CHARACTERIZATION OF THE LIGHT-INDUCED CROSS-LINKING OF THE ALPHA-SUBUNIT OF CYTOCHROME B(559) AND THE D1 PROTEIN IN ISOLATED PHOTOSYSTEM-II REACTION CENTERS
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BARBATO, R
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UNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLANDUNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLAND
BARBATO, R
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FRISO, G
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UNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLANDUNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLAND
FRISO, G
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PONTICOS, M
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UNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLANDUNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLAND
PONTICOS, M
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BARBER, J
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UNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLANDUNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLAND
BARBER, J
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[1] UNIV LONDON IMPERIAL COLL SCI TECHNOL & MED,WOLFSON LABS,DEPT BIOCHEM,PHOTOSYNTH RES GRP,LONDON SW7 2AY,ENGLAND
Illumination of the isolated reaction center of photosystem II generates a protein of 41 kDa molecular mass, Using immunoblotting, it is confirmed that the protein is an adduct of the D1 protein and the a-subunit of cytochrome b(559). Its formation seems to be photochemically induced, being independent of temperature between 4 and 20 degrees C and unaffected by a mixture of protease inhibitors. The maximum levels are detected when the pH is in the region 6.5-8.5 and when illumination intensities are moderate. Although higher light intensities induce a higher rate of formation, the accumulation of elevated levels of the 41-kDa protein does not occur due to light-induced degradation. This degradation is also unaffected by the presence of protease inhibitors, Proteolytic mapping and N-terminal sequencing indicates that the cross-linking process involves the N-terminal serine of the alpha-subunit of cytochrome b(599) and D1 residues in the 239-244 FGQEEE motif close to the Q(B) binding site. In conclusion, the results indicate that the N terminus of the cu-subunit is exposed on the stromal side of photosystem II in such a way as to undergo light-induced cross-linking in the Q(B) region of the D1 protein. They also suggest that the 41-kDa adduct may be an intermediate before the light-induced cleavage of the D1 protein in the FGQEEE region.
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UNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDENUNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDEN
BARBER, J
ANDERSSON, B
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UNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDENUNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDEN
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UNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDENUNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDEN
BARBER, J
ANDERSSON, B
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UNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDENUNIV STOCKHOLM, DEPT BIOCHEM, ARRHENIUS LABS NAT SCI, S-10691 STOCKHOLM, SWEDEN