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首页> 外文期刊>Journal of Molecular Biology >VISUALIZATION OF LARGE DNA MOLECULES BY ELECTRON MICROSCOPY WITH POLYAMINES - APPLICATION TO THE ANALYSIS OF YEAST ENDOGENOUS AND ARTIFICIAL CHROMOSOMES
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VISUALIZATION OF LARGE DNA MOLECULES BY ELECTRON MICROSCOPY WITH POLYAMINES - APPLICATION TO THE ANALYSIS OF YEAST ENDOGENOUS AND ARTIFICIAL CHROMOSOMES

机译:电子显微镜与多胺可视化大分子DNA-在酵母内源性和人工染色体分析中的应用

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摘要

Standard visualization of nucleic acids by electron microscopy requires the use of special spreading techniques. The most common method takes advantage of the formation of a complex between negatively charged nucleic acid molecules and a positively charged monolayer film of proteins or cationic agents. Here, we describe an alternative protocol for the rapid visualization of DNA by electron microscopy based on the complexes formed when nucleic acids are exposed to buffers containing polyamines in the presence of sodium chloride. This procedure has been devised for the detection and analysis of large DNA molecules, such as yeast artificial chromosomes, but can be applied to DNA molecules of small size as well. The formation of DNA-polyamine complexes stabilizes large DNA molecules in solution and prevents shearing. This property allows large DNA molecules to remain intact after passage through microcapillaries used in the generation of transgenic mice by microinjection of fertilized eggs. [References: 27]
机译:通过电子显微镜对核酸进行标准可视化需要使用特殊的铺展技术。最常用的方法是利用带负电的核酸分子与带正电的蛋白质或阳离子试剂的单层膜之间形成复合物。在这里,我们描述了一种替代方案,该方案基于当核酸在氯化钠存在下暴露于含有多胺的缓冲液中时形成的复合物,通过电子显微镜快速观察DNA。已经设计了该程序用于检测和分析大型DNA分子(例如酵母人工染色体),但也可以应用于小尺寸的DNA分子。 DNA-多胺复合物的形成可稳定溶液中的大DNA分子并防止剪切。这种特性使大的DNA分子在通过微注射受精卵的转基因小鼠中使用的微毛细管通过后仍保持完整。 [参考:27]

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