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F1F0-ATP合酶与ADP/ATP转位酶的二维扩散。对线粒体内膜中ATP合成假说的验证。

Two-dimensional diffusion of F1F0-ATP synthase and ADP/ATP translocator. Testing a hypothesis for ATP synthesis in the mitochondrial inner membrane.

作者信息

Gupte S S, Chazotte B, Leesnitzer M A, Hackenbrock C R

机构信息

Department of Cell Biology and Anatomy, University of North Carolina School of Medicine, Chapel Hill 27599-7090.

出版信息

Biochim Biophys Acta. 1991 Nov 4;1069(2):131-8. doi: 10.1016/0005-2736(91)90114-n.

Abstract

We report here the first experimentally determined lateral diffusion coefficients of the F1F0-ATP synthase and the ADP/ATP translocator in isolated inner membranes of rat liver mitochondria. Rabbit IgG developed against the F1F0-ATP synthase isolated from rat liver mitochondria was determined to be immunospecific for the synthase subunits, notably the alpha-beta doublet, gamma and delta subunits of F1 and subunits two, three and four of F0. This IgG, conjugated with lissamine-rhodamine, was used as a fluorescent probe to monitor the diffusion of the synthase in the membrane. IgG to cytochrome bc1 complex, prepared and labeled similarly, was used as a fluorescent probe for diffusion of this redox component. Eosin maleimide was determined to specifically label the ADP/ATP translocator in the isolated inner membrane and was used as a specific probe for the diffusion of the translocator. Using fluorescence recovery after photobleaching, the experimental average lateral diffusion coefficient of the F1F0-ATP synthase was determined to be 8.4 x 10(-10) cm2/s or twice that of cytochrome bc1 complex while the diffusion coefficient of the ADP/ATP translocator was 1.7 x 10(-9) cm2/s or four times that of cytochrome bc1 complex suggesting that all three components are independent two-dimensional diffusants. Using these diffusion coefficients and applying a number of basic assumptions, we calculated the theoretical two-dimensional diffusion-controlled collision frequencies and derived collision efficiencies (protons transferred per collision) between each of the three proton-transferring redox complexes and both the F1F0-ATP synthase and ADP/ATP translocator by treating the redox components as proton donors and the synthase and translocator as proton acceptors. These collision efficiencies support the physical possibility of a diffusion-based, random collision process of proton transfer and ATP synthesis in the mitochondrial inner membrane.

摘要

我们在此报告首次通过实验测定大鼠肝线粒体分离内膜中F1F0 - ATP合酶和ADP/ATP转位酶的横向扩散系数。已确定针对从大鼠肝线粒体分离的F1F0 - ATP合酶产生的兔IgG对合酶亚基具有免疫特异性,特别是F1的α - β二聚体、γ和δ亚基以及F0的亚基二、三、四。这种与丽丝胺罗丹明偶联的IgG用作荧光探针,以监测合酶在膜中的扩散。以类似方式制备和标记的细胞色素bc1复合物的IgG用作该氧化还原成分扩散的荧光探针。已确定马来酰亚胺曙红可特异性标记分离内膜中的ADP/ATP转位酶,并用作转位酶扩散的特异性探针。通过光漂白后荧光恢复,测定F1F0 - ATP合酶的实验平均横向扩散系数为8.4×10(-10) cm2/s,是细胞色素bc1复合物的两倍,而ADP/ATP转位酶的扩散系数为1.7×10(-9) cm2/s,是细胞色素bc1复合物的四倍,这表明所有这三种成分都是独立的二维扩散体。利用这些扩散系数并应用一些基本假设,我们计算了理论二维扩散控制的碰撞频率,并通过将氧化还原成分视为质子供体,将合酶和转位酶视为质子受体,得出了三种质子转移氧化还原复合物与F¡F0 - ATP合酶和ADP/ATP转位酶之间的碰撞效率(每次碰撞转移的质子)。这些碰撞效率支持了线粒体内膜中基于扩散的质子转移和ATP合成随机碰撞过程的物理可能性。

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