Stein A, Raoult D
Unite des Rickettsies, Faculte de Medecine, Marseille, France.
J Clin Microbiol. 1992 Sep;30(9):2462-6. doi: 10.1128/jcm.30.9.2462-2466.1992.
The polymerase chain reaction (PCR) was used for the detection of Coxiella burnetti, an obligate intracellular bacterium and the etiologic agent of Q fever. A pair of primers derived from the C. burnetii superoxide dismutase gene served to amplify a targeted 257-bp fragment of genomic DNA. These primers were chosen on the basis of GenBank analysis, G + C ratio, and absence of secondary structure. This technique allowed the detection of as few as 10 C. burnetii organisms. C. burnetti was detected in tissue culture and in specimens from patients (heart valves). In all, 8 reference isolates and 22 new isolates of C. burnetii from France were successfully amplified. No amplification products were found when PCR was performed with 25 bacterial species that had been isolated in a clinical laboratory from patients with clinically similar infections. Amplification products of C. burnetii were confirmed by restriction enzyme digestion and dot blot hybridization. The method used here, a combination of PCR and restriction analysis, is a faster and more sensitive assay for C. burnetii than standard culture techniques.
聚合酶链反应(PCR)用于检测伯氏考克斯体,这是一种专性胞内细菌,也是Q热的病原体。一对源自伯氏考克斯体超氧化物歧化酶基因的引物用于扩增基因组DNA的一个目标257碱基对片段。这些引物是根据GenBank分析、G+C比例以及不存在二级结构来选择的。该技术能够检测低至10个伯氏考克斯体生物体。在组织培养物以及患者(心脏瓣膜)标本中检测到了伯氏考克斯体。总共成功扩增了来自法国的8株伯氏考克斯体参考菌株和22株新菌株。当用临床实验室从临床症状相似感染患者中分离出的25种细菌进行PCR时,未发现扩增产物。伯氏考克斯体的扩增产物通过限制性酶切消化和斑点印迹杂交得到确认。这里使用的方法,即PCR与限制性分析相结合,对于伯氏考克斯体来说,是一种比标准培养技术更快且更灵敏的检测方法。
