4.4 Article

Resonance Scattering Spectral Detection of Catalase Activity Using Au@Ag Nanoparticle as Probe and Coupling Catalase Catalytic Reaction with Fenton Reaction

Journal

JOURNAL OF FLUORESCENCE
Volume 19, Issue 6, Pages 1009-1015

Publisher

SPRINGER/PLENUM PUBLISHERS
DOI: 10.1007/s10895-009-0500-0

Keywords

Catalase; Au@Ag nanoprobe; Hydroxyl radical; Resonance scattering spectral assay

Funding

  1. National Natural Science Foundation of China [20667001, 20865002]
  2. Natural Science Foundation of Guangxi [0832260]
  3. Research Funds of Guangxi Key Laboratory of Environmental Engineering, Protection and Assessment [0701Z022, 0701k008]

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The Au(core)Ag(shell) (Au@Ag) nanoparticles in size of 30 nm were prepared using 10 nm gold nanoparticles as seeds at 90A degrees C, and were purified by high-speed centrifugation to remove the excess trisodium citrate to obtain Au@Ag nanoprobe. In the medium of pH 4.0 acetate buffer solution-7.2 mu mol/L H(2)O(2)-67 mu mol/L Fe(II), Au@Ag nanoparticles exhibited a resonance scattering (RS) peak at 538 nm. Upon addition of Catalase (Ct), the system produced hydroxyl radical that oxidized the Au@Ag nanoprobe to form the AuAg nanoparticles with partly bare nanogold. Those AuAg nanoparticles aggregated to large nanoclusters that led to the RS peak wavelength red-shift and its RS peak intensity enhanced. The catalase activity (C) is linear to the enhanced RS intensity (Delta I) in the range of 6 to 2,800 U/L, with regression equation of Delta I = 0.168 C-0.2, the correlation coefficient of 0.9952, and detection limit of 2.8 U/L. This method was applied to the detection of serum samples, and the results were agreement with that of the spectrophotometry. A new catalytic mechanism of catalase was proposed with oxywater principle that was agreement with the results of resonance scattering spectroscopy, absorption spectrophotometry, transmission electron microscopy and laser scattering.

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