Reconstitution and Purification of Nucleosomes with Recombinant Histones and Purified DNA

Q2 Biochemistry, Genetics and Molecular Biology
Ilana M. Nodelman, Ashok Patel, Robert F. Levendosky, Gregory D. Bowman
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引用次数: 12

Abstract

Nucleosomes are substrates for a broad range of factors, including those involved in transcription or chromosome maintenance/reorganization and enzymes that covalently modify histones. Given the heterogeneous nature of nucleosomes in vivo (i.e., varying histone composition, post-translational modifications, DNA sequence register), understanding the specificity and activities of chromatin-interacting factors has required in vitro studies using well-defined nucleosome substrates. Here, we provide detailed methods for large-scale PCR preparation of DNA, assembly of nucleosomes from purified DNA and histones, and purification of DNA and mononucleosomes. Such production of well-defined nucleosomes for biochemical and biophysical studies is key for studying numerous proteins and protein complexes that bind and/or alter nucleosomes and for revealing inherent characteristics of nucleosomes. © 2020 Wiley Periodicals LLC.

Basic Protocol 1: Large-scale PCR amplification of DNA

Basic Protocol 2: DNA and nucleosome purification using a Bio-Rad Mini Prep Cell/Prep Cell

Basic Protocol 3: Nucleosome reconstitution via linear gradient salt dialysis

用重组组蛋白和纯化DNA重组和纯化核小体
核小体是多种因子的底物,包括参与转录或染色体维持/重组的因子和共价修饰组蛋白的酶。鉴于核小体在体内的异质性(即不同的组蛋白组成、翻译后修饰、DNA序列登记),了解染色质相互作用因子的特异性和活性需要使用定义明确的核小体底物进行体外研究。在这里,我们提供了详细的方法,大规模PCR制备DNA,组装从纯化的DNA和组蛋白核小体,纯化DNA和单核小体。这种用于生化和生物物理研究的定义明确的核小体的生产是研究结合和/或改变核小体的众多蛋白质和蛋白质复合物以及揭示核小体固有特征的关键。基本方案1:DNA的大规模PCR扩增。基本方案2:使用Bio-Rad Mini Prep Cell/Prep Cell纯化DNA和核小体。基本方案3:通过线性梯度盐透析重建核小体
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Current Protocols in Molecular Biology
Current Protocols in Molecular Biology Biochemistry, Genetics and Molecular Biology-Molecular Biology
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