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Kinetics of prolonged photoinhibition revisited: photoinhibited Photosystem II centres do not protect the active ones against loss of oxygen evolution

机译:重新讨论了长时间光抑制的动力学:光抑制的Photosystem II中心不能保护活性中心免受氧气释放的损害

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Photoinhibition of Photosystem II (PSII) in lincomycin-treated leaves begins as a first-order reaction, but fluorescence measurements have suggested that after prolonged illumination, the number of active PSII centres stabilizes to 15-20% of control. The stabilization has been interpreted to indicate that photoinhibited PSII centres protect the remaining active centres against photoinhibition (Lee, Hong and Chow, Planta 212:332-342, 2001). In an attempt to study the mechanism of this protection, we measured the reaction kinetics of photoinhibition in lincomycin-treated pumpkin (Cucurbita pepo L.) and pepper (Capsicum annuum L.) leaves in vivo. The light-saturated rate of PSII oxygen evolution, assayed from thylakoids and isolated from the treated leaves, was used as a direct measure of the number of remaining active PSII centres, and the fluorescence parameters F (V)/F (M) and (F (V)/F (M))/F (0) (=1/F (0) - 1/F (M)) were measured for comparison. To our surprise, no stabilization of PSII activity was observed and photoinhibition followed first-order kinetics until PSII activity had virtually declined to zero. A series of in vitro experiments was carried out to see whether stabilization of PSII activity occurs if a particular combination of light intensity and wavelength range is applied, or if a specific PSII preparation is used as experimental material. The results of the in vitro experiments confirmed the in vivo result about persistent first-order kinetics. We conclude that photoinhibited PSII centres offer no measurable protection against photoinhibition.
机译:林可霉素处理的叶片中光系统II(PSII)的光抑制作用是作为一级反应而开始的,但是荧光测量表明,长时间照射后,活性PSII中心的数量稳定在对照的15-20%。该稳定作用已被解释为表明光抑制的PSII中心保护其余的活性中心免受光抑制(Lee,Hong和Chow,Planta 212:332-342,2001)。为了研究这种保护的机理,我们测量了林可霉素处理的南瓜(Cucurbita pepo L.)和胡椒(Capsicum annuum L.)叶片在体内的光抑制反应动力学。从类囊体测定并从处理过的叶片中分离出来的PSII氧气放出的光饱和速率用作直接测量剩余的活性PSII中心数量以及荧光参数F(V)/ F(M)和(测量F(V)/ F(M))/ F(0)(= 1 / F(0)-1 / F(M))进行比较。令我们惊讶的是,未观察到PSII活性的稳定,并且光抑制遵循一阶动力学,直到PSII活性几乎降至零为止。进行了一系列的体外实验,以观察如果应用光强度和波长范围的特定组合,或者如果使用特定的PSII制剂作为实验材料,是否会稳定PSII活性。体外实验的结果证实了关于持久性一级动力学的体内结果。我们得出的结论是,光抑制的PSII中心无法提供对光抑制的可测量保护。

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