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Clostridium difficile infection diagnosis in a paediatric population: Comparison of methodologies

机译:小儿难辨梭状芽胞杆菌感染的诊断:方法学比较

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The increasing incidence of Clostridium difficile infection (CDI) in paediatric hospitalised populations, combined with the emergence of hypervirulent strains, community-acquired CDI and the need for prompt treatment and infection control, makes the rapid, accurate diagnosis of CDI crucial. We validated commonly used C. difficile diagnostic tests in a paediatric hospital population. From October 2011 to January 2012, 150 consecutive stools were collected from 75 patients at a tertiary paediatric hospital in Perth, Western Australia. Stools were tested using: C. Diff Quik Chek Complete, Illumigene C. difficile, GeneOhm Cdiff, cycloserine cefoxitin fructose agar (CCFA) culture, and cell culture cytotoxin neutralisation assay (CCNA). The reference standard was growth on CCFA or Cdiff Chromagar and PCR on isolates to detect tcdA, tcdB, cdtA, and cdtB. Isolates were PCR ribotyped. The prevalence of CDI was high (43 % of patients). Quik Chek Complete glutamate dehydrogenase (GDH) demonstrated a low negative predictive value (NPV) (93 %). Both CCNA and Quik Chek Complete toxin A/B had poor sensitivity (33 % and 29 % respectively). Molecular methods both had 89 % sensitivity. Algorithms using GDH + Illumigene or GeneOhm reduced the sensitivity to 85 % and 83 % respectively. Ribotype UK014/20 predominated. GDH NPV and GeneOhm and Illumigene sensitivities were reduced compared with adult studies. Quik Chek Complete and CCNA cannot reliably detect toxigenic CDI. A GDH first algorithm showed reduced sensitivity. In a high prevalence paediatric population, molecular methods alone are recommended over the use of GDH algorithm or culture and CCNA, as they demonstrate the best test performance characteristics.
机译:在儿科住院患者中,难辨梭状芽胞杆菌感染(CDI)的发病率不断增加,再加上出现高毒力菌株,社区获得的CDI以及对及时治疗和感染控制的需求,使得快速,准确地诊断CDI至关重要。我们验证了儿科医院人群中常用的艰难梭菌诊断测试。 2011年10月至2012年1月,在西澳大利亚州珀斯的一家三级儿科医院从75例患者中收集了150份连续大便。使用以下方法测试凳子:C. Diff Quik Chek Complete,艰难梭菌Illumigene C.,GeneOhm Cdiff,环丝氨酸头孢西丁果糖琼脂(CCFA)培养物和细胞培养物细胞毒素中和测定(CCNA)。参考标准是在CCFA或Cdiff Chromagar上生长,在分离株上进行PCR检测tcdA,tcdB,cdtA和cdtB。对分离物进行PCR核糖分型。 CDI的患病率很高(43%的患者)。 Quik Chek完全谷氨酸脱氢酶(GDH)显示出较低的阴性预测值(NPV)(93%)。 CCNA和Quik Chek Complete毒素A / B的敏感性均较差(分别为33%和29%)。分子方法均具有89%的灵敏度。使用GDH + Illumigene或GeneOhm的算法分别将灵敏度降低到85%和83%。核型UK014 / 20占主导。与成人研究相比,GDH NPV和GeneOhm和Illumigene的敏感性降低。 Quik Chek Complete和CCNA无法可靠地检测出有毒的CDI。 GDH优先算法显示出降低的灵敏度。在儿童患病率较高的人群中,建议分子方法优于使用GDH算法或培养物和CCNA,因为它们证明了最佳的测试性能特征。

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