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细胞色素c氧化酶中质子通道结构与水配位的可塑性

Plasticity of proton pathway structure and water coordination in cytochrome c oxidase.

作者信息

Namslauer Andreas, Lepp Håkan, Brändén Magnus, Jasaitis Audrius, Verkhovsky Michael I, Brzezinski Peter

机构信息

Department of Biochemistry and Biophysics, The Arrhenius Laboratories for Natural Sciences, Stockholm University, SE-106 91 Stockholm, Sweden.

出版信息

J Biol Chem. 2007 May 18;282(20):15148-58. doi: 10.1074/jbc.M700348200. Epub 2007 Mar 15.

DOI:10.1074/jbc.M700348200
PMID:17363369
Abstract

Cytochrome c oxidase (CytcO) is a redox-driven, membrane-bound proton pump. One of the proton transfer pathways of the enzyme, the D pathway, used for the transfer of both substrate and pumped protons, accommodates a network of hydrogen-bonded water molecules that span the distance between an aspartate (Asp(132)), near the protein surface, and glutamate Glu(286), which is an internal proton donor to the catalytic site. To investigate how changes in the environment around Glu(286) affect the mechanism of proton transfer through the pathway, we introduced a non-hydrogen-bonding (Ala) or an acidic residue (Asp) at position Ser(197) (S197A or S197D), located approximately 7 A from Glu(286). Although Ser(197) is hydrogen-bonded to a water molecule that is part of the D pathway "proton wire," replacement of the Ser by an Ala did not affect the proton transfer rate. In contrast, the S197D mutant CytcO displayed a turnover activity of approximately 35% of that of the wild-type CytcO, and the O(2) reduction reaction was not linked to proton pumping. Instead, a fraction of the substrate protons was taken from the positive ("incorrect") side of the membrane. Furthermore, the pH dependence of the proton transfer rate was altered in the mutant CytcO. The results indicate that there is plasticity in the water coordination of the proton pathway, but alteration of the electrostatic potential within the pathway results in uncoupling of the proton translocation machinery.

摘要

细胞色素c氧化酶(CytcO)是一种由氧化还原驱动的膜结合质子泵。该酶的质子转移途径之一,即D途径,用于底物和泵出质子的转移,容纳了一个由氢键连接的水分子网络,这些水分子跨越了靠近蛋白质表面的天冬氨酸(Asp(132))和谷氨酸(Glu(286))之间的距离,谷氨酸是催化位点的内部质子供体。为了研究Glu(286)周围环境的变化如何影响通过该途径的质子转移机制,我们在距离Glu(286)约7埃的Ser(197)位置引入了一个非氢键结合(丙氨酸)或酸性残基(天冬氨酸)(S197A或S197D)。尽管Ser(197)通过氢键与作为D途径“质子线”一部分的水分子相连,但用丙氨酸取代丝氨酸并不影响质子转移速率。相反,S197D突变体CytcO的周转活性约为野生型CytcO的35%,并且O(2)还原反应与质子泵浦不相关。取而代之的是,一部分底物质子从膜的正(“错误”)侧获取。此外,突变体CytcO中质子转移速率的pH依赖性发生了改变。结果表明,质子途径的水配位具有可塑性,但途径内静电势的改变导致质子转运机制解偶联。

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