Division of Microbiology, St. Vincent's Hospital, Darlinghurst, NSW, Australia.
Eur J Clin Microbiol Infect Dis. 2010 Apr;29(4):411-6. doi: 10.1007/s10096-010-0876-4. Epub 2010 Feb 14.
Dientamoeba fragilis is a pathogenic protozoan parasite that is notoriously difficult to diagnose. The aim of this study was to determine the gold standard for laboratory detection of D. fragilis. A total of 650 human faecal samples were included in the study. All specimens underwent the following: microscopy using a permanent stain (modified iron-haematoxylin), culture using a modified Boeck and Drbohlav's medium (MBD) and TYGM-9, a conventional polymerase chain reaction (PCR) and a real-time PCR (RT-PCR). The overall prevalence of D. fragilis in the study population was 5.4% (35/650). RT-PCR detected 35 isolates, conventional PCR detected 15 isolates, MBD culture detected 14 isolates, TYGM-9 detected ten isolates, while microscopy detected 12 isolates. RT-PCR detected an additional 15 positive samples compared to the other diagnostic methods, all of which were confirmed by sequencing. When all methods were compared to each other, RT-PCR showed a sensitivity and specificity of 100 and 100%, conventional PCR 42.9 and 100%, MBD culture 40 and 100%, TYGM-9 culture 28.6 and 100%, and microscopy 34.3 and 99%, respectively. These results show that RT-PCR is the diagnostic method of choice for the detection of D. fragilis in clinical samples and, as such, should be considered as the gold standard for diagnosis.
脆弱双核阿米巴是一种具有致病性的原生动物寄生虫,其诊断极具挑战性。本研究旨在确定脆弱双核阿米巴检测的金标准方法。共有 650 个人类粪便样本纳入研究。所有标本均接受以下检查:使用永久染色剂(改良铁苏木精)进行显微镜检查、使用改良 Boeck 和 Drbohlav 培养基(MBD)和 TYGM-9 进行培养、常规聚合酶链反应(PCR)和实时 PCR(RT-PCR)。研究人群中脆弱双核阿米巴的总体流行率为 5.4%(35/650)。RT-PCR 检测到 35 个分离株,常规 PCR 检测到 15 个分离株,MBD 培养检测到 14 个分离株,TYGM-9 培养检测到 10 个分离株,而显微镜检查检测到 12 个分离株。与其他诊断方法相比,RT-PCR 检测到额外的 15 个阳性样本,所有样本均通过测序确认。当所有方法相互比较时,RT-PCR 的灵敏度和特异性分别为 100%和 100%,常规 PCR 为 42.9%和 100%,MBD 培养为 40%和 100%,TYGM-9 培养为 28.6%和 100%,显微镜检查为 34.3%和 99%。这些结果表明,RT-PCR 是检测临床样本中脆弱双核阿米巴的首选诊断方法,因此应被视为诊断的金标准。
