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Photoinactivation of photosystem II complexes and photoprotection by non-functional neighbours in Capsicum annuum L. leaves

机译:辣椒辣椒叶片中非功能性邻居对光系统II复合物的光灭活和光保护

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Leaf segments from Capsicum annuum plants grown at 100 μmol photons m−2 s−1 (low light) or 500 μmol photons m−2 s−1 (high light) were illuminated at three irradiances and three temperatures for several hours. At various times, the remaining fraction (f) of functional photosystem II (PS II) complexes was measured by a chlorophyll fluorescence parameter (1/F o − 1/F m , where F o and F m are the fluorescence yields corresponding to open and closed PS II traps, respectively), which was in turn calibrated by the oxygen yield per saturating single-turnover flash. During illumination of leaf segments in the presence of lincomycin, an inhibitor of chloroplast-encoded protein synthesis, the decline of f from 1.0 to about 0.3 was mono-exponential. Thereafter, f declined much more slowly, the remaining fraction (≈0.2) being able to survive prolonged illumination. The results can be interpreted as being in support of the hypothesis that photoinactivated PS II complexes photoprotect functional neighbours (G. Öquist et al. 1992, Planta 186: 450–460), provided it is assumed that a photoinactivated PS II is initially only a weak quencher of excitation energy, but becomes a much stronger quencher during prolonged illumination when a substantial fraction of PS II complexes has also been photoinactivated. In the absence of lincomycin, photoinactivation and repair of PS II occur in parallel, allowing f to reach a steady-state value that is determined by the treatment irradiance, temperature and growth irradiance. The results obtained in the presence and absence of lincomycin are analysed according to a simple kinetic model which formally incorporates a conversion from weak to strong quenchers, yielding the rate coefficients of photoinactivation and of repair for various conditions, as well as gaining an insight into the influence of f on the rate coefficient of photoinactivation. They demonstrate that the method is a convenient alternative to the use of radiolabelled amino acids for quantifying photoinactivation and repair of PS II in leaves.
机译:在100μmol光子m-2 s-1 (弱光)或500μmol光子m-2 s-1 (强光)下生长的辣椒植物叶片)在三个辐照度和三个温度下照明了几个小时。在不同时间,通过叶绿素荧光参数(1 / F o − 1 / F m ,其中F o 和F m 分别是分别对应于打开和关闭的PS II陷阱的荧光产量),然后通过每个饱和单周转闪光灯的氧气产量对其进行校准。在林可霉素(叶绿体编码的蛋白合成的抑制剂)存在下照亮叶段期间,f从1.0下降到约0.3是单指数的。此后,f下降的速度要慢得多,剩余的分数(≈0.2)能够经受长时间的照明。该结果可以解释为支持以下假设:光灭活的PS II复合物可以保护功能邻域(G.Öquist等人,1992,Planta 186:450-460),前提是假设光灭活的PS II最初只是一个弱的激发能猝灭剂,但当大部分PS II配合物也被光灭活时,在长时间照明过程中会变得更强。在不存在林可霉素的情况下,PS II的光灭活和修复同时发生,从而使f达到由治疗辐照度,温度和生长辐照度决定的稳态值。根据一个简单的动力学模型分析在存在和不存在林可霉素的情况下获得的结果,该动力学模型正式纳入了从弱淬灭剂到强淬灭剂的转化,产生了光灭活和各种条件下修复的速率系数,并深入了解了f对光灭活速率系数的影响。他们证明,该方法是使用放射性标记的氨基酸定量叶片中PS II的光灭活和修复的便捷替代方法。

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