Proline 107 Is a Major Determinant in Maintaining the Structure of the Distal Pocket and Reactivity of the High-Spin Heme of MauG

Feng, Manliang; Jensen, L.M.R.; Yukl, Erik T.; Wei, Xiang; Liu, Aimin; Wilmot, Carrie M.; Davidson, Victor L.

doi:10.1021/bi201882e

Cited by 28 publications

(76 citation statements)

References 34 publications

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“…3E). Both variants were shown to be capable of stabilizing the bis-Fe(IV) species (25,26). In contrast, the NIR spectral feature was not observed in Y294H MauG upon addition of H 2 O 2 ( Fig.…”

Section: Resultsmentioning

confidence: 95%

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Tryptophan-mediated charge-resonance stabilization in the bis -Fe(IV) redox state of MauG

Geng

Dornevil

Davidson

et al. 2013

Proc. Natl. Acad. Sci. U.S.A.

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102

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The diheme enzyme MauG catalyzes posttranslational modifications of a methylamine dehydrogenase precursor protein to generate a tryptophan tryptophylquinone cofactor. The MauG-catalyzed reaction proceeds via a bis -Fe(IV) intermediate in which one heme is present as Fe(IV)=O and the other as Fe(IV) with axial histidine and tyrosine ligation. Herein, a unique near-infrared absorption feature exhibited specifically in bis -Fe(IV) MauG is described, and evidence is presented that it results from a charge-resonance-transition phenomenon. As the two hemes are physically separated by 14.5 Å, a hole-hopping mechanism is proposed in which a tryptophan residue located between the hemes is reversibly oxidized and reduced to increase the effective electronic coupling element and enhance the rate of reversible electron transfer between the hemes in bis -Fe(IV) MauG. Analysis of the MauG structure reveals that electron transfer via this mechanism is rapid enough to enable a charge-resonance stabilization of the bis -Fe(IV) state without direct contact between the hemes. The finding of the charge-resonance-transition phenomenon explains why the bis -Fe(IV) intermediate is stabilized in MauG and does not permanently oxidize its own aromatic residues.

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Section: Resultsmentioning

confidence: 95%

“…PreMADH was expressed in Rhodobacter sphaeroides. These proteins were purified as described previously (9,13,16,25,26).…”

Section: Methodsmentioning

confidence: 99%

Tryptophan-mediated charge-resonance stabilization in the bis -Fe(IV) redox state of MauG

Geng

Dornevil

Davidson

et al. 2013

Proc. Natl. Acad. Sci. U.S.A.

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102

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“…The bis-Fe IV state of MauG describes an alternative strategy by which to stabilize a high-valent heme iron. Several amino acid residues in the proximity of the two hemes have also been implicated in facilitating the formation and stabilizing the bis-Fe IV state (21,(28)(29)(30)(31)(32). The concept of CR stabilization of this high-valent state led to the description of it actually comprising an ensemble of resonance structures including the more traditional high-valent heme species, but with the true bis-Fe IV state as the dominant species (6, 9) (Fig.…”

Section: Two Reaction Steps In the Conversion Of The Bis-fementioning

confidence: 99%

“…Pro107 which also resides in the heme pocket was also shown to be important. Mutations of this residue disrupted the position and orientation of Glu113, which in turn altered the water network (29). Mutations of Pro107 as well as a Q103A mutation also increased the susceptibility of the three Met residues to autooxidation (15,29).…”

Section: Tsmentioning

confidence: 99%

Roles of multiple-proton transfer pathways and proton-coupled electron transfer in the reactivity of the bis -Fe ^IV state of MauG

Williamson

Davidson

2015

Proc. Natl. Acad. Sci. U.S.A.

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The high-valent state of the diheme enzyme MauG exhibits charge–resonance (CR) stabilization in which the major species is a bis-FeIV state with one heme present as FeIV=O and the other as FeIV with axial heme ligands provided by His and Tyr side chains. In the absence of its substrate, the high-valent state is relatively stable and returns to the diferric state over several minutes. It is shown that this process occurs in two phases. The first phase is redistribution of the resonance species that support the CR. The second phase is the loss of CR and reduction to the diferric state. Thermodynamic analysis revealed that the rates of the two phases exhibited different temperature dependencies and activation energies of 8.9 and 19.6 kcal/mol. The two phases exhibited kinetic solvent isotope effects of 2.5 and 2.3. Proton inventory plots of each reaction phase exhibited extreme curvature that could not be fit to models for one- or multiple-proton transfers in the transition state. Each did fit well to a model for two alternative pathways for proton transfer, each involving multiple protons. In each case the experimentally determined fractionation factors were consistent with one of the pathways involving tunneling. The percent of the reaction that involved the tunneling pathway differed for the two reaction phases. Using the crystal structure of MauG it was possible to propose proton–transfer pathways consistent with the experimental data using water molecules and amino acid side chains in the distal pocket of the high-spin heme.

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“…Such studies with biologically relevant diatomic gases have been carried out both experimentally and theoretically with various proteins. Experimentally, by i) mapping the location of Xe-atoms on pressurizing the protein with Xe gas [5], implicitly assuming that the binding sites for Xe-atoms are the same as for diatomic gases, because of similar steric bulk and polarity, ii) locating the preferred channels by using molecules that elongate on the channels that connect the protein-active center to the solvent medium [6], iii) using protein mutants to verify the relevance of key residues as to the displacement of the gaseous molecules [7], and iv) detecting conformational changes for close-lying residues on formation of the complex between the protein and the diatomic gas [8]. Theoretical approaches include PMF [9] and 3D-RISM calculations [10], as well as classical MD [11] and biased MD, such as TAMD [12], and RAMD [13].…”

Section: Basis and Scope Of Present Workmentioning

confidence: 99%

Gates and Binding Pockets for Nitric Oxide with Cytochrome c′, According to Molecular Dynamics

Pietra

2013

Chemistry & Biodiversity

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Random-acceleration molecular-dynamics (RAMD) simulations with models of homodimeric 6-ligated distal-NO and 5-ligated proximal-NO cytochrome c' complexes, in TIP3 H2 O, showed two distinct, non-intercommunicating worlds. In the framework of a long cavity formed by four protein helices with heme at one extremity, NO was observed to follow different pathways with the two complexes to reach the solvent. With the 6-ligated complex, NO was observed to progress by exploiting protein internal channels created by thermal fluctuations, and be temporarily trapped into binding pockets before reaching the preferred gate at the heme end of the cavity. In contrast, with the 5-ligated complex, NO was observed to surface the solvent-exposed helix 7, up to a gate at the other extremity of the protein, only occasionally finding an earlier, direct way out toward the solvent. That only bulk NO gets involved in forming the 5-ligated proximal-NO complex is in agreement with previous experimental observations, while the occurrence of binding pockets suggests that also reservoir NO might play a role with the distal-NO complex.

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Proline 107 Is a Major Determinant in Maintaining the Structure of the Distal Pocket and Reactivity of the High-Spin Heme of MauG

Cited by 28 publications

References 34 publications

Tryptophan-mediated charge-resonance stabilization in the bis -Fe(IV) redox state of MauG

Tryptophan-mediated charge-resonance stabilization in the bis -Fe(IV) redox state of MauG

Roles of multiple-proton transfer pathways and proton-coupled electron transfer in the reactivity of the bis -Fe ^IV state of MauG

Gates and Binding Pockets for Nitric Oxide with Cytochrome c′, According to Molecular Dynamics

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Proline 107 Is a Major Determinant in Maintaining the Structure of the Distal Pocket and Reactivity of the High-Spin Heme of MauG

Cited by 28 publications

References 34 publications

Tryptophan-mediated charge-resonance stabilization in the bis -Fe(IV) redox state of MauG

Tryptophan-mediated charge-resonance stabilization in the bis -Fe(IV) redox state of MauG

Roles of multiple-proton transfer pathways and proton-coupled electron transfer in the reactivity of the bis -Fe IV state of MauG

Gates and Binding Pockets for Nitric Oxide with Cytochrome c′, According to Molecular Dynamics

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Roles of multiple-proton transfer pathways and proton-coupled electron transfer in the reactivity of the bis -Fe ^IV state of MauG