Superoxide dismutase: a photochemical augmentation assay. |
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Authors: | H P Misra I Fridovich |
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Affiliation: | Biological Adaptation Branch, Ames Research Center, National Aeronautics and Space Administration, Moffett Field, California 94035 U.S.A. |
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Abstract: | Cell envelope vesicles containing bacteriorhodopsin, prepared from Halobacterium halobium, have previously been shown to accumulate glutamate to high concentration gradients when illuminated. This active transport is energized by a sodium gradient (Naout+ ? Nain+), which arises from Na+-efflux coupled to the light-induced H+-gradient. The oxidation of dimethyl phenylenediamine (DPD) by the vesicles also can drive uphill glutamate transport, and such transport is inhibited by KCN, azide, ionophores, or uncouplers. KT for glutamate is 1.4 × 10?7m under these conditions, as compared to 1.3 × 10?7m for light-induced transport. The respiration-induced transport of glutamate is dependent on high Na+ concentrations on the vesicle exterior and requires low Na+ concentrations in the interior. When Na+ of increasing concentrations is included in the vesicles, transport proceeds with increasing lags, similarly to the case of light-driven transport. In vesicles to which DPD is added first, and then KCN at increasing time intervals (5 to 15 min), glutamate transport occurs after the addition of KCN, with increasing rates, even though respiration is inhibited. This indicates that the energy generated by DPD-oxidation is conserved over several minutes. These results suggest that in the case of respiration-dependent glutamate transport the translocation is also driven by a Na+-gradient; thus, there is a single glutamate transport system independent of the source of energy. The generation of such an Na+-gradient during DPD-oxidation implies that the respiration component involved, cytochrome oxidase, is functionally equivalent to bacteriorhodopsin, which acts as a proton pump. |
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Keywords: | To whom correspondence should be addressed. |
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