首页> 外文期刊>Biochemistry >Q-band ENDOR (electron nuclear double resonance) of the high-affinity ubisemiquinone center in cytochrome bo3 from Escherichia coli.
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Q-band ENDOR (electron nuclear double resonance) of the high-affinity ubisemiquinone center in cytochrome bo3 from Escherichia coli.

机译:大肠杆菌细胞色素bo3中高亲和力泛半醌中心的Q波段ENDOR(电子核双共振)。

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摘要

Electron nuclear double resonance (ENDOR) was performed on the protein-bound, stabilized, high-affinity ubisemiquinone radical, QH*-, of bo3 quinol oxidase to determine its electronic spin distribution and to probe its interaction with its surroundings. Until this present work, such ENDOR studies of protein-stabilized ubisemiquinone centers have only been done on photosynthetic reaction centers whose function is to reduce a ubiquinol pool. In contrast, QH*- serves to oxidize a ubiquinol pool in the course of electron transfer from the ubiquinol pool to the oxygen-consuming center of terminal bo3 oxidase. As documented by large hyperfine couplings (>10 MHz) to nonexchangeable protons on the QH*- ubisemiquinone ring, we provide evidence for an electronic distribution on QH*- that is different from that of the semiquinones of reaction centers. Since the ubisemiquinone itself is physically nearly identical in both QH*- and the bacterial photosynthetic reaction centers, this electronic difference is evidently a function of the local protein environment. Interaction of QH*- with this local protein environment was explicitly shown by exchangeable deuteron ENDOR that implied hydrogen bonding to the quinone and by weak proton hyperfine couplings to the local protein matrix.
机译:对bo3喹诺尔氧化酶的蛋白质结合的,稳定的,高亲和力的泛半醌基QH *-进行电子核双共振(ENDOR),以确定其电子自旋分布并探究其与周围环境的相互作用。在此工作之前,仅在光合反应中心上进行了蛋白质稳定的泛半醌中心的此类ENDOR研究,其功能是减少泛醌库。相反,QH *-在电子从泛醇池转移至末端bo3氧化酶的耗氧中心的过程中,用于氧化泛醇池。如与QH *-泛半醌环上不可交换质子的大型超精细偶联(> 10 MHz)所证明的,我们为QH *-上的电子分布提供了证据,该电子分布不同于反应中心的半醌。由于泛半醌本身在QH *-和细菌的光合作用反应中心几乎在物理上是相同的,因此这种电子差异显然是局部蛋白质环境的函数。可交换的氘核ENDOR(暗示氢键合到醌上)和质子超精细的弱耦合到局部蛋白基质上明确显示了QH *-与这种局部蛋白环境的相互作用。

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