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结合共焦和原子力显微镜定量研究单病毒与哺乳动物细胞表面的结合。

Combining confocal and atomic force microscopy to quantify single-virus binding to mammalian cell surfaces.

机构信息

Department of Biosystems Science and Engineering, ETH Zurich, Basel, Switzerland.

Institute of Life Sciences, Université catholique de Louvain, Louvain-la-Neuve, Belgium.

出版信息

Nat Protoc. 2017 Nov;12(11):2275-2292. doi: 10.1038/nprot.2017.112. Epub 2017 Oct 5.

DOI:10.1038/nprot.2017.112
PMID:28981124
Abstract

Over the past five years, atomic force microscopy (AFM)-based approaches have evolved into a powerful multiparametric tool set capable of imaging the surfaces of biological samples ranging from single receptors to membranes and tissues. One of these approaches, force-distance curve-based AFM (FD-based AFM), uses a probing tip functionalized with a ligand to image living cells at high-resolution and simultaneously localize and characterize specific ligand-receptor binding events. Analyzing data from FD-based AFM experiments using appropriate probabilistic models allows quantification of the kinetic and thermodynamic parameters that describe the free-energy landscape of the ligand-receptor bond. We have recently developed an FD-based AFM approach to quantify the binding events of single enveloped viruses to surface receptors of living animal cells while simultaneously observing them by fluorescence microscopy. This approach has provided insights into the early stages of the interaction between a virus and a cell. Applied to a model virus, we probed the specific interaction with cells expressing viral cognate receptors and measured the affinity of the interaction. Furthermore, we observed that the virus rapidly established specific multivalent interactions and found that each bond formed in sequence strengthened the attachment of the virus to the cell. Here we describe detailed procedures for probing the specific interactions of viruses with living cells; these procedures cover tip preparation, cell sample preparation, step-by-step FD-based AFM imaging and data analysis. Experienced microscopists should be able to master the entire set of protocols in 1 month.

摘要

在过去的五年中,原子力显微镜(AFM)技术已经发展成为一种强大的多参数工具集,能够对从单个受体到膜和组织的生物样本表面进行成像。其中一种方法是基于力-距离曲线的 AFM(FD-AFM),它使用带有配体的探测尖端来高分辨率地对活细胞进行成像,并同时定位和表征特定的配体-受体结合事件。使用适当的概率模型分析 FD-AFM 实验数据,可以定量描述描述配体-受体键的自由能景观的动力学和热力学参数。我们最近开发了一种基于 FD 的 AFM 方法,用于量化单包膜病毒与活动物细胞表面受体的结合事件,同时通过荧光显微镜进行观察。这种方法深入了解了病毒与细胞相互作用的早期阶段。应用于模型病毒,我们探测了与表达病毒同源受体的细胞的特异性相互作用,并测量了相互作用的亲和力。此外,我们观察到病毒迅速建立了特异性多价相互作用,并且发现每个连续形成的键都增强了病毒与细胞的附着。本文详细介绍了探测病毒与活细胞特异性相互作用的程序;这些程序涵盖了尖端制备、细胞样品制备、逐步 FD-AFM 成像和数据分析。有经验的显微镜专家应该能够在 1 个月内掌握整套方案。

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