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Subunit Movements in Single Membrane-bound H+-ATP Synthases from Chloroplasts during ATP Synthesis

机译:叶绿体在ATP合成过程中单个膜结合的H + -ATP合成酶中的亚基运动

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摘要

Subunit movements within the H+-ATP synthase from chloroplasts (CF0F1) are investigated during ATP synthesis. The γ-subunit (γCys-322) is covalently labeled with a fluorescence donor (ATTO532). A fluorescence acceptor (adenosine 5′-(β,γ-imino)triphosphate (AMPPNP)-ATTO665) is noncovalently bound to a noncatalytic site at one α-subunit. The labeled CF0F1 is integrated into liposomes, and a transmembrane pH difference is generated by an acid base transition. Single-pair fluorescence resonance energy transfer is measured in freely diffusing proteoliposomes with a confocal two-channel microscope. The fluorescence time traces reveal a repetitive three-step rotation of the γ-subunit relative to the α-subunit during ATP synthesis. Some traces show splitting into sublevels with fluctuations between the sublevels. During catalysis the central stalk interacts, with equal probability, with each αβ-pair. Without catalysis the central stalk interacts with only one specific αβ-pair, and no stepping between FRET levels is observed. Two inactive states of the enzyme are identified: one in the presence of AMPPNP and one in the presence of ADP.
机译:在ATP合成过程中研究了来自叶绿体(CF0F1)的H + -ATP合酶内的亚基运动。 γ亚基(γCys-322)用荧光供体(ATTO532)共价标记。荧光受体(腺苷5'-(β,γ-亚氨基)三磷酸(AMPPNP)-ATTO665)非共价结合至一个α-亚基的非催化位点。标记的CF0F1被整合到脂质体中,而跨膜的pH差异是通过酸碱转变产生的。使用共聚焦两通道显微镜在自由扩散的蛋白脂质体中测量单对荧光共振能量转移。荧光时间迹线揭示了在ATP合成过程中,γ亚基相对于α亚基的重复三步旋转。一些迹线显示分裂为多个子级别,各子级别之间存在波动。在催化过程中,中央茎与每个αβ对以相等的概率相互作用。在没有催化的情况下,中心茎仅与一个特定的αβ对相互作用,并且未观察到FRET水平之间的步进。确定了该酶的两种失活状态:一种在AMPPNP存在下,一种在ADP存在下。

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