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原子力显微镜:蛋白质-配体相互作用的解离力、解离速率和能垒的测定

Atomic force microscopy: determination of unbinding force, off rate and energy barrier for protein-ligand interaction.

作者信息

Lee Chih-Kung, Wang Yu-Ming, Huang Long-Sun, Lin Shiming

机构信息

Institute of Applied Mechanics, National Taiwan University, Taipei, Taiwan.

出版信息

Micron. 2007;38(5):446-61. doi: 10.1016/j.micron.2006.06.014. Epub 2006 Jul 28.

Abstract

Recently, atomic force microscopy (AFM) based force measurements have been applied biophysically and clinically to the field of molecular recognition as well as to the evaluation of dynamic parameters for various interactions between proteins and ligands in their native environment. The aim of this review is to describe the use of the AFM to measure the forces that control biological interaction, focusing especially on protein-ligand and protein-protein interaction modes. We first considered the measurements of specific and non-specific unbinding forces which together control protein-ligand interactions. As such, we will look at the theoretical background of AFM force measurement curves for evaluating the unbinding forces of protein-ligand complexes. Three AFM model dynamic parameters developed recently for use in protein-ligand interactions are reviewed: (i) unbinding forces, (ii) off rates, and (iii) binding energies. By reviewing the several techniques developed for measuring forces between biological structures and intermolecular forces in the literature, we show that use of an AFM for these applications provides an excellent tool in terms of spatial resolution and lateral resolution, especially for protein-protein and protein-ligand interactions.

摘要

最近,基于原子力显微镜(AFM)的力测量已在生物物理和临床领域应用于分子识别,以及评估蛋白质与配体在其天然环境中各种相互作用的动态参数。本综述的目的是描述使用AFM测量控制生物相互作用的力,特别关注蛋白质-配体和蛋白质-蛋白质相互作用模式。我们首先考虑了共同控制蛋白质-配体相互作用的特异性和非特异性解离力的测量。因此,我们将研究用于评估蛋白质-配体复合物解离力的AFM力测量曲线的理论背景。综述了最近开发的用于蛋白质-配体相互作用的三个AFM模型动态参数:(i)解离力,(ii)解离速率,和(iii)结合能。通过回顾文献中为测量生物结构之间的力和分子间力而开发的几种技术,我们表明,就空间分辨率和横向分辨率而言,使用AFM进行这些应用提供了一个出色的工具,特别是对于蛋白质-蛋白质和蛋白质-配体相互作用。

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