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Preventing false positives: quantitative evaluation of three protocols for inactivation of polymerase chain reaction amplification products.防止假阳性:三种聚合酶链反应扩增产物灭活方案的定量评估
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基于多重聚合酶链反应的鼻咽拭子标本中百日咳博德特氏菌检测方法

Multiplex PCR-based assay for detection of Bordetella pertussis in nasopharyngeal swab specimens.

作者信息

Wadowsky R M, Michaels R H, Libert T, Kingsley L A, Ehrlich G D

机构信息

Department of Otolaryngology, School of Medicine, University of Pittsburgh, Pennsylvania 15261, USA.

出版信息

J Clin Microbiol. 1996 Nov;34(11):2645-9. doi: 10.1128/jcm.34.11.2645-2649.1996.

DOI:10.1128/jcm.34.11.2645-2649.1996
PMID:8897157
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC229378/
Abstract

A multiplex PCR-based assay was developed for the detection of Bordetella pertussis in nasopharyngeal swab specimens. The assay simultaneously amplified two separate DNA targets (153 and 203 bp) within a B. pertussis repetitive element and a 438-bp target within the beta-actin gene of human DNA (PCR amplification control). PCR products were detected by a sensitive and specific liquid hybridization gel retardation assay. A total of 496 paired nasopharyngeal swab specimens were tested by both the PCR-based assay and culture. Although 30 (6%) of the specimens inhibited the amplification of the beta-actin target, in all 29 specimens studied, the inhibition disappeared on repeat testing or was easily overcome with a 1:8 dilution or less of specimen digest. Of the 495 specimen pairs yielding a final evaluable result by the PCR-based assay, 19.0% were positive by the PCR-based assay, whereas 13.9% were positive by culture (P < 0.0001). After resolving the PCR-positive, culture-negative results by testing an additional aliquot from these specimens by the multiplex PCR-based assay, the PCR-based assay had a sensitivity and specificity of 98.9 and 99.7%, respectively, compared with values of 73.4 and 100%, respectively, for culture. In comparison with patients with culture-confirmed pertussis, those with PCR-positive, culture-negative results were older and more likely to have had prolonged cough, immunization with pertussis vaccine, or treatment with erythromycin. This multiplex PCR-based assay is substantially more sensitive than culture and identifies specimens that contain inhibitors of PCR.

摘要

开发了一种基于多重PCR的检测方法,用于检测鼻咽拭子标本中的百日咳博德特氏菌。该检测方法同时扩增百日咳博德特氏菌重复元件内的两个独立DNA靶标(153和203 bp)以及人类DNAβ-肌动蛋白基因内的一个438 bp靶标(PCR扩增对照)。通过灵敏且特异的液相杂交凝胶阻滞试验检测PCR产物。共对496对鼻咽拭子标本进行了基于PCR的检测方法和培养检测。尽管30份(6%)标本抑制了β-肌动蛋白靶标的扩增,但在所有研究的29份标本中,重复检测时抑制作用消失,或者通过1:8或更低稀释度的标本消化液很容易克服抑制作用。在通过基于PCR的检测方法得出最终可评估结果的495对标本中,基于PCR的检测方法有19.0%呈阳性,而培养检测有13.9%呈阳性(P<0.0001)。通过基于多重PCR的检测方法对这些标本的额外一份样品进行检测以解决PCR阳性、培养阴性的结果后,基于PCR的检测方法的灵敏度和特异性分别为98.9%和99.7%,而培养检测的灵敏度和特异性分别为73.4%和100%。与培养确诊为百日咳的患者相比,PCR阳性、培养阴性结果的患者年龄更大,更有可能有长期咳嗽、接种过百日咳疫苗或接受过红霉素治疗。这种基于多重PCR的检测方法比培养检测灵敏得多,并且能够识别含有PCR抑制剂的标本。