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DNA 盘绕介导的易化扩散

Facilitated diffusion with DNA coiling.

作者信息

Lomholt Michael A, van den Broek Bram, Kalisch Svenja-Marei J, Wuite Gijs J L, Metzler Ralf

机构信息

Department of Physics and Chemistry, MEMPHYS Center for Biomembrane Physics, University of Southern Denmark, Odense M, Denmark.

出版信息

Proc Natl Acad Sci U S A. 2009 May 19;106(20):8204-8. doi: 10.1073/pnas.0903293106. Epub 2009 May 6.

Abstract

When DNA-binding proteins search for their specific binding site on a DNA molecule they alternate between linear 1-dimensional diffusion along the DNA molecule, mediated by nonspecific binding, and 3-dimensional volume excursion events between successive dissociation from and rebinding to DNA. If the DNA molecule is kept in a straight configuration, for instance, by optical tweezers, these 3-dimensional excursions may be divided into long volume excursions and short hops along the DNA. These short hops correspond to immediate rebindings after dissociation such that a rebinding event to the DNA occurs at a site that is close to the site of the preceding dissociation. When the DNA molecule is allowed to coil up, immediate rebinding may also lead to so-called intersegmental jumps, i.e., immediate rebindings to a DNA segment that is far away from the unbinding site when measured in the chemical distance along the DNA, but close by in the embedding 3-dimensional space. This effect is made possible by DNA looping. The significance of intersegmental jumps was recently demonstrated in a single DNA optical tweezers setup. Here we present a theoretical approach in which we explicitly take the effect of DNA coiling into account. By including the spatial correlations of the short hops we demonstrate how the facilitated diffusion model can be extended to account for intersegmental jumping at varying DNA densities. It is also shown that our approach provides a quantitative interpretation of the experimentally measured enhancement of the target location by DNA-binding proteins.

摘要

当DNA结合蛋白在DNA分子上寻找其特定结合位点时,它们在由非特异性结合介导的沿DNA分子的线性一维扩散与连续从DNA解离并重新结合之间的三维体积偏移事件之间交替。例如,如果通过光镊将DNA分子保持在直线构型,这些三维偏移可分为沿DNA的长体积偏移和短跳跃。这些短跳跃对应于解离后的立即重新结合,使得对DNA的重新结合事件发生在靠近前一次解离位点的位点。当允许DNA分子盘绕时,立即重新结合也可能导致所谓的片段间跳跃,即在沿DNA的化学距离测量时,对远离解离位点的DNA片段的立即重新结合,但在嵌入的三维空间中距离很近。这种效应是由DNA环化实现的。片段间跳跃的重要性最近在单个DNA光镊装置中得到了证明。在这里,我们提出一种理论方法,其中我们明确考虑了DNA盘绕的影响。通过包括短跳跃的空间相关性,我们展示了促进扩散模型如何能够扩展以解释在不同DNA密度下的片段间跳跃。还表明我们的方法为通过DNA结合蛋白对实验测量的靶标定位增强提供了定量解释。

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