Literature DB >> 19419145

Electrostatic redesign of the [myoglobin, cytochrome b5] interface to create a well-defined docked complex with rapid interprotein electron transfer.

Peng Xiong1, Judith M Nocek, Amanda K K Griffin, Jingyun Wang, Brian M Hoffman.   

Abstract

Cyt b(5) is the electron-carrier "repair" protein that reduces met-Mb and met-Hb to their O(2)-carrying ferroheme forms. Studies of electron transfer (ET) between Mb and cyt b(5) revealed that they react on a "Dynamic Docking" (DD) energy landscape on which binding and reactivity are uncoupled: binding is weak and involves an ensemble of nearly isoenergetic configurations, only a few of which are reactive; those few contribute negligibly to binding. We set the task of redesigning the surface of Mb so that its reaction with cyt b(5) instead would occur on a conventional "simple docking" (SD) energy landscape, on which a complex exhibits a well-defined (set of) reactive binding configuration(s), with binding and reactivity thus no longer being decoupled. We prepared a myoglobin (Mb) triple mutant (D44K/D60K/E85K; Mb(+6)) substituted with Zn-deuteroporphyrin and monitored cytochrome b(5) (cyt b(5)) binding and electron transfer (ET) quenching of the (3)ZnMb(+6) triplet state. In contrast, to Mb(WT), the three charge reversals around the "front-face" heme edge of Mb(+6) have directed cyt b(5) to a surface area of Mb adjacent to its heme, created a well-defined, most-stable structure that supports good ET pathways, and apparently coupled binding and ET: both K(a) and k(et) are increased by the same factor of approximately 2 x 10(2), creating a complex that exhibits a large ET rate constant, k(et) = 10(6 1) s(-1), and is in slow exchange (k(off) << k(et)). In short, these mutations indeed appear to have created the sought-for conversion from DD to simple docking (SD) energy landscapes.

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Year:  2009        PMID: 19419145      PMCID: PMC2844781          DOI: 10.1021/ja902131d

Source DB:  PubMed          Journal:  J Am Chem Soc        ISSN: 0002-7863            Impact factor:   15.419


  19 in total

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3.  Catalysis of methaemoglobin reduction by erythrocyte cytochrome B5 and cytochrome B5 reductase.

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4.  Properties of methemoglobin reductase and kinetic study of methemoglobin reduction.

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5.  Effects of charged amino acid mutations on the bimolecular kinetics of reduction of yeast iso-1-ferricytochrome c by bovine ferrocytochrome b5.

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7.  Metmyoglobin reductase. Identification and purification of a reduced nicotinamide adenine dinucleotide-dependent enzyme from bovine heart which reduces metmyoglobin.

Authors:  L Hagler; R I Coppes; R H Herman
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9.  Dynamic docking and electron transfer between Zn-myoglobin and cytochrome b(5).

Authors:  Zhao-Xun Liang; Judith M Nocek; Kai Huang; Ryan T Hayes; Igor V Kurnikov; David N Beratan; Brian M Hoffman
Journal:  J Am Chem Soc       Date:  2002-06-19       Impact factor: 15.419

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Authors:  Zhao-Xun Liang; Igor V Kurnikov; Judith M Nocek; A Grant Mauk; David N Beratan; Brian M Hoffman
Journal:  J Am Chem Soc       Date:  2004-03-10       Impact factor: 15.419

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  7 in total

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5.  Evolving the [myoglobin, cytochrome b(5)] complex from dynamic toward simple docking: charging the electron transfer reactive patch.

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6.  Tryptophan-accelerated electron flow across a protein-protein interface.

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7.  Use of 3-aminotyrosine to examine the pathway dependence of radical propagation in Escherichia coli ribonucleotide reductase.

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  7 in total

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