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A real-time PCR assay for detection and quantification of Mycoplasma agalactiae DNA

机译:实时PCR检测和定量无乳支原体DNA的方法

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Aims: The aim of this study was to develop a rapid, sensitive, specific tool for detection and quantification of Mycoplasma agalactiae DNA in sheep milk samples. Methods and Results: A real-time polymerase chain reaction (PCR) assay targeting the membrane-protein 81 gene of M. agalactiae was developed. The assay specifically detected M. agalactiae DNA without cross-amplification of other mycoplasmas and common pathogens of small ruminants. The method was reproducible and highly sensitive, providing precise quantification of M. agalactiae DNA over a range of nine orders of magnitude. Compared with an established PCR assay, the real-time PCR was one-log more sensitive, detecting as few as 10(1) DNA copies per 10 mu l of plasmid template and 6.5 x 10(0) colour changing units of reference strain Ba/2. Conclusions: The real-time PCR assay is a reliable method for the detection and quantification of M. agalactiae DNA in sheep milk samples. The assay is more sensitive than gel-based PCR protocols and provides quantification of the M. agalactiae DNA contained in milk samples. The assay is also quicker than traditional culture methods (2-3 h compared with at least 1 week). Significance and Impact of the Study: The established real-time PCR assay will help study the patterns of shedding of M. agalactiae in milk, aiding pathogenesis and vaccine efficacy studies.
机译:目的:本研究的目的是开发一种快速,灵敏,特异的工具,用于检测和定量羊奶样品中无乳支原体DNA。方法和结果:建立了针对无乳链球菌膜蛋白81基因的实时聚合酶链反应(PCR)方法。该测定法特异性地检测了无乳分枝杆菌DNA,而没有其他支原体和小反刍动物的常见病原体的交叉扩增。该方法可重现且高度灵敏,可在九个数量级的范围内对无乳链球菌DNA进行精确定量。与已建立的PCR分析相比,实时PCR的灵敏度提高了一个对数,每10 ul质粒模板可检测到10(1)个DNA拷贝,而参照菌株Ba的检测单元可检测到6.5 x 10(0)个变色单元/ 2。结论:实时荧光定量PCR是检测和定量羊乳样品中无乳支原体DNA的可靠方法。该测定比基于凝胶的PCR方案更为灵敏,可定量分析牛奶样品中所含的无乳支原体DNA。该测定法也比传统培养方法更快(2-3小时,而至少需要1周)。研究的意义和影响:建立的实时PCR分析将有助于研究牛奶中无乳分枝杆菌脱落的模式,有助于发病机理和疫苗功效研究。

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