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Fast Fenton footprinting: a laboratory-based method for the time-resolved analysis of DNA RNA and proteins

机译:快速Fenton足迹:基于实验室的方法用于时间分辨的DNARNA和蛋白质分析

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摘要

‘Footprinting’ describes assays in which ligand binding or structure formation protects polymers such as nucleic acids and proteins from either cleavage or modification; footprinting allows the accessibility of individual residues to be mapped in solution. Equilibrium and time-dependent footprinting links site-specific structural information with thermodynamic and kinetic transitions. The hydroxyl radical (·OH) is a particularly valuable footprinting probe by virtue of it being among the most reactive of chemical oxidants; it reports the solvent accessibility of reactive sites on macromolecules with as fine as a single residue resolution. A novel method of millisecond time-resolved ·OH footprinting has been developed based on the Fenton reaction, Fe(II) + H2O2 → Fe(III) + ·OH + OH. This method can be implemented in laboratories using widely available three-syringe quench flow mixers and inexpensive reagents to study local changes in the solvent accessibility of DNA, RNA and proteins associated with their biological function.
机译:“脚印”描述了其中配体结合或结构形成可保护聚合物(例如核酸和蛋白质)不被切割或修饰的测定法;足迹可将单个残基的可及性映射到溶液中。平衡和时间依赖的足迹将站点特定的结构信息与热力学和动力学转变联系在一起。羟自由基(·OH)是一种特别有价值的足迹探针,因为它是化学氧化剂中反应性最强的一种。它报告了大分子上反应位点的溶剂可及性,其分离度与单个残基一样好。在Fenton反应的基础上,开发了一种新的毫秒时间分辨·OH足迹的方法,即Fe(II)+ H2O2→Fe(III)+·OH + OH -。该方法可在实验室中使用广泛使用的三针骤冷流动混合器和廉价的试剂来实施,以研究DNA,RNA和蛋白质与其生物学功能相关的溶剂可及性的局部变化。

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