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利用大肠杆菌通过图像细胞术对细菌类核中DNA相对含量进行定量的方法。

Image cytometric method for quantifying the relative amount of DNA in bacterial nucleoids using Escherichia coli.

机构信息

Institute for Molecular Cell Biology, BioCentrum Amsterdam, University of Amsterdam, Kruislaan 316, 1098 SM Amsterdam, The Netherlands.

出版信息

J Microsc. 1999 Oct;196(1):61-68. doi: 10.1046/j.1365-2818.1999.00597.x.

Abstract

An image cytometric method for quantifying integrated fluorescence was developed to measure the relative DNA contents of bacterial nucleoids. Image analysis was performed with newly developed macros in combination with the program Object-Image, all downloadable from . Four aspects of the method were investigated. (i) Good linearity was found over a ten-fold range of fluorescence intensity in a test with a calibration kit of fluorescent latex spheres. (ii) The accuracy of the method was tested with a narrowly distributed Escherichia coli population, which was obtained by growing cells into stationary phase. The width of the image cytometric distribution was approximately 6%, in good agreement with results obtained by flow cytometry. (iii) The error contribution of manual focusing could be kept below 2%, although a strong dependency between integrated fluorescence and focus position was observed. (iv) The results were verified with a flow cytometer, which gave similar distributions for the DNA contents per cell expressed in chromosome equivalents (4.8 fg of DNA). We used the presented method to evaluate whether the DNA conformation had any effect on the total fluorescence of bacterial nucleoids. Experiments using nucleoids with the same amount of DNA in either a dispersed or a compact conformation showed no significant difference in integrated fluorescence, indicating that it is possible to determine the DNA content per nucleoid independently of the actual organization of the DNA.

摘要

开发了一种用于定量积分荧光的图像细胞术方法,以测量细菌类核的相对DNA含量。使用新开发的宏程序结合Object-Image程序进行图像分析,所有这些都可以从……下载。对该方法的四个方面进行了研究。(i)在使用荧光乳胶球校准试剂盒的测试中,在十倍荧光强度范围内发现了良好的线性关系。(ii)用通过使细胞生长至稳定期获得的分布狭窄的大肠杆菌群体测试了该方法的准确性。图像细胞术分布的宽度约为6%,与流式细胞术获得的结果高度一致。(iii)尽管观察到积分荧光与聚焦位置之间存在强烈依赖性,但手动聚焦的误差贡献可保持在2%以下。(iv)用流式细胞仪验证了结果,该仪器给出了以染色体当量表示的每个细胞DNA含量的相似分布(4.8 fg DNA)。我们使用所提出的方法来评估DNA构象是否对细菌类核的总荧光有任何影响。使用具有相同DNA量的分散或紧密构象的类核进行的实验表明,积分荧光没有显著差异,这表明可以独立于DNA的实际组织来确定每个类核的DNA含量。

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