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链霉菌中脱氧核糖核酸同源性的测定方法。

Methods for the determination of deoxyribonucleic Acid homologies in streptomyces.

作者信息

Okanishi M, Gregory K F

机构信息

Department of Microbiology, University of Guelph, Guelph, Ontario, Canada.

出版信息

J Bacteriol. 1970 Dec;104(3):1086-94. doi: 10.1128/jb.104.3.1086-1094.1970.

Abstract

Variations of the membrane filter technique for deoxyribonucleic acid (DNA) hybridizations were studied with respect to Streptomyces species. At the temperatures required for specific hybridization of DNA with the high melting temperature (T(m)) characteristic of Streptomyces, large amounts (up to 97%) of filter-bound DNA became eluted, in all reaction mixtures studied, within 21 hr. In most solutions this leaching was increased by the presence of sheared denatured DNA. Incubation of DNA-loaded filters in a solution of 50% formamide containing 6x standard saline citrate, at 48 C for 40 hr, was judged to be the best set of conditions tested based on relatively good retention of immobilized DNA, very low hybridization with unrelated DNA of a similarly high T(m) (from Sarcina lutea), and the formation of complexes similar in thermal stability to the native DNA. The expression of results as sheared DNA bound in relation to long-chain DNA retained is recommended when a high concentration of sheared DNA relative to immobilized DNA is used.

摘要

针对链霉菌属,研究了用于脱氧核糖核酸(DNA)杂交的膜过滤技术的变体。在DNA与链霉菌高熔点(T(m))特征进行特异性杂交所需的温度下,在所研究的所有反应混合物中,大量(高达97%)结合在滤膜上的DNA在21小时内被洗脱。在大多数溶液中,剪切的变性DNA的存在会增加这种浸出。基于固定化DNA的相对良好保留、与具有相似高T(m)的无关DNA(来自藤黄八叠球菌)的极低杂交以及形成热稳定性与天然DNA相似的复合物,将加载DNA的滤膜在含有6倍标准柠檬酸盐缓冲盐水的50%甲酰胺溶液中于48℃孵育40小时被判定为所测试的最佳条件组合。当使用相对于固定化DNA高浓度的剪切DNA时,建议将结果表示为与保留的长链DNA相关的剪切DNA结合量。

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