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基于荧光相关低温荧光和低温电子显微镜技术检测冷冻电镜网格上的膜融合状态

Fluorescence-Based Detection of Membrane Fusion State on a Cryo-EM Grid using Correlated Cryo-Fluorescence and Cryo-Electron Microscopy.

机构信息

Structural and Computational Biology Unit, European Molecular Biology Laboratory,69117 Heidelberg,Germany.

出版信息

Microsc Microanal. 2019 Aug;25(4):942-949. doi: 10.1017/S1431927619000606. Epub 2019 May 14.

Abstract

Correlated light and electron microscopy (CLEM) has become a popular technique for combining the protein-specific labeling of fluorescence with electron microscopy, both at room and cryogenic temperatures. Fluorescence applications at cryo-temperatures have typically been limited to localization of tagged protein oligomers due to known issues of extended triplet state duration, spectral shifts, and reduced photon capture through cryo-CLEM objectives. Here, we consider fluorophore characteristics and behaviors that could enable more extended applications. We describe how dialkylcarbocanine DiD, and its autoquenching by resonant energy transfer (RET), can be used to distinguish the fusion state of a lipid bilayer at cryo-temperatures. By adapting an established fusion assay to work under cryo-CLEM conditions, we identified areas of fusion between influenza virus-like particles and fluorescently labeled lipid vesicles on a cryo-EM grid. This result demonstrates that cryo-CLEM can be used to localize functions in addition to tagged proteins, and that fluorescence autoquenching by RET can be incorporated successfully into cryo-CLEM approaches. In the case of membrane fusion applications, this method provides both an orthogonal confirmation of functional state independent of the morphological description from cryo-EM and a way to bridge room-temperature kinetic assays and the cryo-EM images.

摘要

相关光和电子显微镜(CLEM)已成为一种将荧光的蛋白质特异性标记与电子显微镜结合的流行技术,可在室温下和低温下进行。由于已知的三重态持续时间延长、光谱位移以及通过低温 CLEM 物镜减少光子捕获等问题,低温荧光应用通常仅限于标记蛋白寡聚体的定位。在这里,我们考虑了可以实现更广泛应用的荧光染料特性和行为。我们描述了二烷基碳菁 DiD 及其通过共振能量转移(RET)的自动猝灭如何用于区分低温下脂质双层的融合状态。通过适应已建立的融合测定法在低温 CLEM 条件下工作,我们确定了流感病毒样颗粒与荧光标记脂质囊泡在冷冻电镜网格上融合的区域。这一结果表明,低温 CLEM 不仅可以用于标记蛋白的定位,还可以成功地将 RET 引起的荧光猝灭纳入低温 CLEM 方法中。在膜融合应用的情况下,该方法提供了与低温 EM 的形态描述无关的功能状态的正交确认,以及将室温动力学测定与低温 EM 图像联系起来的方法。

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