4.8 Article

Characterization of Photochemical Processes for H2 Production by CdS Nanorod-[FeFe] Hydrogenase Complexes

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JOURNAL OF THE AMERICAN CHEMICAL SOCIETY
卷 134, 期 12, 页码 5627-5636

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AMER CHEMICAL SOC
DOI: 10.1021/ja2116348

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  1. U.S. Department of Energy, Division of Chemical Sciences, Geosciences, and Biosciences, Office of Basic Energy Sciences
  2. U.S. Department of Energy [DE-AC36-08-GO28308]
  3. National Renewable Energy Laboratory
  4. University of Colorado
  5. Renewable and Sustainable Energy Institute (RASEI)

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We have developed complexes of CdS nanorods capped with 3-mercaptopropionic acid (MPA) and Clostridium acetobutylicum [FeFe]-hydrogenase I (CaI) that photocatalyze reduction of H+ to H-2 at a CaI turnover frequency of 380-900 s(-1) and photon conversion efficiencies of up to 20% under illumination at 405 nm. In this paper, we focus on the compositional and mechanistic aspects of CdS:CaI complexes that control the photochemical conversion of solar energy into H-2. Self-assembly of CdS with CaI was driven by electrostatics, demonstrated as the inhibition of ferredoxin-mediated H-2 evolution by CaI. Production of H-2 by CdS:CaI was observed only under illumination and only in the presence of a sacrificial donor. We explored the effects of the CdS:CaI molar ratio, sacrificial donor concentration, and light intensity on photocatalytic H-2 production, which were interpreted on the basis of contributions to electron transfer, hole transfer, or rate of photon absorption, respectively. Each parameter was found to have pronounced effects on the CdS:CaI photocatalytic activity. Specifically, we found that under 405 nm light at an intensity equivalent to total AM 1.5 solar flux, H-2 production was limited by the rate of photon absorption (similar to 1 ms(-1)) and not by the turnover of CaI. Complexes were capable of H-2 production for up to 4 h with a total turnover number of 106 before photocatalytic activity was lost. This loss correlated with inactivation of CaI, resulting from the photo-oxidation of the CdS capping ligand MPA.

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