depend on the predicted flavoprotein monooxygenase YxeK. Here, we characterize YxeK and verify its role in S-(2-succino)-adduct detoxification and sulfur metabolism. Detailed biochemical and mechanistic investigation of YxeK including 18 O-isotope-labeling experiments, homology modeling, substrate specificity tests, site-directed mutagenesis, and (pre-)steady-state kinetics provides insight into the enzyme's mechanism of action, which may involve a noncanonical flavin-N5-peroxide species for C-S bond oxygenolysis.

Published
2021

14. Flavin-catalyzed redox tailoring reactions in natural product biosynthesis

Author

Robin Teufel

Subjects
0301 basic medicine, Stereochemistry, Biophysics, Flavin group, 010402 general chemistry, 01 natural sciences, Biochemistry, Redox, Catalysis, Cofactor, 03 medical and health sciences, chemistry.chemical_compound, Biosynthesis, Flavins, Molecular Biology, chemistry.chemical_classification, Natural product, biology, Total synthesis, 0104 chemical sciences, 030104 developmental biology, Enzyme, chemistry, biology.protein, Pharmacophore, Reactive Oxygen Species, Oxidation-Reduction
Abstract

Natural products are distinct and often highly complex organic molecules that constitute not only an important drug source, but have also pushed the field of organic chemistry by providing intricate targets for total synthesis. How the astonishing structural diversity of natural products is enzymatically generated in biosynthetic pathways remains a challenging research area, which requires detailed and sophisticated approaches to elucidate the underlying catalytic mechanisms. Commonly, the diversification of precursor molecules into distinct natural products relies on the action of pathway-specific tailoring enzymes that catalyze, e.g., acylations, glycosylations, or redox reactions. This review highlights a selection of tailoring enzymes that employ riboflavin (vitamin B2)-derived cofactors (FAD and FMN) to facilitate unusual redox catalysis and steer the formation of complex natural product pharmacophores. Remarkably, several such recently reported flavin-dependent tailoring enzymes expand the classical paradigms of flavin biochemistry leading, e.g., to the discovery of the flavin-N5-oxide - a novel flavin redox state and oxygenating species.

Published
2017

15. Structural and Mechanistic Basis of an Oxepin-CoA Forming Isomerase in Bacterial Primary and Secondary Metabolism

Author

Melanie Spieker, Raspudin Saleem-Batcha, and Robin Teufel

Subjects
0303 health sciences, Bacteria, 030306 microbiology, Protein Conformation, Secondary Metabolism, General Medicine, Ligands, Biochemistry, Catalysis, 03 medical and health sciences, Oxepins, Molecular Medicine, Coenzyme A, Isomerases, 030304 developmental biology, Phenylacetates
Abstract

Numerous aromatic compounds are aerobically degraded in bacteria via the central intermediate phenylacetic acid (paa). In one of the key steps of this widespread catabolic pathway, 1,2-epoxyphenylacetyl-CoA is converted by PaaG into the heterocyclic oxepin-CoA. PaaG thereby elegantly generates an α,β-unsaturated CoA ester that is predisposed to undergo β-oxidation subsequent to hydrolytic ring-cleavage. Moreover, oxepin-CoA serves as a precursor for secondary metabolites (e.g., tropodithietic acid) that act as antibiotics and quorum-sensing signals. Here we verify that PaaG adopts a second role in aromatic catabolism by converting

Published
2019

17. The devil is in the details: The chemical basis and mechanistic versatility of flavoprotein monooxygenases

Author

Robin Teufel, Arne Matthews, and Marina Toplak

Subjects
0301 basic medicine, Flavin Mononucleotide, Heteroatom, Biophysics, Flavoprotein, Flavin group, Biochemistry, Redox, Mixed Function Oxygenases, Hydroxylation, 03 medical and health sciences, chemistry.chemical_compound, Bacterial Proteins, Cytochrome P-450 Enzyme System, Molecular Biology, Bond cleavage, Primary (chemistry), Bacteria, Flavoproteins, 030102 biochemistry & molecular biology, biology, Combinatorial chemistry, Oxygen, 030104 developmental biology, Models, Chemical, chemistry, Covalent bond, Biocatalysis, Flavin-Adenine Dinucleotide, biology.protein
Abstract

The ubiquitous flavoenzymes commonly catalyze redox chemistry such as the monooxygenation of organic substrates and are both widely utilized in nature (e.g., in primary and secondary metabolism) and of significant industrial interest. In this work, we highlight the structural and mechanistic characteristics of the distinct types of flavoprotein monooxygenases (FPMOs). We thereby illustrate the chemical basis of FPMO catalysis, which enables reactions such as (aromatic) hydroxylation, epoxidation, (de)halogenation, heteroatom oxygenation, Baeyer-Villiger oxidation, α-hydroxylation of ketones, or non-oxidative carbon-hetero bond cleavage. This seemingly unmatched versatility in oxygenation chemistry results from extensive fine-tuning and regiospecific functionalization of the flavin cofactor that is tightly controlled by the surrounding protein matrix. Accordingly, FPMOs steer the formation of covalent flavin-oxygen adducts for oxygen transfer in the form of the classical flavin-C4a-(hydro)peroxide or the recently discovered N5-functionalized flavins (i.e. the flavin-N5-oxide and the flavin-N5-peroxide), while in rare cases covalent oxygen adduct formation may be foregone entirely. Finally, we speculate about hitherto undiscovered flavin-mediated oxygenation reactions and compare FPMOs to cytochrome P450 monooxygenases, before addressing open questions and challenges for the future investigation of FPMOs.

Published
2021

18. Unusual flavoenzyme catalysis in marine bacteria

Author

Robin Teufel, Bradley S. Moore, and Vinayak Agarwal

Subjects
0301 basic medicine, Primary metabolism, Marine Biology, Flavin group, 010402 general chemistry, 01 natural sciences, Biochemistry, Article, Catalysis, Cofactor, Analytical Chemistry, 03 medical and health sciences, Marine bacteriophage, Flavins, heterocyclic compounds, Secondary metabolism, chemistry.chemical_classification, Bacteria, biology, Chemistry, Enzymes, 0104 chemical sciences, Metabolic pathway, 030104 developmental biology, Enzyme, biology.protein, Oxidation-Reduction
Abstract

Ever since the discovery of the flavin cofactor more than 80 years ago, flavin-dependent enzymes have emerged as ubiquitous and versatile redox catalysts in primary metabolism. Yet, the recent advances in the discovery and characterization of secondary metabolic pathways exposed new roles for flavin-mediated catalysis in the generation of structurally complex natural products. Here, we review a selection of key biosynthetic flavoenzymes from marine bacterial secondary metabolism and illustrate how their functional and mechanistic investigation expanded our view of the cofactor's chemical repertoire and led to the discovery of a previously unknown flavin redox state.

Published
2016

20. Preparation and Characterization of the Favorskiiase Flavoprotein EncM and Its Distinctive Flavin-N5-Oxide Cofactor

Author

Robin, Teufel

Subjects
Bridged-Ring Compounds, Flavoproteins, Flavins, Coenzymes, Crystallization, Protein Engineering, Chromatography, High Pressure Liquid, Recombinant Proteins, Streptomyces, Mixed Function Oxygenases
Abstract

Flavoenzymes often function as oxygenases and have been extensively studied for many decades. Commonly, oxygenation reactions are mediated by a transient C4a-peroxyflavin formed from reaction of reduced flavin with O

Published
2018

21. Enzymatic control of dioxygen binding and functionalization of the flavin cofactor

Author

Bradley S. Moore, Jacob N. Sanders, Bruce A. Palfey, Raspudin Saleem-Batcha, Robin Teufel, Frederick Stull, and K. N. Houk

Subjects
0301 basic medicine, Dinitrocresols, Coenzymes, Flavoprotein, Flavin group, 010402 general chemistry, Crystallography, X-Ray, 01 natural sciences, Redox, Corrections, Cofactor, Catalysis, Mixed Function Oxygenases, 03 medical and health sciences, Bacterial Proteins, monooxygenase, chemistry.chemical_classification, Multidisciplinary, Crystallography, bioengineering, flavin-N5-oxide, biology, FAD, Rational design, Active site, Combinatorial chemistry, 0104 chemical sciences, EncM, Molecular Docking Simulation, Oxygen, 030104 developmental biology, Enzyme, chemistry, biology.protein, X-Ray, Quantum Theory, Oxidation-Reduction
Abstract

The reactions of enzymes and cofactors with gaseous molecules such as dioxygen (O 2 ) are challenging to study and remain among the most contentious subjects in biochemistry. To date, it is largely enigmatic how enzymes control and fine-tune their reactions with O 2 , as exemplified by the ubiquitous flavin-dependent enzymes that commonly facilitate redox chemistry such as the oxygenation of organic substrates. Here we employ O 2 -pressurized X-ray crystallography and quantum mechanical calculations to reveal how the precise positioning of O 2 within a flavoenzyme’s active site enables the regiospecific formation of a covalent flavin–oxygen adduct and oxygenating species (i.e., the flavin-N5-oxide) by mimicking a critical transition state. This study unambiguously demonstrates how enzymes may control the O 2 functionalization of an organic cofactor as prerequisite for oxidative catalysis. Our work thus illustrates how O 2 reactivity can be harnessed in an enzymatic environment and provides crucial knowledge for future rational design of O 2 -reactive enzymes.

Published
2018

22. Insights into the enzymatic formation, chemical features, and biological role of the flavin-N5-oxide

Author

Raspudin Saleem-Batcha and Robin Teufel

Subjects
0301 basic medicine, Models, Molecular, Oxygenase, Vanillyl-alcohol oxidase, Coenzymes, Flavoprotein, Flavin group, 010402 general chemistry, 01 natural sciences, Biochemistry, Redox, Cofactor, Catalysis, Analytical Chemistry, 03 medical and health sciences, Flavins, Escherichia coli, Rhodococcus, heterocyclic compounds, biology, Flavoproteins, Chemistry, Substrate (chemistry), Monooxygenase, Combinatorial chemistry, 0104 chemical sciences, 030104 developmental biology, biology.protein, Oxygenases, Oxidation-Reduction
Abstract

Flavoenzymes are versatile catalysts that mostly facilitate redox reactions such as the oxygenation of organic substrates. Commonly, flavin monooxygenases employ a flavin-C4a-(hydro)peroxide as oxygenating species. Recently, however, a modified N5-functionalized flavin cofactor featuring a distinct nitrone moiety — the flavin-N5-oxide — was reported for the first time as oxygenating species in the bacterial enzyme EncM that catalyzes the dual oxidation of a reactive poly-β-ketone substrate. Meanwhile, additional flavoenzymes have been reported that form the flavin-N5-oxide. Here, we highlight aspects of the discovery and characterization of this novel flavin redox state with a focus on recent findings that shed more light onto its chemical features and enzymatic formation. We furthermore provide a rationale for the oxygenase functionality of EncM by contrast with structurally related flavin oxidases and dehydrogenases from the vanillyl alcohol oxidase/p-cresol methylhydroxylase flavoprotein (VAO/PCMH) superfamily. In addition, the possible biological roles of the flavin-N5-oxide are discussed.

Published
2018

23. Preparation and Characterization of the Favorskiiase Flavoprotein EncM and Its Distinctive Flavin-N5-Oxide Cofactor

Author

Robin Teufel

Subjects
0301 basic medicine, Natural product, biology, Chemistry, Flavoprotein, Flavin group, Oxidative phosphorylation, Redox, Cofactor, 03 medical and health sciences, chemistry.chemical_compound, Polyketide, 030104 developmental biology, Biochemistry, Biosynthesis, biology.protein
Abstract

Flavoenzymes often function as oxygenases and have been extensively studied for many decades. Commonly, oxygenation reactions are mediated by a transient C4a-peroxyflavin formed from reaction of reduced flavin with O2. EncM, however, employs a previously unrecognized flavin-oxygenating species, the flavin-N5-oxide, which is key to a complex oxidative Favorskii-type rearrangement and cyclization cascade in the biosynthesis of the bacterial polyketide antibiotic enterocin produced by the marine bacterium Streptomyces maritimus. Here, the methodology and key experiments are described that led to the discovery of this novel flavin redox species and granted insight into one of the most astounding single-enzyme-catalyzed reaction cascades in natural product biosynthesis.

Published
2018

24. Unusual 'Head-to-Torso' Coupling of Terpene Precursors as a New Strategy for the Structural Diversification of Natural Products

Author

Robin Teufel

Subjects
chemistry.chemical_classification, Terpenoid biosynthesis, 010405 organic chemistry, Chemistry, Stereochemistry, Structural diversity, 010402 general chemistry, 01 natural sciences, Terpenoid, 0104 chemical sciences, Terpene, Polyketide, Enzyme, Prenylation, Terpene synthase
Abstract

Terpenoids are ubiquitous in nature and exhibit an immense structural diversity. Commonly, terpenoid biosynthesis involves prenyl diphosphate synthases (terpene synthases) that produce linear prenyl diphosphates with various chain lengths via conventional “head-to-tail” coupling of C5 units. Structural diversification, in contrast, is often mediated by terpene cyclases and additional tailoring enzymes. Recently, however, a few unusual prenyl diphosphate synthases were reported that catalyze noncanonical “head-to-torso” coupling reactions and thus formation of various branched prenyl diphosphates such as isosesquilavandulyl diphosphate. Here, I describe these enzymes in detail and illustrate how these branching reactions are key to formation of various structurally distinct natural products such as the complex polycyclic merochlorin antibiotics from a marine bacterium.

Published
2018

25. A Multitasking Vanadium-Dependent Chloroperoxidase as an Inspiration for the Chemical Synthesis of the Merochlorins

Author

Bradley S. Moore, Robin Teufel, Leonard Kaysser, and Stefan Diethelm

Subjects
Sesterterpenes, 010405 organic chemistry, Chemistry, Vanadium, chemistry.chemical_element, Stereoisomerism, General Chemistry, Chloride peroxidase, General Medicine, 010402 general chemistry, 01 natural sciences, Chemical synthesis, Article, Catalysis, 0104 chemical sciences, Terpene, Cyclization, Biocatalysis, Biomimetic synthesis, Organic chemistry, Reactivity (chemistry), Chloride Peroxidase, Oxidation-Reduction
Abstract

The vanadium-dependent chloroperoxidase Mcl24 was discovered to mediate a complex series of unprecedented transformations in the biosynthesis of the merochlorin meroterpenoid antibiotics. In particular, a site-selective naphthol chlorination is followed by a sequence of oxidative dearomatization/terpene cyclization reactions to build up the stereochemically complex carbon framework of the merochlorins in one step. Inspired by the enzyme reactivity, we developed a chemical chlorination protocol paralleling the biocatalytic process. These chemical studies led to the identification of previously overlooked merochlorin natural products.

Published
2014

27. One-Pot Enzymatic Synthesis of Merochlorin A and B

Author

Matthew T. Villaume, Mary K. Carbullido, Leonard Kaysser, Bradley S. Moore, Robin Teufel, Stefan Diethelm, and Phil S. Baran

Subjects
Sesterterpenes, Stereochemistry, Prenyltransferase, 010402 general chemistry, 01 natural sciences, Chemical synthesis, Streptomyces, Article, Catalysis, Polyketide, chemistry.chemical_compound, Hemiterpenes, Organophosphorus Compounds, Bacterial Proteins, Biosynthesis, Haloperoxidase, Moiety, biology, ATP synthase, Terpenes, 010405 organic chemistry, General Chemistry, biology.organism_classification, 0104 chemical sciences, chemistry, Cyclization, biology.protein
Abstract

The polycycles merochlorin A and B are complex halogenated meroterpenoid natural products with significant antibacterial activities and are produced by the marine bacterium Streptomyces sp. strain CNH-189. Heterologously produced enzymes and chemical synthesis are employed herein to fully reconstitute the merochlorin biosynthesis in vitro. The interplay of a dedicated type III polyketide synthase, a prenyl diphosphate synthase, and an aromatic prenyltransferase allow formation of a highly unusual aromatic polyketide-terpene hybrid intermediate which features an unprecedented branched sesquiterpene moiety from isosesquilavandulyl diphosphate. As supported by in vivo experiments, this precursor is furthermore chlorinated and cyclized to merochlorin A and isomeric merochlorin B by a single vanadium-dependent haloperoxidase, thus completing the remarkably efficient pathway.

Published
2014
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28. Enzymatic control of O2 reactivity and functionalization of the flavin cofactor

Author

Robin Teufel and Raspudin Saleem Batcha

Subjects
chemistry.chemical_classification, biology, Flavin group, Condensed Matter Physics, Biochemistry, Combinatorial chemistry, Cofactor, Inorganic Chemistry, Enzyme, chemistry, Structural Biology, biology.protein, Surface modification, General Materials Science, Reactivity (chemistry), Physical and Theoretical Chemistry
Published
2019

29. Flavin-mediated dual oxidation controls an enzymatic Favorskii-type rearrangement

Author

Akimasa Miyanaga, Gordon V. Louie, Phil S. Baran, Joseph P. Noel, Bradley S. Moore, Bruce A. Palfey, Frederick Stull, Robin Teufel, and Quentin Michaudel

Subjects
Bridged-Ring Compounds, Models, Molecular, Protein Conformation, Stereochemistry, Flavin mononucleotide, Flavoprotein, Flavin group, Crystallography, X-Ray, 010402 general chemistry, 01 natural sciences, Redox, Article, Cofactor, Mixed Function Oxygenases, Substrate Specificity, chemistry.chemical_compound, Bacterial Proteins, Flavins, Flavin adenine dinucleotide, Multidisciplinary, Flavoproteins, biology, 010405 organic chemistry, Substrate (chemistry), Streptomyces, Anti-Bacterial Agents, 0104 chemical sciences, Models, Chemical, chemistry, Cyclization, Isotope Labeling, Polyketides, Biocatalysis, biology.protein, Oxidation-Reduction
Abstract

Structural and functional studies reveal how the bacterial flavoenzyme EncM catalyses the oxygenation–dehydrogenation dual oxidation of a highly reactive substrate, and show that EncM maintains a stable flavin oxygenating species that promotes substrate oxidation and triggers a rarely seen Favorskii-type rearrangement. Flavoproteins, which contain either a flavin adenine dinucleotide or a flavin mononucleotide cofactor, are redox-active proteins involved in a broad range of biological processes including bioluminescence, photosynthesis and DNA repair. Here the authors undertook structural and functional studies to examine how the bacterial flavoenzyme EncM catalyses the oxygenation–dehydrogenation oxidation of a highly reactive substrate. They observed previously unknown flavin redox biochemistry: EncM maintains a stable flavin-oxygenating species that promotes substrate oxidation and triggers a rarely seen, Favorskii-type rearrangement that is central to the biosynthesis of the marine antibiotic enterocin. Flavoproteins catalyse a diversity of fundamental redox reactions and are one of the most studied enzyme families1,2. As monooxygenases, they are universally thought to control oxygenation by means of a peroxyflavin species that transfers a single atom of molecular oxygen to an organic substrate1,3,4. Here we report that the bacterial flavoenzyme EncM5,6 catalyses the peroxyflavin-independent oxygenation–dehydrogenation dual oxidation of a highly reactive poly(β-carbonyl). The crystal structure of EncM with bound substrate mimics and isotope labelling studies reveal previously unknown flavin redox biochemistry. We show that EncM maintains an unexpected stable flavin-oxygenating species, proposed to be a flavin-N5-oxide, to promote substrate oxidation and trigger a rare Favorskii-type rearrangement that is central to the biosynthesis of the antibiotic enterocin. This work provides new insight into the fine-tuning of the flavin cofactor in offsetting the innate reactivity of a polyketide substrate to direct its efficient electrocyclization.

Published
2013

30. Studies on the Mechanism of Ring Hydrolysis in Phenylacetate Degradation

Author

Wolfgang Eisenreich, Georg Fuchs, Carla Gantert, Robin Teufel, Michaela Voss, and Wolfgang Haehnel

Subjects
chemistry.chemical_classification, biology, Stereochemistry, Coenzyme A, Aldehyde dehydrogenase, Cell Biology, Enoyl-CoA hydratase, Ring (chemistry), Biochemistry, Aldehyde, Tropolone, chemistry.chemical_compound, Phenylacetate, chemistry, biology.protein, NAD+ kinase, Molecular Biology
Abstract

The widespread, long sought-after bacterial aerobic phenylalanine/phenylacetate catabolic pathway has recently been elucidated. It proceeds via coenzyme A (CoA) thioesters and involves the epoxidation of the aromatic ring of phenylacetyl-CoA, subsequent isomerization to an uncommon seven-membered C-O-heterocycle (oxepin-CoA), and non-oxygenolytic ring cleavage. Here we characterize the hydrolytic oxepin-CoA ring cleavage catalyzed by the bifunctional fusion protein PaaZ. The enzyme consists of a C-terminal (R)-specific enoyl-CoA hydratase domain (formerly MaoC) that cleaves the ring and produces a highly reactive aldehyde and an N-terminal NADP+-dependent aldehyde dehydrogenase domain that oxidizes the aldehyde to 3-oxo-5,6-dehydrosuberyl-CoA. In many phenylacetate-utilizing bacteria, the genes for the pathway exist in a cluster that contains an NAD+-dependent aldehyde dehydrogenase in place of PaaZ, whereas the aldehyde-producing hydratase is encoded outside of the cluster. If not oxidized immediately, the reactive aldehyde condenses intramolecularly to a stable cyclic derivative that is largely prevented by PaaZ fusion in vivo. Interestingly, the derivative likely serves as the starting material for the synthesis of antibiotics (e.g. tropodithietic acid) and other tropone/tropolone related compounds as well as for ω-cycloheptyl fatty acids. Apparently, bacteria made a virtue out of the necessity of disposing the dead-end product with ring hydrolysis as a metabolic branching point.

Published
2011

31. Bacterial phenylalanine and phenylacetate catabolic pathway revealed

Author

Robin Teufel, Wael Ismail, Wolfgang Eisenreich, Georg Fuchs, Victoria Mascaraque, Wolfgang Haehnel, M. Voss, and Julián Perera

Subjects
Oxygenase, Multidisciplinary, Bacteria, biology, Pseudomonas putida, Catabolism, Phenylalanine, Biological Sciences, biology.organism_classification, medicine.disease_cause, Biodegradation, Environmental, Phenylacetate, Biochemistry, Multigene Family, Gene cluster, Escherichia coli, medicine, Genome, Bacterial, Metabolic Networks and Pathways, Styrene, Phenylacetates
Abstract

Aromatic compounds constitute the second most abundant class of organic substrates and environmental pollutants, a substantial part of which (e.g., phenylalanine or styrene) is metabolized by bacteria via phenylacetate. Surprisingly, the bacterial catabolism of phenylalanine and phenylacetate remained an unsolved problem. Although a phenylacetate metabolic gene cluster had been identified, the underlying biochemistry remained largely unknown. Here we elucidate the catabolic pathway functioning in 16% of all bacteria whose genome has been sequenced, including Escherichia coli and Pseudomonas putida . This strategy is exceptional in several aspects. Intermediates are processed as CoA thioesters, and the aromatic ring of phenylacetyl-CoA becomes activated to a ring 1,2-epoxide by a distinct multicomponent oxygenase. The reactive nonaromatic epoxide is isomerized to a seven-member O-heterocyclic enol ether, an oxepin. This isomerization is followed by hydrolytic ring cleavage and β-oxidation steps, leading to acetyl-CoA and succinyl-CoA. This widespread paradigm differs significantly from the established chemistry of aerobic aromatic catabolism, thus widening our view of how organisms exploit such inert substrates. It provides insight into the natural remediation of man-made environmental contaminants such as styrene. Furthermore, this pathway occurs in various pathogens, where its reactive early intermediates may contribute to virulence.

Published
2010

32. 3-Hydroxypropionyl-Coenzyme A Dehydratase and Acryloyl-Coenzyme A Reductase, Enzymes of the Autotrophic 3-Hydroxypropionate/4-Hydroxybutyrate Cycle in the Sulfolobales

Author

Johannes W. Kung, Robin Teufel, Birgit E. Alber, Georg Fuchs, and Daniel Kockelkorn

Subjects
Archaeal Proteins, Coenzyme A, Hydroxybutyrates, Reductase, Biology, Models, Biological, Microbiology, Genes, Archaeal, chemistry.chemical_compound, Enoyl-CoA Hydratase, Molecular Biology, Sequence Homology, Amino Acid, Chloroflexus aurantiacus, Enoyl-CoA hydratase, biology.organism_classification, Enzymes and Proteins, chemistry, Biochemistry, Metallosphaera sedula, Dehydratase, Acyl Coenzyme A, Propionates, Oxidoreductases, Sulfolobales, Metabolic Networks and Pathways, NADP, Metallosphaera
Abstract

A 3-hydroxypropionate/4-hydroxybutyrate cycle operates in autotrophic CO 2 fixation in various Crenarchaea , as studied in some detail in Metallosphaera sedula . This cycle and the autotrophic 3-hydroxypropionate cycle in Chloroflexus aurantiacus have in common the conversion of acetyl-coenzyme A (CoA) and two bicarbonates via 3-hydroxypropionate to succinyl-CoA. Both cycles require the reductive conversion of 3-hydroxypropionate to propionyl-CoA. In M. sedula the reaction sequence is catalyzed by three enzymes. The first enzyme, 3-hydroxypropionyl-CoA synthetase, catalyzes the CoA- and MgATP-dependent formation of 3-hydroxypropionyl-CoA. The next two enzymes were purified from M. sedula or Sulfolobus tokodaii and studied. 3-Hydroxypropionyl-CoA dehydratase, a member of the enoyl-CoA hydratase family, eliminates water from 3-hydroxypropionyl-CoA to form acryloyl-CoA. Acryloyl-CoA reductase, a member of the zinc-containing alcohol dehydrogenase family, reduces acryloyl-CoA with NADPH to propionyl-CoA. Genes highly similar to the Metallosphaera CoA synthetase, dehydratase, and reductase genes were found in autotrophic members of the Sulfolobales . The encoded enzymes are only distantly related to the respective three enzyme domains of propionyl-CoA synthase from C. aurantiacus , where this trifunctional enzyme catalyzes all three reactions. This indicates that the autotrophic carbon fixation cycles in Chloroflexus and in the Sulfolobales evolved independently and that different genes/enzymes have been recruited in the two lineages that catalyze the same kinds of reactions.

Published
2009

33. Biochemical establishment and characterization of EncM's flavin-N5-oxide cofactor

Author

Robin Teufel, Bruce A. Palfey, Michael J. Meehan, Quentin Michaudel, Frederick Stull, Pieter C. Dorrestein, and Bradley S. Moore

Subjects
Nitrosamines, Stereochemistry, Flavin group, Oxidative phosphorylation, Photochemistry, Biochemistry, Catalysis, Cofactor, Article, Substrate Specificity, chemistry.chemical_compound, Colloid and Surface Chemistry, Bacterial Proteins, Flavins, biology, Chemistry, Superoxide, Proteolytic enzymes, Substrate (chemistry), Oxides, General Chemistry, Monooxygenase, Streptomyces, Covalent bond, biology.protein, Oxidation-Reduction, Signal Transduction
Abstract

The ubiquitous flavin-dependent monooxygenases commonly catalyze oxygenation reactions by means of a transient C4a-peroxyflavin. A recent study, however, suggested an unprecedented flavin-oxygenating species, proposed as the flavin-N5-oxide (Fl(N5[O])), as key to an oxidative Favorskii-type rearrangement in the biosynthesis of the bacterial polyketide antibiotic enterocin. This stable superoxidized flavin is covalently tethered to the enzyme EncM and converted into FADH2 (Fl(red)) during substrate turnover. Subsequent reaction of Fl(red) with molecular oxygen restores the postulated Fl(N5[O]) via an unknown pathway. Here, we provide direct evidence for the Fl(N5[O]) species via isotope labeling, proteolytic digestion, and high-resolution tandem mass spectrometry of EncM. We propose that formation of this species occurs by hydrogen-transfer from Fl(red) to molecular oxygen, allowing radical coupling of the formed protonated superoxide and anionic flavin semiquinone at N5, before elimination of water affords the Fl(N5[O]) cofactor. Further biochemical and spectroscopic investigations reveal important features of the Fl(N5[O]) species and the EncM catalytic mechanism. We speculate that flavin-N5-oxides may be intermediates or catalytically active species in other flavoproteins that form the anionic semiquinone and promote access of oxygen to N5.

Published
2015

34. ChemInform Abstract: One-Pot Enzymatic Synthesis of Merochlorin A and B

Author

Robin Teufel, Phil S. Baran, Matthew T. Villaume, Bradley S. Moore, Mary K. Carbullido, Leonard Kaysser, and Stefan Diethelm

Subjects
Terpene, Chemistry, Organic chemistry, General Medicine, Enzymatic synthesis
Abstract

These are the first examples of total enzymatic syntheses of meroterpenoid natural products.

Published
2015

35. Direct capture and heterologous expression of Salinispora natural product genes for the biosynthesis of enterocin

Author

Bradley S. Moore, Max Crüsemann, Bailey Bonet, Robin Teufel, and Nadine Ziemert

Subjects
Bridged-Ring Compounds, Pharmaceutical Science, Marine Biology, 01 natural sciences, Streptomyces, Analytical Chemistry, Microbiology, 03 medical and health sciences, chemistry.chemical_compound, Polyketide synthase, Drug Discovery, Metabolome, Gene, 030304 developmental biology, Pharmacology, 0303 health sciences, Biological Products, Natural product, biology, Molecular Structure, 010405 organic chemistry, Drug discovery, Organic Chemistry, biology.organism_classification, Note, 0104 chemical sciences, Actinobacteria, Metabolic pathway, Complementary and alternative medicine, Biochemistry, chemistry, Multigene Family, biology.protein, Molecular Medicine, Heterologous expression, Polyketide Synthases
Abstract

Heterologous expression of secondary metabolic pathways is a promising approach for the discovery and characterization of bioactive natural products. Herein we report the first heterologous expression of a natural product from the model marine actinomycete genus Salinispora. Using the recently developed method of yeast-mediated transformation-associated recombination for natural product gene clusters, we captured a type II polyketide synthase pathway from Salinispora pacifica with high homology to the enterocin pathway from Streptomyces maritimus and successfully produced enterocin in two different Streptomyces host strains. This result paves the way for the systematic interrogation of Salinispora’s promising secondary metabolome.

Published
2014

36. Probing the structural requisites for enzymatic flavin-N5-oxide formation

Author

Robin Teufel and Raspudin Saleem Batcha

Subjects
Inorganic Chemistry, chemistry.chemical_classification, chemistry.chemical_compound, Enzyme, Structural Biology, Chemistry, Oxide, General Materials Science, Flavin group, Physical and Theoretical Chemistry, Condensed Matter Physics, Biochemistry, Combinatorial chemistry
Published
2016

37. An oxygenase that forms and deoxygenates toxic epoxide

Author

Thorsten Friedrich, Georg Fuchs, and Robin Teufel

Subjects
Enzyme complex, Oxygenase, Multidisciplinary, Catabolism, Stereochemistry, Coenzyme A, Iron, Molecular Sequence Data, Epoxide, Phenylalanine, Monooxygenase, Oxygen, chemistry.chemical_compound, chemistry, Biochemistry, Multienzyme Complexes, Pseudomonas, Biocatalysis, Oxygenases, Epoxy Compounds, Thiolester Hydrolases, Intracellular, Phenylacetates
Abstract

The epoxidase PaaABCE, which converts phenylacetyl-CoA into its ring-1,2-epoxide, is shown to be also able to mediate the NADPH-dependent removal of that epoxide, ensuring that the intracellular concentrations of the toxic epoxide does not exceed a certain ‘acceptable’ concentration. Here, Teufel et al. biochemically characterize the epoxidase PaaABCE, which is responsible for phenylalanine/phenylacetate degradation in many bacteria. They find that this di-iron-containing enzyme complex, which converts phenylacetyl-CoA into its ring-1,2-epoxide, is also able to mediate the NADPH-dependent removal of that epoxide. The authors suggest that this 'bifunctionality' may ensure that the intracellular concentrations of the toxic epoxide do not exceed a certain 'acceptable' concentration if, for example, the subsequent steps in the catabolic pathway are impeded. Catabolism may give rise to toxic intermediates that compromise cell vitality, such as epoxide formation in the recently elucidated and apparently universal bacterial coenzyme A (CoA)-dependent degradation of phenylacetic acid1. This compound is central to the catabolism of a variety of aromatics, such as phenylalanine, lignin-related compounds or environmental contaminants2,3. The key phenylacetyl-CoA monooxygenase (epoxidase) of the pathway, PaaABCE1,4,5, is also connected to the production of various primary and secondary metabolites6,7,8,9, as well as to the virulence of certain pathogens1,10,11. However, the enzyme complex has so far not been investigated in detail. Here we characterize the bacterial multicomponent monooxygenase PaaABCE that, surprisingly, not only transforms phenylacetyl-CoA into its ring-1,2-epoxide, but also mediates the NADPH-dependent removal of the epoxide oxygen, regenerating phenylacetyl-CoA with formation of water. We provide evidence for a catalytic di-iron centre that is probably the key to the unprecedented deoxygenation of an organic compound by an oxygenase. Presumably, the bifunctionality is vital to avoid toxic intracellular epoxide levels if the subsequent catabolic steps are impeded. Our data suggest that detoxification is assisted by two thioesterases (PaaI and PaaY) forming non-reactive breakdown products. Hence, PaaABCE may harbour an intrinsic escape mechanism from its own toxic product and represents the archetype of a bifunctional oxygenase/deoxygenase. Analogous reactions may possibly be catalysed by other di-iron epoxidases.

Published
2011

38. Studies on the mechanism of ring hydrolysis in phenylacetate degradation: a metabolic branching point

Author

Robin, Teufel, Carla, Gantert, Michaela, Voss, Wolfgang, Eisenreich, Wolfgang, Haehnel, and Georg, Fuchs

Subjects
Bacterial Proteins, Hydrolysis, Oxepins, Rhodocyclaceae, Enzymology, Coenzyme A, Aldehyde Dehydrogenase, NAD, Enoyl-CoA Hydratase, Phenylacetates
Abstract

The widespread, long sought-after bacterial aerobic phenylalanine/phenylacetate catabolic pathway has recently been elucidated. It proceeds via coenzyme A (CoA) thioesters and involves the epoxidation of the aromatic ring of phenylacetyl-CoA, subsequent isomerization to an uncommon seven-membered C-O-heterocycle (oxepin-CoA), and non-oxygenolytic ring cleavage. Here we characterize the hydrolytic oxepin-CoA ring cleavage catalyzed by the bifunctional fusion protein PaaZ. The enzyme consists of a C-terminal (R)-specific enoyl-CoA hydratase domain (formerly MaoC) that cleaves the ring and produces a highly reactive aldehyde and an N-terminal NADP(+)-dependent aldehyde dehydrogenase domain that oxidizes the aldehyde to 3-oxo-5,6-dehydrosuberyl-CoA. In many phenylacetate-utilizing bacteria, the genes for the pathway exist in a cluster that contains an NAD(+)-dependent aldehyde dehydrogenase in place of PaaZ, whereas the aldehyde-producing hydratase is encoded outside of the cluster. If not oxidized immediately, the reactive aldehyde condenses intramolecularly to a stable cyclic derivative that is largely prevented by PaaZ fusion in vivo. Interestingly, the derivative likely serves as the starting material for the synthesis of antibiotics (e.g. tropodithietic acid) and other tropone/tropolone related compounds as well as for ω-cycloheptyl fatty acids. Apparently, bacteria made a virtue out of the necessity of disposing the dead-end product with ring hydrolysis as a metabolic branching point.

Published
2011

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