Redox‐Polymer‐Based High‐Current‐Density Gas‐Diffusion H<sub>2</sub>‐Oxidation Bioanode Using [FeFe] Hydrogenase from <i>Desulfovibrio desulfuricans</i> in a Membrane‐free Biofuel Cell

Szczesny, Julian; Birrell, James A.; Conzuelo, Felipe; Lubitz, Wolfgang; Ruff, Adrian; Schuhmann, Wolfgang

doi:10.1002/anie.202006824

Cited by 23 publications

(18 citation statements)

References 47 publications

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“…Additionally, we observed complex redox behavior in Cp HydA1 PDT , the hydrogenase containing F-clusters, which can only be explained through a redox anticooperative interaction between [4Fe–4S] H and the F-clusters. Because [FeFe] hydrogenases have recently come to the fore as potentially useful catalysts for incorporation into redox-hydrogel-based fuel cells, − understanding their mechanism and how their structure influences their activity is of particular relevance.…”

Section: Introductionmentioning

confidence: 99%

Insight into the Redox Behavior of the [4Fe–4S] Subcluster in [FeFe] Hydrogenases

et al. 2020

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[FeFe] hydrogenases are efficient catalysts for interconverting hydrogen with protons and electrons, whose catalytic mechanism remains a subject of controversy. Their active site, the H‑cluster, is composed of a [4Fe–4S] subcluster ([4Fe–4S]H) covalently attached to a [2Fe] subcluster ([2Fe]H). The two subclusters are strongly redox-coupled, and proton-coupled electron transfer (PCET) within the H-cluster is thought to be essential for catalytic activity. Additionally, proton-coupled reduction of [4Fe–4S]H has been proposed. Here, we investigated the pH dependence of the redox behavior of [4Fe–4S]H using infrared (IR) spectroelectrochemistry with two different [FeFe] hydrogenases: CrHydA1 from Chlamydomonas reinhardtii and CpHydA1 from Clostridium pasteurianum. Contrary to previous reports, we find that, under our experimental conditions, the redox potential of [4Fe–4S]H is independent of pH around physiological values for both enzymes. We also found redox anticooperativity behavior between [4Fe–4S]H and the accessory [4Fe–4S] clusters (F-clusters) in CpHydA1, which tunes catalysis at the active site. Taken together, these results indicate that the catalytic cycle of [FeFe] hydrogenases likely does not involve protonation at or near [4Fe–4S]H, and instead, favors a model in which protonation of [2Fe]H drives catalysis. Our findings shed new light on the catalytic mechanism of [FeFe] hydrogenases and highlight the importance of the F-clusters in fine-tuning catalysis.

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Section: Introductionmentioning

confidence: 99%

Insight into the Redox Behavior of the [4Fe–4S] Subcluster in [FeFe] Hydrogenases

et al. 2020

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“…This potential difference is sufficiently large to invoke a high driving force for H 2 oxidation, but it is still low enough to guarantee a large open‐circuit voltage in a corresponding biofuel cell. [ 33 ] The optimization of the polymer loading on the electrode in a two‐layer approach (Figure 2b), similar to the ones described in our previous work, [ 16–18 ] yielded highly stable GDEs with immobilized [NiFe] hydrogenase from Desulfovibrio vulgaris Miyazaki F ( Dv MF).…”

Section: Resultsmentioning

confidence: 65%

“…In our previous work, we combined the benefits of redox polymers, namely protection of the enzyme and high catalyst loading, with the concept of gas diffusion electrodes to fabricate high performance H 2 oxidation bioanodes using various hydrogenases as biocatalysts. [ 17,18,30 ] Surprisingly, the catalytic current response of these electrodes did not scale with the intrinsic activity of the employed hydrogenase. [ 17 ] Since H 2 mass transport limitation could be ruled out when using GDEs, the limited current densities achieved, especially in the case of the most active [FeFe] hydrogenase, [ 18 ] may be attributed to insufficient electron transfer kinetics within the redox polymer film.…”

Section: Introductionmentioning

confidence: 99%

“…[ 17,18,30 ] Surprisingly, the catalytic current response of these electrodes did not scale with the intrinsic activity of the employed hydrogenase. [ 17 ] Since H 2 mass transport limitation could be ruled out when using GDEs, the limited current densities achieved, especially in the case of the most active [FeFe] hydrogenase, [ 18 ] may be attributed to insufficient electron transfer kinetics within the redox polymer film. [ 17 ] To prevent direct electron transfer with the immobilized hydrogenase, which would lead to undesired enzyme inactivation, an initial coating of the GDE surface with a layer of only the redox polymer without any enzyme was used as an adhesion layer between the electrode surface and the catalytically active layer comprising a mixture of redox polymer and hydrogenase.…”

Section: Introductionmentioning

confidence: 99%

“…We assume that by this the probability of the collision between adjacent viologen units within the redox polymer layer is insufficient to allow charge transfer at the rate necessary for the most active hydrogenase at high enzyme loading and unlimited H 2 supply within the GDE. [ 17,18,30 ]…”

Section: Introductionmentioning

confidence: 99%

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Enhancing the catalytic current response of H₂ oxidation gas diffusion bioelectrodes using an optimized viologen‐based redox polymer and [NiFe] hydrogenase

Lielpētere

Becker

Szczesny

et al. 2021

Electrochemical Science Adv

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Using viologen-based redox polymers to wire a variety of different hydrogenases to electrodes and gas diffusion electrodes is the basis to mitigate high potential deactivation of the enzyme, deactivation by molecular O 2 , as well as for highcurrent density H 2 oxidation bioanodes. To overcome electron transfer limitations by electron hopping within the viologen-modified polymer film, a new redox polymer was designed with the highest possible viologen content together with monomers bearing crosslinking units. In combination with an immobilization sequence consisting of oxidative grafting of amino functions, covalent attachment of polymer units to these functionalities, and crosslinking of the polymer layers, an unprecedently fast electron transfer became possible. This enabled a very high current density normalized by the amount of the [NiFe] hydrogenase embedded within a viologen polymer on gas diffusion electrodes.

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A Pyrene‐Triazacyclononane Anchor Affords High Operational Stability for CO₂RR by a CNT‐Supported Histidine‐Tagged CODH

et al. 2022

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An original 1-acetato-4-(1-pyrenyl)-1,4,7-triazacyclononane (AcPyTACN) was synthesized for the immobilization of a His-tagged recombinant CODH from Rhodospirillum rubrum (RrCODH) on carbonnanotube electrodes. The strong binding of the enzyme at the Ni-AcPyTACN complex affords a high current density of 4.9 mA cm À 2 towards electroenzymatic CO 2 reduction and a high stability of more than 6 × 10 6 TON when integrated on a gas-diffusion bioelectrode.

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Redox‐Polymer‐Based High‐Current‐Density Gas‐Diffusion H₂‐Oxidation Bioanode Using [FeFe] Hydrogenase from Desulfovibrio desulfuricans in a Membrane‐free Biofuel Cell

Cited by 23 publications

References 47 publications

Insight into the Redox Behavior of the [4Fe–4S] Subcluster in [FeFe] Hydrogenases

Insight into the Redox Behavior of the [4Fe–4S] Subcluster in [FeFe] Hydrogenases

Enhancing the catalytic current response of H₂ oxidation gas diffusion bioelectrodes using an optimized viologen‐based redox polymer and [NiFe] hydrogenase

A Pyrene‐Triazacyclononane Anchor Affords High Operational Stability for CO₂RR by a CNT‐Supported Histidine‐Tagged CODH

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Redox‐Polymer‐Based High‐Current‐Density Gas‐Diffusion H2‐Oxidation Bioanode Using [FeFe] Hydrogenase from Desulfovibrio desulfuricans in a Membrane‐free Biofuel Cell

Cited by 23 publications

References 47 publications

Insight into the Redox Behavior of the [4Fe–4S] Subcluster in [FeFe] Hydrogenases

Insight into the Redox Behavior of the [4Fe–4S] Subcluster in [FeFe] Hydrogenases

Enhancing the catalytic current response of H2 oxidation gas diffusion bioelectrodes using an optimized viologen‐based redox polymer and [NiFe] hydrogenase

A Pyrene‐Triazacyclononane Anchor Affords High Operational Stability for CO2RR by a CNT‐Supported Histidine‐Tagged CODH

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Product

Resources

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Redox‐Polymer‐Based High‐Current‐Density Gas‐Diffusion H₂‐Oxidation Bioanode Using [FeFe] Hydrogenase from Desulfovibrio desulfuricans in a Membrane‐free Biofuel Cell

Enhancing the catalytic current response of H₂ oxidation gas diffusion bioelectrodes using an optimized viologen‐based redox polymer and [NiFe] hydrogenase

A Pyrene‐Triazacyclononane Anchor Affords High Operational Stability for CO₂RR by a CNT‐Supported Histidine‐Tagged CODH