利用SYBR Green检测衣原体Real-Time PCR方法的建立  被引量:2

Development of a Real-Time PCR Assay for Detection and Quantitation of Chlamydia Using SYBR Green and the Light Cycler

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作  者:杨建民[1] 郝永新[1] 赵德明[1] 何诚[1] 

机构地区:[1]中国农业大学动物医学院国家动物海绵状脑病实验室,北京100094

出  处:《畜牧兽医学报》2006年第1期84-90,共7页ACTA VETERINARIA ET ZOOTECHNICA SINICA

基  金:国家自然科学基金项目(30370072);北京自然科学基金项目(6052014)

摘  要:利用SYBR Green建立了检测种特异性衣原体的Real-Time PCR方法。本方法应用衣原体种特异性的高度保守特异引物,能够扩增627bp特异片段;使用定量标准基因组DNA,本方法能准确检测最少250fg衣原体DNA。Real-TimePCR方法与免疫荧光方法的检测结果表明:检测4种衣原体临床样本,Real-TimePCR敏感性均在96%~98%;特异性均为100%;这两种方法符合率达97%以上(n=60);批内和批间重复性试验结果表明,本方法具有良好的准确性。本方法的建立对于快速、准确检测临床样本种特异性衣原体提供了一种切实有效的方法。Here, we presented a Chlamydiaceae-specific 23S rRNA--based real-time PCR assay for simultaneous detection and quantltation of four members of Chlamydiaceae family, C. trachomatis, C. psittaci, C. pneumoniae and C. Decorum, using SYBR Green and LightcyclerTM. The as- say was characterized using plasmid constructs of the bacteria and verified on standard strains of all four species of the Chlamydiaceae and a large cohort of clinical samples collected from human and animals by comparison with fluorescence immunohistochemistry method. The results showed that the present real-time PCR assay was of high specificity and sensitivity. It was capable of detecting as few as 250 fg of chlamydial DNA (equivalent to 10^-1 IFU) and was applicable to both liquid cultures and clinical samples. This assay may therefore offer a rapid, economic and reliable method for screening of the chlamydiaceae pathogens.

关 键 词:SYBR Green 衣原体 REAL-TIME PCR 检测 

分 类 号:S852.67[农业科学—基础兽医学] S854.43[农业科学—兽医学]

 

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