Magnetic Circular Dichroism Spectroscopic Studies of Mononuclear Non-heme Iron Sites PDF Download

Author: Elizabeth Gottlieb Pavel
Publisher:
ISBN:
Category :
Languages : en
Pages : 342

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Author: Jing Zhou
Publisher:
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Category :
Languages : en
Pages : 398

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Publisher: Elsevier
ISBN: 0443313059
Category : Science
Languages : en
Pages : 348

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Mononuclear Non-heme Iron Dependent Enzymes, Volume 703 focuses on methods for studying, characterizing, and leveraging the chemistry of mononuclear non-heme iron dependent enzymes. Chapters in this new release include Photoreduction for Rieske oxygenase chemistry, Insights into the Mechanisms of Rieske Oxygenases from Studying the Unproductive Activation of Dioxygen, Non-heme iron and 2-oxoglutarate enzymes catalyze cyclopropane and azacyclopropane formations, Obtaining precise metrics of substrate positioning in Fe(II)/2OG dependent enzymes using Hyperfine Sublevel Correlation Spectroscopy, Xe-pressurization studies for revealing substrate-entrance tunnels, and much more. Additional chapters cover A tale of two dehydrogenases involved in NADH recycling, Rieske oxygenases and/or their partner reductase proteins, Expression, assay and inhibition of 9-cis-epoxycarotenoid dioxygenase (NCED) from Solanum lycopersicum and Zea mays, Biocatalysis and non-heme iron enzymes, In vitro analysis of the three-component Rieske oxygenase cumene dioxygenase from Pseudomonas fluorescens IP01, Structure and function of carbazole 1,9a-dioxygenase, Characterization of a Mononuclear Nonheme Iron-dependent Mono-oxygenase OzmD in Oxazinomycin Biosynthesis, and much more. Provides detailed articles regarding how to study the structures and mechanisms of mononuclear non-heme iron dependent enzymes Guides readers on how to use partner proteins in non-heme iron enzyme catalysis Includes strategies to employ mononuclear non-heme iron enzymes in biocatalytic applications

Author: Mark A. Pavlosky
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ISBN:
Category :
Languages : en
Pages : 368

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Author: Sabine Pulver
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Category :
Languages : en
Pages : 492

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Author: Tami E. Westre
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Category :
Languages : en
Pages : 674

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Author: Yan Zhang
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Category :
Languages : en
Pages : 438

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Author: James Malcolm McCormick
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Category :
Languages : en
Pages : 536

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Author: Andrea Decker
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Category :
Languages : en
Pages : 606

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Author: Shaun Di Hang Wong
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ISBN:
Category :
Languages : en
Pages :

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Mononuclear non-heme iron (NHFe) enzymes catalyze a wide variety of biologically-important reactions such as hydroxylation, halogenation, desaturation, ring closure, and electrophilic aromatic substitution. The key intermediate in the catalytic cycle is the S = 2 Fe(IV)=O species, capable of abstracting an H-atom from inert C--H bonds as strong as 106 kcal/mol. The Fe(IV)=O intermediate in enzymes is transient and difficult to trap; as such, stable synthetic analogs have proven invaluable for spectroscopic elucidation of the geometric/electronic structure of the Fe(IV)=O unit and how it is activated for reactivity. Such biomimetic Fe(IV)=O model complexes can be either intermediate-spin (S = 1) or high-spin (S = 2) in contrast to the S = 2 ground state of enzyme intermediates. For an S = 1 Fe(IV)=O species, the Fe--oxo [beta] [pi]*-frontier molecular orbital (FMO) [from the combination of Fe d(xz/yz) and oxo p(x/y)] is involved in H-atom abstraction, and this FMO requires a side-on approach ([pi]-attack) to achieve maximum overlap with the substrate C--H bond. Through magnetic circular dichroism (MCD) and nuclear vibrational resonance spectroscopy (NRVS) studies, the reactivity of the S = 1 Fe(IV)=O unit has been shown to be affected by the oxo contribution in the [pi]*-FMO, where a larger oxo contribution results in greater orbital overlap (with the substrate C--H) and higher reactivity; also, the [pi]-attack pathway results in steric clashes between substrate and ligand, giving a significant steric contribution to the energy of the reaction barrier. For an S = 2 Fe(IV)=O species, the Fe--oxo [alpha] [sigma]*-FMO [Fe d(z2) and oxo p(z)] is spin-polarized (exchange-stabilized) to an energy level comparable with its [pi]*-FMO, making it accessible as a second pathway ([sigma]-attack) for reactivity. In the S = 2 Fe(IV)=O model complex ligated by TMG3tren, this [sigma]*-FMO is active but is axially hindered by the ligand, again giving a large steric contribution to the reaction barrier; however, the intrinsic electronic reaction barriers of the S = 2 [sigma]*-FMO and the S = 1 [pi]*-FMO are comparable, suggesting they are similarly active in H-atom abstraction. Furthermore, MCD excited-state spectroscopy in combination with multiconfigurational calculations on the S = 2 model reveal two different [pi]-pathways for reactivity involving Fe(III)--oxyl[p(x), [pi]] character, in addition to the [sigma]-pathway involving Fe(III)--oxyl[p(z), [sigma]] character, showing that the S = 2 Fe(IV)=O unit is activated for both [pi] and [sigma] H-atom abstraction reactivities. Finally, the S = 2 enzyme intermediate for the halogenase SyrB2 was trapped and structurally characterized by NRVS, revealing two possible 5-coordinate trigonal bipyramidal candidates with the Fe--oxo vector oriented either perpendicular or parallel to the substrate C--H bond. Importantly, this difference in orientation leads to Fe(III)--OH products oriented efficiently for different rebound reactivities -- native halogenation in the case of perpendicular orientation and non-native hydroxylation in the case of parallel orientation.