Yield Gel via Quantitative Gel Electrophoresis

核酸凝胶电泳 琼脂糖 琼脂糖凝胶电泳 凝胶电泳 分子量大小标记 色谱法 电泳 污渍 DNA 化学 颜色标记 聚丙烯酰胺凝胶电泳 蛋白质凝胶电泳 染色 生物 生物化学 遗传学
作者
Victoria R Parks,Duarte Torres
出处
期刊:Methods in molecular biology [Springer Science+Business Media]
卷期号:: 129-147
标识
DOI:10.1007/978-1-0716-3295-6_9
摘要

Quantitative gel electrophoresis, also referred to as yield gel via gel electrophoresis, is an early quantification method that was developed to provide an estimate of the quality and the quantity of DNA extracted from evidence or reference samples. To conduct quantitative gel electrophoresis, an agarose gel that is combined with a nucleic acid gel stain is prepared. The gel stain intercalates between double-stranded DNA and can be visualized using UV light. DNA extract samples, along with DNA standards (ranging from 250 to 5 ng), and a 1 KB ladder are combined with a 6X loading dye and loaded on the agarose gel. Voltage is applied to facilitate DNA migration through the gel from the negative to the positive electrode, separating DNA fragments by size. After electrophoresis is complete, the results are visualized using UV light, and an image is captured for analysis. High-quality and -quantity DNA should contain a compact band comparable to that of the high molecular weight standards and ladder, with some smearing down the sample well. If a DNA extract sample does not produce a compact band and presents with only a smear, this is an indication that DNA degradation has occurred. This chapter provides instructions on how to successfully prepare an agarose gel, load DNA extract samples and corresponding controls, appropriately set up and run quantitative gel electrophoresis, interpret the results, and ensure comprehension of the method so troubleshooting can be performed if needed.
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