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基于荧光的磷光成像斑点印迹DNA杂交检测法的优化,用于评估大肠杆菌毒力基因谱。

Optimization of a fluorescent-based phosphor imaging dot blot DNA hybridization assay to assess E. coli virulence gene profiles.

作者信息

Zhang L, Gillespie B W, Marrs C F, Foxman B

机构信息

Department of Epidemiology, School of Public Health, University of Michigan, Ann Arbor, MI 48109, USA.

出版信息

J Microbiol Methods. 2001 Apr;44(3):225-33. doi: 10.1016/s0167-7012(01)00222-6.

Abstract

To increase the efficiency and consistency in screening Escherichia coli for virulence genes, a Phosphor Imager was adopted for signal detection in Dot Blot DNA hybridization replacing X-ray film read by eye. We assessed not only the reliability of the instrument-based procedure, but the impact of going from an outcome measured by visualization on a semi-quantitative scale to a digitized readout on an interval scale. We analyzed technical and biological variability of the assay and the factors contributing to the variability. In spite of high variability both within and between membranes in the Phosphor Imager readings, we were able to define classification rules for gene presence that were remarkably consistent. Using the X-ray film signal detection procedure with Southern confirmation as a gold standard, we obtained a sensitivity and specificity of 87-99% for a rule requiring no retesting for all but one gene probe.

摘要

为提高筛选大肠杆菌毒力基因的效率和一致性,采用磷光成像仪在斑点印迹DNA杂交中进行信号检测,取代了肉眼读取的X射线胶片。我们不仅评估了基于仪器方法的可靠性,还评估了从半定量可视化测量结果转变为区间尺度数字化读数的影响。我们分析了该检测方法的技术和生物学变异性以及导致变异性的因素。尽管磷光成像仪读数在膜内和膜间都存在高度变异性,但我们能够定义出基因存在的分类规则,这些规则非常一致。以X射线胶片信号检测程序并经Southern印迹确认作为金标准,对于除一个基因探针外无需重新检测的规则,我们获得了87 - 99%的灵敏度和特异性。

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