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Covalent modification of chloroplast Photosystem II polypeptides by p-nitrothiophenol
Authors:JE Mullet  CJ Arntzen  Y Kobayashi  Y Inoue
Institution:1. USDA/SEA/AR, Department of Botany, University of Illinois, Urbana, IL 61801 U.S.A.;2. RIKEN, The Institute of Physical and Chemical Research, Wako-shi, Saitama 351 Japan
Abstract:Illumination of the chlorophyll ab light-harvesting complex in the presence of p-nitrothio14C]phenol caused quenching of fluorescence emission at 685 nm (77 K) relative to 695 nm and covalent modification of light-harvesting complex polypeptides. Fluorescence quenching saturated with one p-nitrothiophenol bound per light-harvesting complex polypeptide (10–13 chlorophylls); 12 maximal quenching occurred with one p-nitrothiophenol bound per light-harvesting complex polypeptides (190–247 chlorophylls). This result provides direct evidence for excitation energy transfer between light-harvesting complex subunits which contain 4–6 polypeptides plus 40–78 chlorophylls per complex.Illumination of chloroplasts or Photosystem II (PS II) particles in the presence of p-nitrothio14C]phenol caused inhibition of PS II activity and labeling of several polypeptides including those of 42–48 kilodaltons previously identified as PS II reaction center polypeptides. In chloroplasts, inhibition of oxygen evolution accelerated p-nitrothiophenol modification reactions; DCMU or donors to PS II decreased p-nitrothiophenol modification. These results are consistent with the hypothesis that accumulation of oxidizing equivalents on the donor side of PS II creates a ‘reactive state’ in which polypeptides of PS II are susceptible to p-nitrothiophenol modification.
Keywords:Photosystem II  Fluorescence quenching  Protein modification  Light-harvesting complex  Reaction center  CCCP  carbonyl cyanide m-chlorophenylhydrazone  DCIP  2  6-dichlorophenolindophenol  DCMU  3-(3′  4′-dichlorophenyl)-1  1-dimethylurea  LHC  PS II  Photosystem II  Chl  chlorophyll  Tricine  To whom reprint requests should be addressed  
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