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本文引用的文献

1
The F -ATPase from Trypanosoma brucei is elaborated by three copies of an additional p18-subunit.布氏锥虫的 F-ATP 酶由三个额外的 p18 亚基组成。
FEBS J. 2018 Feb;285(3):614-628. doi: 10.1111/febs.14364. Epub 2017 Dec 30.
2
Trypanosoma brucei TbIF1 inhibits the essential F1-ATPase in the infectious form of the parasite.布氏锥虫TbIF1抑制该寄生虫感染形式下的关键F1-ATP酶。
PLoS Negl Trop Dis. 2017 Apr 17;11(4):e0005552. doi: 10.1371/journal.pntd.0005552. eCollection 2017 Apr.
3
In situ structure of trypanosomal ATP synthase dimer reveals a unique arrangement of catalytic subunits.原生质体锥虫 ATP 合酶二聚体的结构揭示了催化亚基的独特排列。
Proc Natl Acad Sci U S A. 2017 Jan 31;114(5):992-997. doi: 10.1073/pnas.1612386114. Epub 2017 Jan 17.
4
Atypical composition and structure of the mitochondrial dimeric ATP synthase from Euglena gracilis.眼虫 Euglena gracilis 线粒体二聚体 ATP 合酶的非典型组成和结构。
Biochim Biophys Acta Bioenerg. 2017 Apr;1858(4):267-275. doi: 10.1016/j.bbabio.2017.01.007. Epub 2017 Jan 12.
5
Cryo-EM structures of the autoinhibited ATP synthase in three rotational states.处于三种旋转状态的自抑制ATP合酶的冷冻电镜结构。
Elife. 2016 Dec 21;5:e21598. doi: 10.7554/eLife.21598.
6
Structure of the mitochondrial ATP synthase from determined by electron cryo-microscopy.通过电子冷冻显微镜确定的来自[具体来源]的线粒体ATP合酶的结构。 (你提供的原文中“from”后面缺少具体信息)
Proc Natl Acad Sci U S A. 2016 Nov 8;113(45):12709-12714. doi: 10.1073/pnas.1615902113. Epub 2016 Oct 24.
7
Regulation of the thermoalkaliphilic F1-ATPase from Caldalkalibacillus thermarum.嗜热嗜碱栖热芽孢杆菌中嗜热嗜碱F1-ATP酶的调控
Proc Natl Acad Sci U S A. 2016 Sep 27;113(39):10860-5. doi: 10.1073/pnas.1612035113. Epub 2016 Sep 12.
8
Structure of a Complete ATP Synthase Dimer Reveals the Molecular Basis of Inner Mitochondrial Membrane Morphology.完整ATP合酶二聚体的结构揭示了线粒体内膜形态的分子基础。
Mol Cell. 2016 Aug 4;63(3):445-56. doi: 10.1016/j.molcel.2016.05.037. Epub 2016 Jun 30.
9
The MPI bioinformatics Toolkit as an integrative platform for advanced protein sequence and structure analysis.MPI生物信息学工具包作为用于高级蛋白质序列和结构分析的综合平台。
Nucleic Acids Res. 2016 Jul 8;44(W1):W410-5. doi: 10.1093/nar/gkw348. Epub 2016 Apr 29.
10
MASSIF-1: a beamline dedicated to the fully automatic characterization and data collection from crystals of biological macromolecules.MASSIF-1:一条专门用于对生物大分子晶体进行全自动表征和数据收集的光束线。
J Synchrotron Radiat. 2015 Nov;22(6):1540-7. doi: 10.1107/S1600577515016604. Epub 2015 Oct 3.

来自 的 ATP 合酶具有复杂的经典 F 结构域和常规催化位点。

ATP synthase from has an elaborated canonical F-domain and conventional catalytic sites.

机构信息

The Medical Research Council Mitochondrial Biology Unit, University of Cambridge, Cambridge CB2 0XY, United Kingdom.

Institute of Parasitology, Biology Centre, Czech Academy of Sciences, 37005 České Budějovice, Czech Republic.

出版信息

Proc Natl Acad Sci U S A. 2018 Feb 27;115(9):2102-2107. doi: 10.1073/pnas.1720940115. Epub 2018 Feb 12.

DOI:10.1073/pnas.1720940115
PMID:29440423
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5834723/
Abstract

The structures and functions of the components of ATP synthases, especially those subunits involved directly in the catalytic formation of ATP, are widely conserved in metazoans, fungi, eubacteria, and plant chloroplasts. On the basis of a map at 32.5-Å resolution determined in situ in the mitochondria of by electron cryotomography, it has been proposed that the ATP synthase in this species has a noncanonical structure and different catalytic sites in which the catalytically essential arginine finger is provided not by the α-subunit adjacent to the catalytic nucleotide-binding site as in all species investigated to date, but rather by a protein, p18, found only in the euglenozoa. A crystal structure at 3.2-Å resolution of the catalytic domain of the same enzyme demonstrates that this proposal is incorrect. In many respects, the structure is similar to the structures of F-ATPases determined previously. The αβ-spherical portion of the catalytic domain in which the three catalytic sites are found, plus the central stalk, are highly conserved, and the arginine finger is provided conventionally by the α-subunits adjacent to each of the three catalytic sites found in the β-subunits. Thus, the enzyme has a conventional catalytic mechanism. The structure differs from previous described structures by the presence of a p18 subunit, identified only in the euglenozoa, associated with the external surface of each of the three α-subunits, thereby elaborating the F-domain. Subunit p18 is a pentatricopeptide repeat (PPR) protein with three PPRs and appears to have no function in the catalytic mechanism of the enzyme.

摘要

ATP 合酶各组件的结构和功能在后生动物、真菌、真细菌和植物叶绿体中广泛保守,特别是那些直接参与 ATP 催化形成的亚基。根据电镜 cryotomography 在 线粒体中以 32.5-Å 分辨率确定的图谱,该物种中的 ATP 合酶具有非典型结构和不同的催化位点,其中催化必需的精氨酸指由不是所有迄今为止研究过的物种中紧邻催化核苷酸结合位点的 α 亚基提供,而是由一种仅在 Euglenozoa 中发现的蛋白质 p18 提供。相同酶的催化结构域的 3.2-Å 分辨率晶体结构表明,该提议是不正确的。在许多方面,该结构与之前确定的 F-ATPases 结构相似。在其中发现三个催化位点的催化结构域的 αβ-球形部分,加上中央茎,高度保守,并且精氨酸指由每个β亚基中的三个催化位点附近的 α 亚基常规提供。因此,该酶具有常规的催化机制。该结构与以前描述的结构不同,存在一个仅在 Euglenozoa 中发现的 p18 亚基,与三个 α 亚基的每个外部表面相关联,从而详细阐述了 F 结构域。亚基 p18 是一个五肽重复(PPR)蛋白,具有三个 PPR ,并且似乎在酶的催化机制中没有功能。