低温电子显微镜中空气-水界面吸附问题的理论框架和实验解决方案。

Joon S Kang, Xueting Zhou, Yun-Tao Liu, Kaituo Wang, Z Hong Zhou
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引用次数: 0

摘要

随着低温电子显微镜(cryoEM)作为确定生物复合物原子结构的一种首选方法在结构生物学领域得到广泛应用,越来越多的人认识到,许多在传统负染色电子显微镜下表现良好的复合物往往会在低温电子显微镜网格上出现优先取向、聚集或神秘 "消失 "的现象。然而,人们对这种错误行为的原因并不十分清楚,这就限制了解决这一问题的系统方法。在此,我们提出了一种理论公式来解释这些观察结果。我们的理论预测,所有颗粒都会迁移到空气-水界面(AWI),以降低总的潜在表面能--这就合理地解释了表面活性剂的使用,它是降低水溶液表面张力的直接解决方案。通过对经过广泛测试的样品 GroEL 进行低温电子断层扫描(cryoET),我们证明了在标准缓冲溶液中,几乎所有颗粒都会迁移到 AWI。通过引入表面活性剂逐步降低表面张力,暴露在表面的颗粒比例有所下降。通过进行单颗粒冷冻电镜实验,我们证实了合适的表面活性剂不会损坏生物复合物,从而表明它们可以为高分辨率冷冻电镜提供一种实用、简单和通用的解决方案。将这一解决方案应用于现实世界中的一个 AWI 吸附问题,该问题涉及一个更具挑战性的膜蛋白,即 ClC-1 通道,我们利用冷冻电镜测定了该通道的近原子结构。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Theoretical framework and experimental solution for the air-water interface adsorption problem in cryoEM.

As cryogenic electron microscopy (cryoEM) gains traction in the structural biology community as a method of choice for determining atomic structures of biological complexes, it has been increasingly recognized that many complexes that behave well under conventional negative-stain electron microscopy tend to have preferential orientation, aggregate or simply mysteriously "disappear" on cryoEM grids. However, the reasons for such misbehavior are not well understood, which limits systematic approaches to solving the problem. Here, we have developed a theoretical formulation that explains these observations. Our formulation predicts that all particles migrate to the air-water interface (AWI) to lower the total potential surface energy-rationalizing the use of surfactant, which is a direct solution to reduce the surface tension of the aqueous solution. By performing cryogenic electron tomography (cryoET) on the widely-tested sample, GroEL, we demonstrate that, in a standard buffer solution, nearly all particles migrate to the AWI. Gradually reducing the surface tension by introducing surfactants decreased the percentage of particles exposed to the surface. By conducting single-particle cryoEM, we confirm that suitable surfactants do not damage the biological complex, thus suggesting that they might provide a practical, simple, and general solution to the problem for high-resolution cryoEM. Applying this solution to a real-world AWI adsorption problem involving a more challenging membrane protein, namely, the ClC-1 channel, has resulted in its near-atomic structure determination using cryoEM.

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