Crystal Structure, Exogenous Ligand Binding, and Redox Properties of an Engineered Diiron Active Site in a Bacterial Hemerythrin

Crystal Structure, Exogenous Ligand Binding, and Redox Properties of an Engineered Diiron Active Site in a Bacterial Hemerythrin

A nonheme diiron active site in a 13 kDa hemerythrin-like domain of the bacterial chemotaxis protein DcrH-Hr contains an oxo bridge, two bridging carboxylate groups from Glu and Asp residues, and five terminally ligated His residues. We created a unique diiron coordination sphere containing five His...

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Veröffentlicht in:Inorganic chemistry 2013-11, Vol.52 (22), p.13014-13020
Hauptverfasser: Okamoto, Yasunori, Onoda, Akira, Sugimoto, Hiroshi, Takano, Yu, Hirota, Shun, Kurtz, Donald M, Shiro, Yoshitsugu, Hayashi, Takashi
Format: Artikel
Sprache:eng
Schlagworte:
Amino Acid Substitution
Catalytic Domain
Crystallography, X-Ray
Desulfovibrio - chemistry
Desulfovibrio - enzymology
Desulfovibrio - genetics
Hemerythrin - chemistry
Hemerythrin - genetics
Hemerythrin - metabolism
Ligands
Models, Molecular
Oxidation-Reduction
Oxygen - metabolism
Protein Engineering
Spectrum Analysis, Raman
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container_end_page 13020
container_issue 22
container_start_page 13014
container_title Inorganic chemistry
container_volume 52
creator Okamoto, Yasunori
Onoda, Akira
Sugimoto, Hiroshi
Takano, Yu
Hirota, Shun
Kurtz, Donald M
Shiro, Yoshitsugu
Hayashi, Takashi
description A nonheme diiron active site in a 13 kDa hemerythrin-like domain of the bacterial chemotaxis protein DcrH-Hr contains an oxo bridge, two bridging carboxylate groups from Glu and Asp residues, and five terminally ligated His residues. We created a unique diiron coordination sphere containing five His and three Glu/Asp residues by replacing an Ile residue with Glu in DcrH-Hr. Direct coordination of the carboxylate group of E119 to Fe2 of the diiron site in the I119E variant was confirmed by X-ray crystallography. The substituted Glu is adjacent to an exogenous ligand-accessible tunnel. UV–vis absorption spectra indicate that the additional coordination of E119 inhibits the binding of the exogenous ligands azide and phenol to the diiron site. The extent of azide binding to the diiron site increases at pH ≤ 6, which is ascribed to protonation of the carboxylate ligand of E119. The diferrous state (deoxy form) of the engineered diiron site with the extra Glu residue is found to react more slowly than wild type with O2 to yield the diferric state (met form). The additional coordination of E119 to the diiron site also slows the rate of reduction from the met form. All these processes were found to be pH-dependent, which can be attributed to protonation state and coordination status of the E119 carboxylate. These results demonstrate that modifications of the endogenous coordination sphere can produce significant changes in the ligand binding and redox properties in a prototypical nonheme diiron-carboxylate protein active site.
doi_str_mv 10.1021/ic401632x
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subjects Amino Acid Substitution
Catalytic Domain
Crystallography, X-Ray
Desulfovibrio - chemistry
Desulfovibrio - enzymology
Desulfovibrio - genetics
Hemerythrin - chemistry
Hemerythrin - genetics
Hemerythrin - metabolism
Ligands
Models, Molecular
Oxidation-Reduction
Oxygen - metabolism
Protein Engineering
Spectrum Analysis, Raman
title Crystal Structure, Exogenous Ligand Binding, and Redox Properties of an Engineered Diiron Active Site in a Bacterial Hemerythrin
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