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The EPR signals from the S0 and S2 states of the Mn cluster in photosystem II relax differently.

机译:来自光系统II中Mn簇的S0和S2状态的EPR信号有不同的弛豫。

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The oxygen evolving complex (OEC) of photosystem II (PSII) gives rise to manganese-derived electron paramagnetic resonance (EPR) signals in the S0 and S2 oxidation states. These signals exhibit different microwave power saturation behavior between 4 and 10 K. Below 8 K, the S0 state EPR signal is a faster relaxer than the S2 multiline signal, but above 8 K, the S0 signal is the slower relaxer of the two. The different temperature dependencies of the relaxation of the S0 and S2 ground-state Mn signals are due to differences in the spin-lattice relaxation process. The dominating spin-lattice relaxation mechanism is concluded to be a Raman mechanism in the S0 state, with a T(4.1) temperature dependence of the relaxation rate. It is proposed that the relaxation of the S2 state arises from a Raman mechanism as well, with a T(6.8) temperature dependence of the relaxation rate, although the data also fit an Orbach process. If both signals relax through a Raman mechanism, the different exponents are proposed to reflect structural differences in the proteins surrounding the Mn cluster between the S0 and S2 states. The saturation of SII(slow) from the Y(D)(ox) radical on the D2 protein was also studied, and found to vary between the S0 and the S2 states of the enzyme in a manner similar to the EPR signals from the OEC. Furthermore, we found that the S2 multiline signal in the second turnover of the enzyme is significantly more difficult to saturate than in the first turnover. This suggests differences in the OEC between the first and second cycles of the enzyme. The increased relaxation rate may be caused by the appearance of a relaxation enhancer, or it may be due to subtle structural changes as the OEC is brought into an active state.
机译:光系统II(PSII)的析氧复合物(OEC)产生处于S0和S2氧化态的锰衍生的电子顺磁共振(EPR)信号。这些信号在4至10 K之间表现出不同的微波功率饱和特性。低于8 K时,S0状态EPR信号比S2多线信号具有更快的松弛度,但高于8 K时,S0状态则是两者中较慢的松弛度。 S0和S2基态Mn信号弛豫的不同温度相关性是由于自旋晶格弛豫过程的不同引起的。主要的自旋晶格弛豫机制被认为是S0状态下的拉曼机制,其弛豫速率与T(4.1)有关。有人提出,S2态的弛豫也是由拉曼机理引起的,弛豫速率与温度成T(6.8)依赖关系,尽管数据也适合于Orbach过程。如果两个信号都通过拉曼机制放松,则提出了不同的指数来反映S0和S2状态之间Mn簇周围蛋白质的结构差异。还研究了D2蛋白上Y(D)(ox)自由基引起的SII(慢)的饱和度,发现该酶的S0和S2状态之间的饱和度与OEC的EPR信号相似。此外,我们发现酶的第二次转换中的S2多系信号比第一次转换中的饱和信号明显更难饱和。这表明酶的第一和第二循环之间的OEC不同。增加的弛豫速率可能是由于弛豫增强剂的出现引起的,或者可能是由于OEC进入活性状态时发生的细微结构变化。

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