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关于细菌F型ATP合酶ε亚基的ATP结合位点。

On the ATP binding site of the ε subunit from bacterial F-type ATP synthases.

作者信息

Krah Alexander, Takada Shoji

机构信息

Department of Biophysics, Graduate School of Science, Kyoto University, Kitashirakawa-Oiwakecho, Sakyo-ku, Kyoto, 606-8502, Japan.

Department of Biophysics, Graduate School of Science, Kyoto University, Kitashirakawa-Oiwakecho, Sakyo-ku, Kyoto, 606-8502, Japan.

出版信息

Biochim Biophys Acta. 2016 Apr;1857(4):332-40. doi: 10.1016/j.bbabio.2016.01.007. Epub 2016 Jan 15.

DOI:10.1016/j.bbabio.2016.01.007
PMID:26780667
Abstract

F-type ATP synthases are reversible machinery that not only synthesize adenosine triphosphate (ATP) using an electrochemical gradient across the membrane, but also can hydrolyze ATP to pump ions under certain conditions. To prevent wasteful ATP hydrolysis, subunit ε in bacterial ATP synthases changes its conformation from the non-inhibitory down- to the inhibitory up-state at a low cellular ATP concentration. Recently, a crystal structure of the ε subunit in complex with ATP was solved in a non-biologically relevant dimeric form. Here, to derive the functional ATP binding site motif, we carried out molecular dynamics simulations and free energy calculations. Our results suggest that the ATP binding site markedly differs from the experimental resolved one; we observe a reorientation of several residues, which bind to ATP in the crystal structure. In addition we find that an Mg(2+) ion is coordinated by ATP, replacing interactions of the second chain in the crystal structure. Thus we demonstrate more generally the influence of crystallization effects on ligand binding sites and their respective binding modes. Furthermore, we propose a role for two highly conserved residues to control the ATP binding/unbinding event, which have not been considered before. Additionally our results provide the basis for the rational development of new biosensors based on subunit ε, as shown previously for novel sensors measuring the ATP concentration in cells.

摘要

F型ATP合酶是一种可逆的机制,它不仅能利用跨膜电化学梯度合成三磷酸腺苷(ATP),而且在某些条件下还能水解ATP以泵送离子。为防止ATP的浪费性水解,细菌ATP合酶中的ε亚基在细胞内ATP浓度较低时,会将其构象从非抑制性的向下状态转变为抑制性的向上状态。最近,ε亚基与ATP复合物的晶体结构以一种与生物学无关的二聚体形式得到了解析。在此,为了推导功能性ATP结合位点基序,我们进行了分子动力学模拟和自由能计算。我们的结果表明,ATP结合位点与实验解析的位点明显不同;我们观察到几个在晶体结构中与ATP结合的残基发生了重新定向。此外,我们发现一个Mg(2+)离子与ATP配位,取代了晶体结构中第二条链的相互作用。因此,我们更普遍地证明了结晶效应对配体结合位点及其各自结合模式的影响。此外,我们提出了两个高度保守的残基在控制ATP结合/解离事件中的作用,这在以前从未被考虑过。另外,我们的结果为基于ε亚基的新型生物传感器的合理开发提供了基础,如之前用于测量细胞内ATP浓度的新型传感器所示。

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