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一种在中子大分子晶体学中确定氘/氢对比度图谱的技术。

A technique for determining the deuterium/hydrogen contrast map in neutron macromolecular crystallography.

作者信息

Chatake Toshiyuki, Fujiwara Satoru

机构信息

Research Reactor Institute, Kyoto University, Asashironishi 2, Kumatori, Osaka, Japan.

Quantum Beam Science Center, Japan Atomic Energy Agency, 2-4 Shirakata-Shirane, Tokai, Naka, Ibaraki, Japan.

出版信息

Acta Crystallogr D Struct Biol. 2016 Jan;72(Pt 1):71-82. doi: 10.1107/S2059798315021269. Epub 2016 Jan 1.

DOI:10.1107/S2059798315021269
PMID:26894536
Abstract

A difference in the neutron scattering length between hydrogen and deuterium leads to a high density contrast in neutron Fourier maps. In this study, a technique for determining the deuterium/hydrogen (D/H) contrast map in neutron macromolecular crystallography is developed and evaluated using ribonuclease A. The contrast map between the D2O-solvent and H2O-solvent crystals is calculated in real space, rather than in reciprocal space as performed in previous neutron D/H contrast crystallography. The present technique can thus utilize all of the amplitudes of the neutron structure factors for both D2O-solvent and H2O-solvent crystals. The neutron D/H contrast maps clearly demonstrate the powerful detectability of H/D exchange in proteins. In fact, alternative protonation states and alternative conformations of hydroxyl groups are observed at medium resolution (1.8 Å). Moreover, water molecules can be categorized into three types according to their tendency towards rotational disorder. These results directly indicate improvement in the neutron crystal structure analysis. This technique is suitable for incorporation into the standard structure-determination process used in neutron protein crystallography; consequently, more precise and efficient determination of the D-atom positions is possible using a combination of this D/H contrast technique and standard neutron structure-determination protocols.

摘要

氢和氘之间中子散射长度的差异导致中子傅里叶图中具有高的密度对比度。在本研究中,开发了一种在中子大分子晶体学中确定氘/氢(D/H)对比度图的技术,并使用核糖核酸酶A进行了评估。D2O溶剂晶体和H2O溶剂晶体之间的对比度图是在实空间中计算的,而不是像以前的中子D/H对比度晶体学那样在倒易空间中计算。因此,本技术可以利用D2O溶剂晶体和H2O溶剂晶体的中子结构因子的所有振幅。中子D/H对比度图清楚地证明了蛋白质中H/D交换的强大可检测性。事实上,在中等分辨率(1.8 Å)下观察到了羟基的替代质子化状态和替代构象。此外,水分子可以根据其旋转无序的倾向分为三种类型。这些结果直接表明中子晶体结构分析得到了改进。该技术适用于纳入中子蛋白质晶体学中使用的标准结构测定过程;因此,结合这种D/H对比度技术和标准中子结构测定方案,可以更精确、高效地确定D原子的位置。

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