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荧光相关光谱法监测 RNA 二聚化。

RNA dimerization monitored by fluorescence correlation spectroscopy.

机构信息

Institute for Biochemistry and Molecular Biology, Department of Chemistry, Hamburg University, Germany.

出版信息

Eur Biophys J. 2011 Aug;40(8):907-21. doi: 10.1007/s00249-011-0701-8. Epub 2011 Jun 15.

DOI:10.1007/s00249-011-0701-8
PMID:21674181
Abstract

Fluorescence correlation spectroscopy (FCS) provides a versatile tool to investigate molecular interaction under native conditions, approximating infinite dilution. One precondition for its application is a sufficient difference between the molecular weights of the fluorescence-labelled unbound and bound ligand. In previous studies, an 8-fold difference in molecular weights or correspondingly a 1.6-fold difference in diffusion coefficients was required to accurately distinguish between two diffusion species by FCS. In the presented work, the hybridization of two complementary equally sized RNA single strands was investigated at an excellent signal-to-noise ratio enabled by the highly photostable fluorophore Atto647N. The fractions of ssRNA and dsRNA were quantified by applying multicomponent model analysis of single autocorrelation functions and globally fitting several autocorrelation functions. By introducing a priori knowledge into the fitting procedure, 1.3- to 1.4-fold differences in diffusion coefficients of single- and double-stranded RNA of 26, 41, and 54 nucleotides could be accurately resolved. Global fits of autocorrelation functions of all titration steps enabled a highly accurate quantification of diffusion species fractions and mobilities. At a high signal-to-noise ratio, the median of individually fitted autocorrelation functions allowed a robust representation of heterogeneous data. These findings point out the possibility of studying molecular interaction of equally sized molecules based on their diffusional behavior, which significantly broadens the application spectrum of FCS.

摘要

荧光相关光谱(FCS)提供了一种通用的工具,可在近似于无限稀释的天然条件下研究分子相互作用。其应用的一个前提条件是,荧光标记的未结合和结合配体的分子量之间有足够的差异。在以前的研究中,需要分子量相差 8 倍或扩散系数相差 1.6 倍,才能通过 FCS 准确地区分两种扩散物种。在本工作中,利用高度光稳定的荧光染料 Atto647N 实现了优异的信噪比,研究了两条互补的等大小 RNA 单链的杂交。通过对单自相关函数的多组分模型分析和全局拟合几个自相关函数,定量了 ssRNA 和 dsRNA 的分数。通过在拟合过程中引入先验知识,可以准确分辨 26、41 和 54 个核苷酸的单链和双链 RNA 的扩散系数差异 1.3 到 1.4 倍。所有滴定步骤的自相关函数的全局拟合能够高度准确地定量扩散物种分数和迁移率。在高信噪比下,个别拟合自相关函数的中位数允许对异质数据进行稳健的表示。这些发现指出了基于扩散行为研究等大小分子的分子相互作用的可能性,这显著拓宽了 FCS 的应用范围。

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