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构象交换在膜转运蛋白中在蛋白质晶体中发生改变。

Conformational exchange in a membrane transport protein is altered in protein crystals.

机构信息

Departments of Chemistry, University of Virginia, Charlottesville, Virginia, USA.

出版信息

Biophys J. 2010 Sep 8;99(5):1604-10. doi: 10.1016/j.bpj.2010.06.026.

Abstract

Successful macromolecular crystallography requires solution conditions that may alter the conformational sampling of a macromolecule. Here, site-directed spin labeling is used to examine a conformational equilibrium within BtuB, the Escherichia coli outer membrane transporter for vitamin B(12). Electron paramagnetic resonance (EPR) spectra from a spin label placed within the N-terminal energy coupling motif (Ton box) of BtuB indicate that this segment is in equilibrium between folded and unfolded forms. In bilayers, substrate binding shifts this equilibrium toward the unfolded form; however, EPR spectra from this same spin-labeled mutant indicate that this unfolding transition is blocked in protein crystals. Moreover, crystal structures of this spin-labeled mutant are consistent with the EPR result. When the free energy difference between substates is estimated from the EPR spectra, the crystal environment is found to alter this energy by 3 kcal/mol when compared to the bilayer state. Approximately half of this energy change is due to solutes or osmolytes in the crystallization buffer, and the remainder is contributed by the crystal lattice. These data provide a quantitative measure of how a conformational equilibrium in BtuB is modified in the crystal environment, and suggest that more-compact, less-hydrated substates will be favored in protein crystals.

摘要

成功的大分子晶体学需要溶液条件,这些条件可能会改变大分子的构象采样。在这里,通过定点自旋标记来研究大肠杆菌外膜维生素 B(12)转运蛋白 BtuB 中的构象平衡。放置在 BtuB 的 N 端能量偶联基序(Ton 盒)内的自旋标记的电子顺磁共振(EPR)谱表明,该片段在折叠和未折叠形式之间处于平衡状态。在双层膜中,底物结合将这种平衡推向未折叠形式;然而,来自同一自旋标记突变体的 EPR 谱表明,这种展开转变在蛋白质晶体中被阻断。此外,该自旋标记突变体的晶体结构与 EPR 结果一致。当从 EPR 谱估计亚态之间的自由能差时,与双层状态相比,发现晶体环境会使这种能量改变 3 千卡/摩尔。这种能量变化的大约一半是由于结晶缓冲液中的溶质或渗透物引起的,其余部分是由晶格贡献的。这些数据提供了一种定量的方法来衡量 BtuB 中的构象平衡在晶体环境中是如何被改变的,并表明在蛋白质晶体中更紧凑、更脱水的亚稳态将更受青睐。

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