Active Multienzyme Assemblies for Long-Chain Olefinic Hydrocarbon Biosynthesis

Christenson, James K.; Jensen, Matthew R.; Goblirsch, B.R.; Mohamed, Fatuma A.; Zhang, Wei; Wilmot, Carrie M.; Wackett, Lawrence P.

doi:10.1128/jb.00890-16

Cited by 17 publications

(20 citation statements)

References 26 publications

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“…It is hypothesized that the final decarboxylation to form the cis -olefin product is catalyzed by OleB (α/β-hydrolase superfamily) [10]. OleBCD were proposed to form a multi-enzyme assembly that may function to efficiently move the hydrophobic pathway intermediates between enzyme active sites, preserve the stereochemistry, and sequester the highly reactive β-lactone from the cell [11]. As well as initiating the pathway, OleA has been proposed to act as a shuttle between fatty acid metabolism and the OleBCD assembly feeding its β-keto acid product to OleD [11].…”

Section: Introductionmentioning

confidence: 99%

OleA Glu117 is key to condensation of two fatty-acyl coenzyme A substrates in long-chain olefin biosynthesis

Jensen

Goblirsch

Christenson

et al. 2017

Biochemical Journal

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In the interest of decreasing dependence on fossil fuels, microbial hydrocarbon biosynthesis pathways are being studied for renewable, tailored production of specialty chemicals and biofuels. One candidate is long-chain olefin biosynthesis, a widespread bacterial pathway that produces waxy hydrocarbons. Found in three- and four-gene clusters, oleABCD encode the enzymes necessary to produce cis-olefins that differ by alkyl chain length, degree of unsaturation, and alkyl chain branching. The first enzyme in the pathway, OleA, catalyzes the Claisen condensation of two fatty acyl-coenzyme A molecules to form a β-keto acid. In this report, the mechanistic role of Xanthomonas campestris OleA Glu117 is investigated through mutant enzymes. Crystal structures were determined for each mutant as well as their complex with the inhibitor cerulenin. Complemented by substrate modelling, these structures suggest that Glu117 aids in substrate positioning for productive carbon-carbon bond formation. Analysis of acyl-coenzyme A substrate hydrolysis shows diminished activity in all mutants. When the active site lacks an acidic residue in the 117 position, OleA cannot form condensed product, demonstrating Glu117 has a critical role upstream of the essential condensation reaction. Profiling of pH dependence shows that the apparent pKa for Glu117 is impacted by mutagenesis. Taken together, we propose that Glu117 is the general base needed to prime condensation via deprotonation of the second, non-covalently bound substrate during turnover. This is the first example of a member of the thiolase superfamily of condensing enzymes to contain an active site base originating from the second monomer of the dimer. Summary Statement OleA is the first reported thiolase enzyme whose active site general base, a glutamic acid (Glu117), is derived from a homodimeric interface. Structural and functional characterization of glutamatic acid mutants establishes its mechanistic role in initiating olefin biosynthesis.

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Section: Introductionmentioning

confidence: 99%

OleA Glu117 is key to condensation of two fatty-acyl coenzyme A substrates in long-chain olefin biosynthesis

Jensen

Goblirsch

Christenson

et al. 2017

Biochemical Journal

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“…The lactone synthase OleC forms a heat-labile internal ester between the β-hydroxy and the carboxyl group and one molecule of water is released. Finally, the lactone decarboxylase OleB liberates one molecule of CO 2 and converts the internal lactone into an alkene with a cis-configured internal double bond (internal olefins) at the connection point of the two original fatty acid precursors (Beller et al [3]) (Sukovich et al [14]) (Frias et al [7]) (Christenson et al [4]) (Christenson, Richman et al [6]) (Christenson, Jensen et al [5]).…”

Section: Open Accessmentioning

confidence: 99%

“…The nature of such internal olefin hydrocarbons was first characterized in the Gram-positive Sarcina lutea (now Kocuria rhizophila) (Albro and Dittmer [1]) (Tornabene et al [17]), and the oleABCD genes were first described in the Gram-positive Micrococcus luteus NCTC2665 (Beller et al [3]). Nevertheless, the catalytic mechanism of OleA as well as the order and nature of the reaction steps of the OleABCD enzymes, as summarized above, were finally elucidated mainly in the Gram-negative species Shewanella oneidensis (Sukovich et al [14]) and Xanthomonas campestris (Frias et al [7]) (Christenson et al [4]) (Christenson et al [6]) (Christenson et al [5]). In addition, the first report on the phylogenetic distribution and diversity of olefin production in bacteria by Sukovich et al [13] described bacterial olefin production as a predominately Gram-negative capability using species from four Gram-negative phyla (Proteobacteria, Planctomycetes, Chloroflexi, Verrucomicrobia) and one Gram-positive phylum (Actinobacteria) (Sukovich et al [13]).…”

Section: Open Accessmentioning

confidence: 99%

Distribution and diversity of olefins and olefin-biosynthesis genes in Gram-positive bacteria

Surger

Angelov

Liebl

2020

Biotechnol Biofuels

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Background: The natural production of olefins (unsaturated aliphatic hydrocarbons) by certain bacterial genera represents an alternative and sustainable source of biofuels and lubricant components. The biochemical steps of olefin biosynthesis via the ole pathway encoded by oleABCD have been unraveled recently, and the occurrence of olefins has been reported for several Gram-negative and Gram-positive bacteria. However, the distribution and diversity of olefins among the Gram-positive bacteria has not been studied in detail. Results:We report the distribution of olefin synthesis gene clusters in the bacterial domain and focus on the olefin composition and the determinants of olefin production within the phylum of Actinobacteria. The olefin profiles of numerous genera of the Micrococcales order were analyzed by GC/MS. We describe for the first time olefin synthesis in representatives of the genera Pseudarthrobacter, Paenarthrobacter, Glutamicibacter, Clavibacter, Rothia, Dermacoccus, Kytococcus, Curtobacterium, and Microbacterium. By exchange of the native ole genes of Micrococcus luteus with the corresponding genes of actinobacteria producing different olefins, we demonstrate that the olefin composition can be manipulated with respect to chain length and isomer composition. Conclusions:This study provides a catalogue of the diversity of olefin structures found in the Actinobacteria. Our ole gene swapping data indicate that the olefin structures are fundamentally determined by the substrate specificity of OleA, and at the same time by the availability of a sufficient supply of suitable fatty acyl-CoA substrates from cellular fatty acid metabolism. This makes OleA of Gram-positive bacteria a promising target for structural analysis and protein engineering aiming to generate olefin chain lengths and isomer profiles which are designed to match the requirements of various industrial applications.

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“…OleC, a β-lactone synthetase, then generates a β-lactone moiety (Christenson et al, 2017b) which is subsequently de-carboxylated by OleB, a β-lactone decarboxylase, yielding the final olefin product (Christenson et al, 2017c). Recent work has demonstrated that OleBCD together form a large multimeric enzyme complex that processes the β-keto intermediate formed by OleA activity (Christenson et al, 2017a). Weak interactions between the OleBCD complex and OleA in vitro suggests that OleA condenses the precursor acyl groups and possibly transfers the β-keto acid product directly to the OleBCD complex for further processing (Christenson et al, 2017a).…”

Section: Introductionmentioning

confidence: 99%

“…Recent work has demonstrated that OleBCD together form a large multimeric enzyme complex that processes the β-keto intermediate formed by OleA activity (Christenson et al, 2017a). Weak interactions between the OleBCD complex and OleA in vitro suggests that OleA condenses the precursor acyl groups and possibly transfers the β-keto acid product directly to the OleBCD complex for further processing (Christenson et al, 2017a). In the absence of downstream processing by OleBCD, the OleA catalyzed β-keto acid intermediate undergoes spontaneous decarboxylation to form a ketone product (Sukovich et al, 2010b; Frias et al, 2011; Figure 1).…”

Section: Introductionmentioning

confidence: 99%

Linkage of Marine Bacterial Polyunsaturated Fatty Acid and Long-Chain Hydrocarbon Biosynthesis

2019

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Various marine gamma-proteobacteria produce omega-3 polyunsaturated fatty acids, such as eicosapentaenoic acid (20:5, EPA) and docosahexaenoic acid (22:6, DHA), which are incorporated into membrane phospholipids. Five genes, designated pfaABCDE , encode the polyketide/fatty acid synthase necessary for production of these long-chain fatty acids. In addition to de novo biosynthesis of EPA and DHA, the “Pfa synthase” is also involved with production of a long-chain polyunsaturated hydrocarbon product (31:9, PUHC) in conjunction with the oleABCD hydrocarbon biosynthesis pathway. In this work, we demonstrate that OleA mediates the linkage between these two pathways in vivo . Co-expression of pfaA-E along with oleA from Shewanella pealeana in Escherichia coli yielded the expected product, a 31:8 ketone along with a dramatic ∼10-fold reduction in EPA content. The decrease in EPA content was independent of 31:8 ketone production as co-expression of an OleA active site mutant also led to identical decreases in EPA content. We also demonstrate that a gene linked with either pfa and/or ole operons in diverse bacterial lineages, herein designated pfaT , plays a role in maintaining optimal production of Pfa synthase derived products in Photobacterium and Shewanella species.

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Active Multienzyme Assemblies for Long-Chain Olefinic Hydrocarbon Biosynthesis

Cited by 17 publications

References 26 publications

OleA Glu117 is key to condensation of two fatty-acyl coenzyme A substrates in long-chain olefin biosynthesis

OleA Glu117 is key to condensation of two fatty-acyl coenzyme A substrates in long-chain olefin biosynthesis

Distribution and diversity of olefins and olefin-biosynthesis genes in Gram-positive bacteria

Linkage of Marine Bacterial Polyunsaturated Fatty Acid and Long-Chain Hydrocarbon Biosynthesis

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