基于两步聚合酶链反应的检测方法用于鉴定黎巴嫩感染儿童中耳积液的细菌病因
Two-step PCR-based assay for identification of bacterial etiology of otitis media with effusion in infected Lebanese children.
作者信息
Matar G M, Sidani N, Fayad M, Hadi U
机构信息
Department of Microbiology and Immunology, Faculty of Medicine, American University of Beirut, New York, New York 10022, USA.
出版信息
J Clin Microbiol. 1998 May;36(5):1185-8. doi: 10.1128/JCM.36.5.1185-1188.1998.
We developed and evaluated a two-step PCR-based assay with universal primers and genus- or species-specific primers for the detection of the most prevalent bacterial etiologies of otitis media with effusion (OME) in children from Lebanese hospitals. These etiologies included Haemophilus, Streptococcus, and Moraxella (Branhamella) catarrhalis, which were detected in middle-ear effusion (MEE) samples taken from children with OME. A total of 47 MEE samples were aspirated from 36 patients during insertion of a tympanostomy tube performed particularly for OME. The duration of effusion in all patients was > or =2 months. DNA was extracted from MEE samples, and PCR was initially done with DNA extracts by using the universal primers RW01 and DG74, which flank an approximately 370-bp fragment found in the 16S rRNA gene of all bacterial species. For the identification of specific bacteria, we used in three separate reaction mixtures the following genus- or species-specific primers: (i) a Haemophilus-specific probe (probe RDR125) as a primer along with DG74, (ii) a Streptococcus-specific primer (primer STR1; designed by us) along with DG74, and (iii) an M. catarrhalis-specific primer pair (primer pair MCA1-MCA2). Thirty-five MEE samples (74.5%) gave the expected 370-bp band, indicating the presence of bacterial DNA in the tested samples. Of the 35 PCR-positive samples tested, 33 (94.3%) were positive for Haemophilus, 3 (8.6%) were positive for Streptococcus, and 10 (28.6%) were positive for M. catarrhalis. Ten samples (28.6%) exhibited a mixed infection and were positive for both Haemophilus and M. catarrhalis. Culture was simultaneously performed for all 47 MEE samples. Ten of the 47 MEE samples (21.3%) exhibited bacterial growth. These 10 were PCR positive for bacterial DNA. The remaining 25 PCR-positive samples were negative by culture, thus showing about 53% discordance between PCR results and those of culture. The PCR assay proved to be more sensitive than culture, more rapid, less cumbersome, and more cost-effective than the available PCR-Southern hybridization-based assays.
我们开发并评估了一种基于两步聚合酶链反应(PCR)的检测方法,该方法使用通用引物以及属特异性或种特异性引物,用于检测黎巴嫩医院儿童中耳积液性中耳炎(OME)最常见的细菌病原体。这些病原体包括流感嗜血杆菌、链球菌和卡他莫拉菌(布兰汉菌属),它们在OME患儿的中耳积液(MEE)样本中被检测到。在为OME患儿进行鼓膜置管时,从36例患者中抽取了47份MEE样本。所有患者的积液持续时间均≥2个月。从MEE样本中提取DNA,首先使用通用引物RW01和DG74对DNA提取物进行PCR,这两个引物位于所有细菌物种16S rRNA基因中一个约370bp片段的两侧。为了鉴定特定细菌,我们在三个单独的反应混合物中使用了以下属特异性或种特异性引物:(i)一种流感嗜血杆菌特异性探针(探针RDR125)作为引物与DG74一起使用,(ii)一种链球菌特异性引物(引物STR1;由我们设计)与DG74一起使用,以及(iii)一对卡他莫拉菌特异性引物(引物对MCA1 - MCA2)。35份MEE样本(74.5%)产生了预期的370bp条带,表明测试样本中存在细菌DNA。在35份PCR阳性测试样本中,33份(94.3%)流感嗜血杆菌呈阳性,3份(8.6%)链球菌呈阳性,10份(28.6%)卡他莫拉菌呈阳性。10份样本(28.6%)表现为混合感染,流感嗜血杆菌和卡他莫拉菌均呈阳性。对所有47份MEE样本同时进行培养。47份MEE样本中有10份(21.3%)出现细菌生长。这10份样本的细菌DNA PCR呈阳性。其余25份PCR阳性样本培养结果为阴性,因此PCR结果与培养结果之间的不一致率约为53%。事实证明,与现有的基于PCR - Southern杂交的检测方法相比,PCR检测方法更灵敏、更快速、更简便且更具成本效益。
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