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FURTHER IN VIVO STUDIES ON THE PARTICIPATION OF SINGLET OXYGEN IN THE PHOTODYNAMIC INACTIVATION AND INDUCTION OF GENETIC CHANGES IN SACCHAROMYCES CEREVISIAE
Authors:Katsumi  Kobayashi Takashi  Ito
Institution:Institute of Physics, College of General Education, University of Tokyo, Komaba, Meguroku, Tokyo 153, Japan
Abstract:Abstract —In vivo participation of singlet excited oxygen (1O2, 1Δ9) in the photodynamic inactivation and induction of genetic changes (gene conversion) in acridine orange-sensitized yeast cells was investigated by using N3-, an efficient 1O2 quencher, and D2O, a known agent for the enhancement of the lifetime of 1O2. The addition of N3- protected the cells from both photodynamic actions. From an analysis of the concentration-dependent protection, about 80% of the induction of the genetic change is explainable on the basis of 1O2 mechanism. The quantitative estimation of the N3- protection in the inactivation was not possible because of the sigmoidal nature of the inactivation curve. The replacement of H2O with D2O during illumination was effective in enhancing the photodynamic inactivation but almost completely ineffective for the gene conversion induction. The deuterium effect with the cell system was clearly not as large as would be expected from in vitro experiments. This, however, could be explained from the kinetic consideration that natural quenchers of lO2 in the cell would mask the deuterium effect. By experiments with different cell stages it was demonstrated that these two modifying effects were dependent on the intracellular reaction environment. The conclusion is that 1O2 must be the major intermediate responsible for the photodynamic actions in acridine orangesensitized yeast cells.
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