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用于分离超螺旋、连环和打结DNA分子的电泳迁移率测定

Electrophoretic Mobility Assay to Separate Supercoiled, Catenated, and Knotted DNA Molecules.

作者信息

Cebrián Jorge, Martínez Victor, Hernández Pablo, Krimer Dora B, Martínez-Robles María-Luisa, Schvartzman Jorge B, Fernández-Nestosa María José

机构信息

Department of Cellular and Molecular Biology, Margarita Salas Center for Biological Research (CSIC), Madrid, Spain.

Polytechnic School, National University of Asuncion, San Lorenzo, Paraguay.

出版信息

Bio Protoc. 2024 May 5;14(9):e4983. doi: 10.21769/BioProtoc.4983.

Abstract

Two-dimensional (2D) agarose gel electrophoresis is the method of choice to analyze DNA topology. The possibility to use strains with different genetic backgrounds in combination with nicking enzymes and different concentrations of norfloxacin improves the resolution of 2D gels to study the electrophoretic behavior of three different families of DNA topoisomers: supercoiled DNA molecules, post-replicative catenanes, and knotted DNA molecules. Here, we describe the materials and procedures required to optimize their separation by 2D gels. Understanding the differences in their electrophoretic behavior can help explain some important physical characteristics of these different types of DNA topoisomers. Key features • Preparative method to enrich DNA samples of supercoiled, catenated, and knotted families of topoisomers, later analyzed by 2D gels (or other techniques, e.g., microscopy). • 2D gels facilitate the separation of the topoisomers of any given circular DNA molecule. • Separation of DNA molecules with the same molecular masses but different shapes can be optimized by modifying the conditions of 2D gels. • Evaluating the roles of electric field and agarose concentration on the electrophoretic mobility of DNA topoisomers sheds light on their physical characteristics.

摘要

二维(2D)琼脂糖凝胶电泳是分析DNA拓扑结构的首选方法。将具有不同遗传背景的菌株与切口酶和不同浓度的诺氟沙星结合使用,能够提高二维凝胶的分辨率,以研究三种不同类型DNA拓扑异构体的电泳行为:超螺旋DNA分子、复制后连环体和打结DNA分子。在此,我们描述了通过二维凝胶优化其分离所需的材料和步骤。了解它们电泳行为的差异有助于解释这些不同类型DNA拓扑异构体的一些重要物理特性。关键特性 • 用于富集超螺旋、连环和打结拓扑异构体家族DNA样本的制备方法,随后通过二维凝胶(或其他技术,如显微镜)进行分析。 • 二维凝胶有助于分离任何给定环状DNA分子的拓扑异构体。 • 通过改变二维凝胶的条件,可以优化具有相同分子量但不同形状的DNA分子的分离。 • 评估电场和琼脂糖浓度对DNA拓扑异构体电泳迁移率的作用有助于了解它们的物理特性。

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