Characterization of a Citrulline 4‐Hydroxylase from Nonribosomal Peptide GE81112 Biosynthesis and Engineering of Its Substrate Specificity for the Chemoenzymatic Synthesis of Enduracididine

Zwick, Christian R.; Sosa, Max; Renata, Hans

doi:10.1002/anie.201910659

Cited by 41 publications

(27 citation statements)

References 42 publications

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“…These enzymes were studied spectroscopically and kinetically and their substrate specificity tested. Recent studies on the nonheme iron enzyme GetI showed it to hydroxylate l ‐Arg at the C 4 ‐position, although it was not clear whether arginine is its natural substrate [7] . A similar situation was found in the ethylene forming enzyme that apart from catabolizing αKG into ethene and three CO 2 molecules, also appears to bind and activate an arginine residue but hydroxylate it at the C 5 ‐position [8] .…”

Section: Introductionmentioning

confidence: 94%

What Determines the Selectivity of Arginine Dihydroxylation by the Nonheme Iron Enzyme OrfP?

Ali

Henchman

Visser

2020

Chemistry A European J

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The nonheme iron enzyme OrfP reacts with l‐Arg selectively to form the 3R,4R‐dihydroxyarginine product, which in mammals can inhibit the nitric oxide synthase enzymes involved in blood pressure control. To understand the mechanisms of dioxygen activation of l‐Arg by OrfP and how it enables two sequential oxidation cycles on the same substrate, we performed a density functional theory study on a large active site cluster model. We show that substrate binding and positioning in the active site guides a highly selective reaction through C3−H hydrogen atom abstraction. This happens despite the fact that the C3−H and C4−H bond strengths of l‐Arg are very similar. Electronic differences in the two hydrogen atom abstraction pathways drive the reaction with an initial C3−H activation to a low‐energy 5σ‐pathway, while substrate positioning destabilizes the C4−H abstraction and sends it over the higher‐lying 5π‐pathway. We show that substrate and monohydroxylated products are strongly bound in the substrate binding pocket and hence product release is difficult and consequently its lifetime will be long enough to trigger a second oxygenation cycle.

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Section: Introductionmentioning

confidence: 94%

What Determines the Selectivity of Arginine Dihydroxylation by the Nonheme Iron Enzyme OrfP?

Ali

Henchman

Visser

2020

Chemistry A European J

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“…Between June and October of 2019, additional papers describing pathways to free-standing α-amino acids have appeared in the biosynthetic literature. For interested readers, these references are cited here without further description. − …”

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confidence: 99%

Biosynthetic Pathways to Nonproteinogenic α-Amino Acids

2019

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Natural nonproteinogenic amino acids vastly outnumber the well-known 22 proteinogenic amino acids. Such amino acids are generated in specialized metabolic pathways. In these pathways, diverse biosynthetic transformations, ranging from isomerizations to the stereospecific functionalization of C–H bonds, are employed to generate structural diversity. The resulting nonproteinogenic amino acids can be integrated into more complex natural products. Here we review recently discovered biosynthetic routes to freestanding nonproteinogenic α-amino acids, with an emphasis on work reported between 2013 and mid-2019.

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“…In 2019, we determined that GetI functions as a citrulline-4-hydroxylase, instead of a chlorohistidine hydroxylase, and is probably responsible for the biosynthesis of the second monomer of all three GE81112s. 63 Furthermore, sequencebased rational mutagenesis identified a variant of GetI, containing four mutations away from wild-type, that exhibits a complete switch in substrate preference from citrulline to arginine. The functional characterization of GetI provided an opportunity to construct the first two amino acid monomers of GE81112 B1 chemoenzymatically.…”

Section: Chemoenzymatic Synthesis Of Ge81112 B1 and Related Analoguesmentioning

confidence: 99%

Exploration of Iron- and α-Ketoglutarate-Dependent Dioxygenases as Practical Biocatalysts in Natural Product Synthesis

Renata

2020

Synlett

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Catalytic C–H oxidation is a powerful transformation with enormous promise to streamline access to complex molecules. In recent years, biocatalytic C–H oxidation strategies have received tremendous attention due to their potential to address unmet regio- and stereoselectivity challenges that are often encountered with the use of small-molecule-based catalysts. This Account provides an overview of recent contributions from our laboratory in this area, specifically in the use of iron- and α-ketoglutarate-dependent dioxygenases in chemoenzymatic syntheses of complex natural products.1 Introduction2 Overview of Natural Oxygenases3 C5 Hydroxylation of Aliphatic Amino Acids4 Chemoenzymatic Synthesis of Tambromycin5 Chemoenzymatic Synthesis of Cepafungin I and Related Analogues6 Chemoenzymatic Synthesis of GE81112 B1 and Related Analogues7 Conclusion and Future Direction

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Characterization of a Citrulline 4‐Hydroxylase from Nonribosomal Peptide GE81112 Biosynthesis and Engineering of Its Substrate Specificity for the Chemoenzymatic Synthesis of Enduracididine

Cited by 41 publications

References 42 publications

What Determines the Selectivity of Arginine Dihydroxylation by the Nonheme Iron Enzyme OrfP?

What Determines the Selectivity of Arginine Dihydroxylation by the Nonheme Iron Enzyme OrfP?

Biosynthetic Pathways to Nonproteinogenic α-Amino Acids

Exploration of Iron- and α-Ketoglutarate-Dependent Dioxygenases as Practical Biocatalysts in Natural Product Synthesis

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