Evidence against proton gradient formation being the cause of chlorophyll fluorescence quenching by methosulfate |
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Authors: | Rudolf E Slovacek Thomas T Bannister |
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Institution: | Department of Biology, University of Rochester, Rochester, N. Y. U.S.A. |
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Abstract: | In strong illumination, 3-(3,4-dichlorophenyl)-1, 1-dimethylurea (DCMU)-poisoned chloroplasts exhibit a high yield of chlorophyll fluorescence while turnover, proton uptake, and phosphorylation are inhibited and a pH gradient is undetectable. When 10 μM methosulfate (PMS) is included, the fluorescence yield in light is substantially reduced, and when 100 μM ascorbate is also included, the yield is diminished approximately to the level in darkness. Only very slight increases in turnover and proton uptake (but no detectable pH gradient) accompany the fluorescence yield decline.When 10 μM PMS and 15 mM ascorbate are added to poisoned chloroplasts (the oxygen concentration being greatly reduced), turnover, proton uptake, the pH gradient and phosphorylation all reach high levels. In this case, the yield of chlorophyll fluorescence is low and is the same in both light and dark. Further addition of an uncoupler eliminates proton uptake, the pH gradient and phosphorylation but does not significantly elevate the fluorescence yield. From these observations we suggest that, in DCMU-poisoned chloroplasts, the fluorescence quenching with PMS occurs by a mechanism unrelated to the generation of a phosphorylation potential.With chloroplasts unpoisoned by DCMU, PMS quenches fluorescence and considerably stimulates proton uptake, the pH gradient and phosphorylation. However, in this case, PMS serves to restore net electron transport. |
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Keywords: | CMU DCMU 3-(3 4-dichlorophenyl)-1 1-dimethylurea FCCP NADP NADPH nicotinamide adenine dinucleotide phosphate and it's reduced form PMS reaction center pigment for Photosystem I |
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