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一种分析细菌核酸杂交的新方法。枯草芽孢杆菌核糖体核糖核酸的分析。

A new approach to the analysis of hybridization of bacterial nucleic acids. Analysis of the ribosomal ribonucleic acids of Bacillus subtilis.

作者信息

Avery R J, Midgley J E

出版信息

Biochem J. 1969 Nov;115(3):383-94. doi: 10.1042/bj1150383.

Abstract

A new graphical analytical technique is described for the hybridization of bacterial RNA with denatured homologous DNA immobilized on cellulose nitrate membrane filters. To a constant amount of DNA, various amounts of bacterial RNA were added and the percentage of input RNA bound was plotted against the DNA/RNA weight ratio in a given experiment. When RNA samples were used that hybridize to denatured DNA as a single species, the resulting curves (RNA-hybridization-efficiency curves) could be analysed to show the percentage of the DNA capable of specifically binding the RNA and could also be used to detect the presence of minor RNA contaminants in a purified specimen. The method could also estimate the relative amounts of two species of RNA in a mixture when these were hybridized independently to different DNA cistrons or cistron groups. As an example of RNA that can be studied in this way, the 16s and 23s ribosomal RNA species of Bacillus subtilis were chosen. These each behave in DNA-RNA hybridization as a single species and bind independently to different groups of DNA cistrons. The results obtained from hybridization-efficiency curves were compared with those obtained by the more usual method of saturating the specific DNA regions with excess of ribosomal RNA (hybridization-saturation curves). It was confirmed by both approaches that 0.15 (+/-0.02)% of B. subtilis DNA would hybridize with 16s ribosomal RNA, 0.30 (+/-0.02)% would hybridize with 23s ribosomal RNA, and 0.46 (+/-0.02)% would hybridize with (16s+23s) ribosomal RNA. This agreement suggested that mass-action equilibria between hybridized and free RNA had a negligible effect on the hybridization curves over the range of DNA and RNA concentrations employed.

摘要

本文描述了一种新的图形分析技术,用于细菌RNA与固定在硝酸纤维素膜滤器上的变性同源DNA的杂交。在给定实验中,向恒定数量的DNA中加入不同量的细菌RNA,并将结合的输入RNA百分比与DNA/RNA重量比作图。当使用能作为单一物种与变性DNA杂交的RNA样品时,所得曲线(RNA杂交效率曲线)可用于分析能够特异性结合RNA的DNA百分比,也可用于检测纯化样品中微量RNA污染物的存在。当混合物中的两种RNA分别与不同的DNA顺反子或顺反子组独立杂交时,该方法还可估计它们的相对含量。作为可用这种方法研究的RNA的一个例子,选择了枯草芽孢杆菌的16s和23s核糖体RNA。它们在DNA-RNA杂交中均表现为单一物种,并独立结合到不同的DNA顺反子组。将杂交效率曲线得到的结果与用过量核糖体RNA饱和特定DNA区域的更常用方法(杂交饱和曲线)得到的结果进行了比较。两种方法均证实,0.15(±0.02)%的枯草芽孢杆菌DNA可与16s核糖体RNA杂交,0.30(±0.02)%可与23s核糖体RNA杂交,0.46(±0.02)%可与(16s+23s)核糖体RNA杂交。这种一致性表明,在所使用的DNA和RNA浓度范围内,杂交RNA与游离RNA之间的质量作用平衡对杂交曲线的影响可忽略不计。

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