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Simultaneous monitoring of the two coupled motors of a single F_oF_1-ATP synthase by three-color FRET using duty cycle-optimized triple-ALEX

机译:使用占空比优化的三重ALEX通过三色FRET同时监视单个F_oF_1-ATP合酶的两个耦合电机

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F_oF_1-ATP synthase is the enzyme that provides the 'chemical energy currency' adenosine triphosphate, ATP, for living cells. The formation of ATP is accomplished by a stepwise internal rotation of subunits within the enzyme. Briefly, proton translocation through the membrane-bound F_o part of ATP synthase drives a 10-step rotary motion of the ring of c subunits with respect to the non-rotating subunits a and b. This rotation is transmitted to the y and e subunits of the F_1 sector resulting in 120° steps. In order to unravel this symmetry mismatch we monitor subunit rotation by a single-molecule fluorescence resonance energy transfer (FRET) approach using three fluorophores specifically attached to the enzyme: one attached to the F_1 motor, another one to the F_o motor, and the third one to a non-rotating subunit. To reduce photophysical artifacts due to spectral fluctuations of the single fluorophores, a duty cycle-optimized alternating three-laser scheme (DCO-ALEX) has been developed. Simultaneous observation of the stepsizes for both motors allows the detection of reversible elastic deformations between the rotor parts of F_o and F_1.
机译:F_oF_1-ATP合酶是为活细胞提供“化学能通量”三磷酸腺苷ATP的酶。 ATP的形成通过酶中亚基的逐步内部旋转来完成。简而言之,质子通过ATP合酶的膜结合的F_o部分的易位驱动c个亚基环相对于非旋转亚基a和b的10步旋转运动。该旋转被传输到F_1扇区的y和e子单元,从而产生120°阶跃。为了解决这种对称性不匹配问题,我们使用单分子荧光共振能量转移(FRET)方法,通过使用三种特定附着于酶的荧光团来监测亚基旋转:一个附着于F_1马达,另一个附着于F_o马达,第三个附着于F_o马达。一个到一个非旋转的子单元。为了减少由于单个荧光团的光谱波动而引起的光物理伪影,已开发了占空比优化的交替三激光方案(DCO-ALEX)。同时观察两个电机的步距可以检测F_o和F_1的转子部件之间的可逆弹性变形。

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