The Hydricity and Reactivity Relationship in [ FeFe ]-hydrogenases

Artz, Jacob H.; Mulder, David W.; Ratzloff, Michael W.; Peters, John A.; King, Paul W.

doi:10.21203/rs.3.rs-77874/v1

Cited by 2 publications

(2 citation statements)

References 43 publications

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“…In the realm of structurefunction relationships, Kisgeropoulos et al investigated the effect of amino acid exchanges of the primary proteinaceous proton acceptor in [FeFe]-hydrogenase. The data expand previous work (Cornish et al, 2011;Morra et al, 2012;Duan et al, 2018;Artz et al, 2020), demonstrating that the pK a of the proton acceptor is one factor controlling the catalytic bias of the enzyme. Three further articles dealt with functional aspects of hydrogenases.…”

supporting

confidence: 89%

Editorial: Hydrogenase: structure, function, maturation, and application

Frielingsdorf,

Pinske,

Valetti

et al. 2023

Front. Microbiol.

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supporting

confidence: 89%

Editorial: Hydrogenase: structure, function, maturation, and application

Frielingsdorf,

Pinske,

Valetti

et al. 2023

Front. Microbiol.

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“…Using redox-dye mediated assays on the purified CrHydA1 C169S variant, H 2 oxidation and evolution activities were determined and compared to CaI C298S (Cornish et al, 2011) and CpII C169S (Artz et al, 2020a; Table 2). The reactivity results show a collective shift toward H 2 oxidation reactivity for all the enzymes.…”

Section: Cys→ser Variant Pka and Activity Profilesmentioning

confidence: 99%

The Contribution of Proton-Donor pKa on Reactivity Profiles of [FeFe]-hydrogenases

et al. 2022

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The [FeFe]-hydrogenases are enzymes that catalyze the reversible activation of H2 coupled to the reduction–oxidation of electron carriers. Members of the different taxonomic groups of [FeFe]-hydrogenases display a wide range of preference, or bias, for H2 oxidation or H2 production reactions, despite sharing a common catalytic cofactor, or H-cluster. Identifying the properties that control reactivity remains an active area of investigation, and models have emerged that include diversity in the catalytic site coordination environments and compositions of electron transfer chains. The kinetics of proton-coupled electron transfer at the H-cluster might be expected to be a point of control of reactivity. To test this hypothesis, systematic changes were made to the conserved cysteine residue that functions in proton exchange with the H-cluster in the three model enzymes: CaI, CpII, and CrHydA1. CaI and CpII both employ electron transfer accessory clusters but differ in bias, whereas CrHydA1 lacks accessory clusters having only the H-cluster. Changing from cysteine to either serine (more basic) or aspartate (more acidic) modifies the sidechain pKa and thus the barrier for the proton exchange step. The reaction rates for H2 oxidation or H2 evolution were surveyed and measured for model [FeFe]-hydrogenases, and the results show that the initial proton-transfer step in [FeFe]-hydrogenase is tightly coupled to the control of reactivity; a change from cysteine to more basic serine favored H2 oxidation in all enzymes, whereas a change to more acidic aspartate caused a shift in preference toward H2 evolution. Overall, the changes in reactivity profiles were profound, spanning 105 in ratio of the H2 oxidation-to-H2 evolution rates. The fact that the change in reactivity follows a common trend implies that the effect of changing the proton-transfer residue pKa may also be framed as an effect on the scaling relationship between the H-cluster di(thiolmethyl)amine (DTMA) ligand pKa and Em values of the H-cluster. Experimental observations that support this relationship, and how it relates to catalytic function in [FeFe]-hydrogenases, are discussed.

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The Hydricity and Reactivity Relationship in [ FeFe ]-hydrogenases

Cited by 2 publications

References 43 publications

Editorial: Hydrogenase: structure, function, maturation, and application

Editorial: Hydrogenase: structure, function, maturation, and application

The Contribution of Proton-Donor pKa on Reactivity Profiles of [FeFe]-hydrogenases

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