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Fluorometric Determination of Deoxyribonucleic Acid in Bacteria with Ethidium Bromide

机译:溴化乙锭荧光法测定细菌中的脱氧核糖核酸

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A simple, sensitive, and rapid method is presented for the determination of deoxyribonucleic acid (DNA) in both gram-positive and gram-negative bacteria. It is based upon the fluorometric determination of DNA with ethidium bromide after alkaline digestion of the bacteria to hydrolyze the interfering ribonucleic acid. The assay takes less than 2 hr. Its sensitivity is at least 0.2 μg of DNA in a final solution of 4 ml and it uses commonly available filter or double monochromator fluorometers. Judicious choice of light source and filters allows an additional 10-fold increase in sensitivity with a filter fluorometer. Turbidity caused by bacteria or insoluble polysaccharides does not interfere with the fluorescence measurements. There was no significant difference between the results obtained with this method and those obtained with the indole and diphenylamine methods when these assays were applied to Escherichia coli and sucrose- or glucose-grown Streptococcus mutans. The method was also tested by determining the specific growth rate of E. coli. This new procedure should be especially useful for the determination of bacterial DNA in dilute suspensions and for the estimation of bacterial growth or DNA replication where more conventional methods are not applicable or sensitive enough.
机译:提出了一种简单,灵敏,快速的方法来测定革兰氏阳性和革兰氏阴性细菌中的脱氧核糖核酸(DNA)。它是基于细菌碱性消化以水解干扰的核糖核酸后,用溴化乙锭对DNA进行荧光测定。该测定少于2小时。在4 ml的最终溶液中,它的灵敏度至少为0.2μgDNA,并且使用常用的滤光片或双单色仪荧光计。明智地选择光源和滤光片可使滤光片荧光计的灵敏度再提高10倍。由细菌或不溶性多糖引起的浊度不会干扰荧光测量。当将这些测定法应用于大肠杆菌和蔗糖或葡萄糖生长的变形链球菌时,该方法获得的结果与吲哚和二苯胺方法获得的结果之间没有显着差异。还通过确定大肠杆菌的特定生长率来测试该方法。在更常规的方法不适用或不够灵敏的情况下,这种新方法对于确定稀悬液中的细菌DNA以及估算细菌的生长或DNA复制特别有用。

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