优质单分子DNA底物的高产量纯化。

Journal of biological methods Pub Date : 2021-02-24 eCollection Date: 2021-01-01 DOI:10.14440/jbm.2021.350
Yue Lu, Piero Bianco
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引用次数: 1

摘要

涉及DNA或RNA的单分子研究,需要高质量的核酸底物的均匀制备。在过去的几年中,已经发表了各种方法,描述了不同的纯化方法,但即使在经验丰富的实验室科学家手中,这些方法也令人沮丧地与可变产量不一致。为了解决这些问题,我们提出了一种优化的、直接的、基于柱的方法,这种方法是可重复的,并能产生高产量的底物或高质量的底物成分。该方法成功的核心是使用无孔阴离子交换树脂。除了使用这种树脂外,我们还鼓励对基材施工中的每个步骤进行优化。完全优化的方法产生高产量的发夹DNA底物的特殊质量。虽然该底物适用于单分子磁镊子实验,但所描述的方法很容易适用于大多数涉及70-15000 bp核酸的单分子研究的DNA底物的生产。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

High-yield purification of exceptional-quality, single-molecule DNA substrates.

High-yield purification of exceptional-quality, single-molecule DNA substrates.

High-yield purification of exceptional-quality, single-molecule DNA substrates.

High-yield purification of exceptional-quality, single-molecule DNA substrates.

Single-molecule studies involving DNA or RNA, require homogeneous preparations of nucleic acid substrates of exceptional quality. Over the past several years, a variety of methods have been published describing different purification methods but these are frustratingly inconsistent with variable yields even in the hands of experienced bench scientists. To address these issues, we present an optimized and straightforward, column-based approach that is reproducible and produces high yields of substrates or substrate components of exceptional quality. Central to the success of the method presented is the use of a non-porous anion exchange resin. In addition to the use of this resin, we encourage the optimization of each step in the construction of substrates. The fully optimized method produces high yields of a hairpin DNA substrate of exceptional quality. While this substrate is suitable for single-molecule, magnetic tweezer experiments, the described method is readily adaptable to the production of DNA substrates for the majority of single-molecule studies involving nucleic acids ranging in size from 70-15000 bp.

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