Quantitation of Nucleic Acids and Proteins

Current Protocols Essential Laboratory Techniques Pub Date : 2011-07-01 DOI:10.1002/9780470089941.et0202s5

Sean R. Gallagher, Philippe Desjardins

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引用次数: 15

Abstract

Reliable quantitation of nanogram and microgram amounts of DNA and RNA in solution is essential to researchers in molecular biology. Two methods for direct absorbance measurements at 260 nm are described—the first is a traditional cuvette-based method, and the second is a microvolume method that requires no cuvettes or capillaries. In addition, three fluorescence techniques using Hoechst 33258, ethidium bromide, and PicoGreen reagent are presented in this unit. These five procedures cover a range from 5 to 10 ng/ml DNA to 15,000 µg/ml DNA. Reliable quantitation of proteins is possible using several types of assays. UV spectroscopy is the simplest approach but is limited in sensitivity. More sensitive assays that use Coomassie blue binding, bicinchoninic acid (BCA), and the Lowry reaction are also described. All assays are prone to amino acid composition errors and interference from assay solution components. Flow charts and tables to help with appropriate method selection are included. Curr. Protoc. Essential Lab. Tech. 5:2.2.1-2.2.36. © 2011 by John Wiley & Sons, Inc.

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核酸和蛋白质的定量

溶液中DNA和RNA的纳克和微克量的可靠定量对分子生物学研究人员至关重要。描述了两种直接测量260 nm吸光度的方法，第一种是传统的基于比色皿的方法，第二种是不需要比色皿或毛细管的微体积方法。此外，本单元还介绍了使用Hoechst 33258、溴化乙啶和PicoGreen试剂的三种荧光技术。这五个程序涵盖范围从5至10 ng/ml DNA到15,000 μ g/ml DNA。可靠的定量蛋白质是可能使用几种类型的分析。紫外光谱法是最简单的方法，但灵敏度有限。更敏感的测定，使用考马斯蓝结合，比辛胆酸(BCA)，和Lowry反应也进行了描述。所有的分析都容易出现氨基酸组成错误和分析溶液组分的干扰。包括流程图和表格，以帮助适当的方法选择。咕咕叫。Protoc。基本的实验室。科技,5:2.2.1-2.2.36。©2011 by John Wiley &儿子,Inc。

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Current Protocols Essential Laboratory Techniques

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