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测量细胞表面受体-配体结合动力学:从黏附频率到热波动方法。

Measuring Receptor-Ligand Binding Kinetics on Cell Surfaces: From Adhesion Frequency to Thermal Fluctuation Methods.

作者信息

Chen Wei, Zarnitsyna Veronika I, Sarangapani Krishna K, Huang Jun, Zhu Cheng

机构信息

Woodruff School of Mechanical Engineering, Georgia Institute of Technology, Atlanta, GA 30332, USA.

出版信息

Cell Mol Bioeng. 2008 Dec 1;1(4):276-288. doi: 10.1007/s12195-008-0024-8.

Abstract

Interactions between surface-anchored receptors and ligands mediate cell-cell and cell-environment communications in many biological processes. Molecular interactions across two apposing cell membrane are governed by two-dimensional (2D) kinetics, which are physically distinct from and biologically more relevant than three-dimensional (3D) kinetics with at least one interacting molecular species in the fluid phase. Here we review two assays for measuring 2D binding kinetics: the adhesion frequency assay and the thermal fluctuation assay. The former measures the binding frequency as a function of contact duration and extracts the force-free 2D kinetics parameters by nonlinearly fitting the data with a probabilistic model. The latter detects bond formation/dissociation by monitoring the reduction/resumption of thermal fluctuations of a force sensor. Both assays are mechanically based and operate at the level of mostly single molecular interaction, which requires ultrasensitive force techniques. Characterization of one such technique, the biomembrane force probe, is presented.

摘要

表面锚定受体与配体之间的相互作用在许多生物过程中介导细胞间和细胞与环境间的通讯。两个相对细胞膜之间的分子相互作用受二维(2D)动力学支配,这在物理上与至少一种相互作用分子处于液相的三维(3D)动力学不同,且在生物学上更具相关性。在此,我们综述两种用于测量二维结合动力学的测定方法:粘附频率测定法和热涨落测定法。前者将结合频率作为接触持续时间的函数进行测量,并通过用概率模型对数据进行非线性拟合来提取无外力二维动力学参数。后者通过监测力传感器热涨落的降低/恢复来检测键的形成/解离。这两种测定方法均基于力学原理,且大多在单分子相互作用水平上运行,这需要超灵敏的力技术。本文介绍了其中一种技术——生物膜力探针的特性。

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