用于检测tcdB的商业实时荧光定量PCR检测法与细胞培养细胞毒性检测法及产毒培养法在临床样本中直接检测产毒素艰难梭菌的比较。
Comparison of a commercial real-time PCR assay for tcdB detection to a cell culture cytotoxicity assay and toxigenic culture for direct detection of toxin-producing Clostridium difficile in clinical samples.
作者信息
Stamper Paul D, Alcabasa Romina, Aird Deborah, Babiker Wisal, Wehrlin Jennifer, Ikpeama Ijeoma, Carroll Karen C
机构信息
Department of Pathology, Division of Medical Microbiology, The Johns Hopkins University School of Medicine, Baltimore, Maryland, USA.
出版信息
J Clin Microbiol. 2009 Feb;47(2):373-8. doi: 10.1128/JCM.01613-08. Epub 2008 Dec 10.
Rapid detection of toxin-producing strains of Clostridium difficile is essential for optimal management of patients with C. difficile infection. The BD GeneOhm (San Diego, CA) Cdiff assay, a real-time PCR assay that amplifies tcdB, was compared to a cell culture neutralization assay (Wampole C. difficile Toxin B [TOX-B] test; TechLab, Blacksburg, VA) and to toxigenic culture. Using liquid (n = 273) and soft (n = 131) stool specimens from 377 symptomatic patients, all testing was performed on the same day by independent laboratory staff according to the manufacturers' protocols. Toxigenic bacterial culture was performed as follows. A 0.5-ml aliquot of stool was heated to 80 degrees C for 10 min, followed by inoculation onto modified cycloserine cefoxitin fructose agar with and without horse blood (Remel, Lenexa, KS) and into prereduced chopped-meat broth. Of the 404 stool specimens tested, 340 were negative and 40 were positive (10.0% prevalence) both by PCR for tcdB and by cytotoxin production. The overall agreement between the BD GeneOhm Cdiff assay and the TOX-B test was 94.8% (380/401). When the TOX-B test was used as the reference method, the initial sensitivity, specificity, and positive and negative predictive values of the BD GeneOhm Cdiff assay were 90.9% (40/44), 95.2% (340/357), 70.2% (40/57), and 98.8% (340/344), respectively. When toxigenic culture was used as the "gold standard," the sensitivity, specificity, and positive and negative predictive values of the BD GeneOhm Cdiff assay were 83.6%, 98.2%, 89.5%, and 97.1%, respectively, and those of the TOX-B test were 67.2%, 99.1%, 93.2%, and 94.4%, respectively. PCRs for three samples were inhibited upon initial testing; one sample was resolved upon retesting. One sample produced nonspecific cytotoxin results. The BD GeneOhm Cdiff assay performed well compared to a standard cell culture neutralization assay and to toxigenic culture for the detection of toxigenic C. difficile directly from fecal specimens.
快速检测产毒素艰难梭菌菌株对于艰难梭菌感染患者的最佳治疗至关重要。将BD GeneOhm(加利福尼亚州圣地亚哥)Cdiff检测法(一种扩增tcdB的实时PCR检测法)与细胞培养中和检测法(Wampole艰难梭菌毒素B [TOX - B]检测;弗吉尼亚州布莱克斯堡的TechLab公司)以及产毒培养法进行比较。使用来自377例有症状患者的液体粪便标本(n = 273)和软便标本(n = 131),所有检测均由独立实验室工作人员在同一天按照制造商的方案进行。产毒细菌培养按如下方法进行。取0.5 ml粪便等分试样加热至80摄氏度10分钟,然后接种到含和不含马血的改良环丝氨酸头孢西丁果糖琼脂平板(Remel公司,堪萨斯州莱内克萨)以及预还原的碎肉肉汤中。在检测的404份粪便标本中,tcdB的PCR检测和细胞毒素产生检测结果均为阴性的有340份,阳性的有40份(患病率为10.0%)。BD GeneOhm Cdiff检测法与TOX - B检测法的总体一致性为94.8%(380/401)。当以TOX - B检测法作为参考方法时,BD GeneOhm Cdiff检测法的初始灵敏度、特异性、阳性预测值和阴性预测值分别为90.9%(40/44)、95.2%(340/357)、70.2%(40/57)和98.8%(340/344)。当以产毒培养法作为“金标准”时,BD GeneOhm Cdiff检测法的灵敏度、特异性、阳性预测值和阴性预测值分别为83.6%、98.2%、89.5%和97.1%,TOX - B检测法的相应值分别为67.2%、99.1%、93.2%和94.4%。最初检测时,有3份样本的PCR反应受到抑制;1份样本复测时得到解决。1份样本产生了非特异性细胞毒素结果。与标准细胞培养中和检测法和产毒培养法相比,BD GeneOhm Cdiff检测法在直接从粪便标本中检测产毒艰难梭菌方面表现良好。
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