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实时荧光定量PCR检测贝氏柯克斯体方法的建立
引用本文:亚红祥,张丽娟.实时荧光定量PCR检测贝氏柯克斯体方法的建立[J].中国热带医学,2011,11(8):916-917.
作者姓名:亚红祥  张丽娟
作者单位:1. 云南省地方病防治所,云南,大理,671000;中国疾病预防控制中心传染病预防控制所,北京,102206
2. 中国疾病预防控制中心传染病预防控制所,北京,102206
摘    要:目的建立检测贝氏柯克斯体的Real-Time PCR方法。方法根据贝氏柯克斯体特有的htpAB基因相关重复序列(IS1111a)进行PCR扩增片断485bp,以克隆的IS1111a基因片断作标准DNA模板,建立Real-Time PCR检测方法。结果建立的Real-Time PCR标准曲线的循环阈值(Ct)与模板拷贝数呈良好的线性关系(r=0.999);重复性测试Ct变异系数CV≤6.1%;其灵敏性约为普通PCR的10倍;以其它相关立克次体和病原菌DNA为模板应用于该方法,结果均为阴性。结论所建立的Real-Time PCR方法具有很好的特异性、灵敏性和重复性,可代替普通PCR用于贝氏柯克斯体的感染早期的快速定性、定量检测。

关 键 词:Real-TimePCR  贝氏柯克斯体  定性检测  定量检测

Quantitative detection of Coxiella burneti by real-time PCR
YA Hong-xiang,ZHANG Li-juan.Quantitative detection of Coxiella burneti by real-time PCR[J].China Tropical Medicine,2011,11(8):916-917.
Authors:YA Hong-xiang  ZHANG Li-juan
Institution:YA Hong-xiang,ZHANG Li-juan.(1.Yunnan Provincial institute for control of Endemic Diseases,Dali 671000,Yunnan,P.R.China,2.National Institute of Communicable Disease Control and Prevention,Chinese CDC,Beijing 102206,P.R.China)
Abstract:Objective To establish real-time PCR for detection of Coxiella burneti.Methods A 485-bp fragment of Coxiella burneti.was amplified according to the htpAB-associated repetitive element(ISlllla) of coxiella burneti,cloned the fragment of ISlllla gene as the target sequence of amplification in real-time PCR assay.Results A linear relationship between threshold cycle(Ct) of the real-time PCR and the copy number was observed(r=0.999),the coefficient of variation was CV≤6.1% in real-time PCR assay;its sensitivity was about 10 times higher than that of the general PCR in detection the homologous DNA assay;the results of detection of the DNA from other rickettsial agents and some pathogenic bacteria was negative.Conclusion The real-time PCR method established is highly specific,sensitive and reproducible and it can replace the general PCR technique in detection of coxiella burneti.
Keywords:Real-time PCR  coxiella burneti  Qualitative detection  Quantitative detection  
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