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一种用于研究蛋白质-DNA相互作用的简化甲醛固定和免疫沉淀技术。

A simplified formaldehyde fixation and immunoprecipitation technique for studying protein-DNA interactions.

作者信息

Dedon P C, Soults J A, Allis C D, Gorovsky M A

机构信息

Department of Biology, University of Rochester, New York 14627.

出版信息

Anal Biochem. 1991 Aug 15;197(1):83-90. doi: 10.1016/0003-2697(91)90359-2.

Abstract

Using the single cell eukaryote Tetrahymena thermophila, a simple method was developed for studying protein-DNA associations by cross-linking proteins to DNA with formaldehyde and immunoprecipitating the solubilized chromatin fragments with a specific antiserum. The protocol uses crude antiserum and involves only three steps: cross-linking, shearing to solubilize the chromatin, and immunoprecipitation. Methods for optimizing certain critical parameters, such as fixation time and NaCl concentration, are described. The method is likely to be generally useful for a variety of nuclear antigens.

摘要

利用单细胞真核生物嗜热栖热四膜虫,开发了一种简单的方法来研究蛋白质与DNA的结合,即通过甲醛将蛋白质与DNA交联,并用特异性抗血清免疫沉淀溶解的染色质片段。该方案使用粗抗血清,仅涉及三个步骤:交联、剪切以溶解染色质和免疫沉淀。文中描述了优化某些关键参数(如固定时间和NaCl浓度)的方法。该方法可能对多种核抗原普遍有用。

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