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PCR-Based Diagnosis of Helicobacter pylori Infection and Real-Time Determination of Clarithromycin Resistance Directly from Human Gastric Biopsy Samples

机译:直接基于人类胃活检样本的基于PCR的幽门螺杆菌感染诊断和克拉霉素抗性的实时测定

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摘要

A novel PCR detection assay that amplifies the Helicobacter pylori-specific vacuolating cytotoxin gene (vacA) and thus enables rapid diagnosis of infection is described. Additionally, a real-time probe hybridization melting point analysis assay to detect all three mutations in the 23S rRNA gene associated with clarithromycin resistance was applied directly to antral gastric biopsy samples. Comparison with culture and an alternative PCR assay targeting the 16S rrn gene showed that the vacA assay was sensitive and specific when tested on biopsy samples from 121 patients. Clarithromycin susceptibilities could be determined in the majority (92.3%) of culture-positive gastric biopsy samples analyzed, four of which generated melting peaks indicative of clarithromycin resistance by either an A→G or A→C mutation. The presence of the mutations correlated with the clarithromycin disk diffusion sensitivities of matched cultures. This PCR-based system was simple to perform and could be completed in 3 to 4 h, thereby overcoming the delays associated with conventional culture methods for H. pylori identification and susceptibility testing.
机译:描述了一种新颖的PCR检测方法,可扩增幽门螺杆菌特异性空泡细胞毒素基因(vacA),从而能够快速诊断感染。此外,将实时探针杂交熔点分析法检测与克拉霉素抗性相关的23S rRNA基因中的所有三个突变直接应用于胃窦胃活检样品。与培养物和针对16S rrn基因的另一种PCR检测方法的比较表明,对来自121例患者的活检样品进行测试时,vacA检测方法既灵敏又特异性。可以在分析的大部分培养阳性胃活检样本中确定克拉霉素敏感性,其中四个样本通过A→G或A→C突变产生了对克拉霉素耐药的熔解峰。突变的存在与匹配培养物的克拉霉素盘扩散敏感性相关。这种基于PCR的系统操作简单,可在3-4小时内完成,从而克服了幽门螺杆菌鉴定和药敏试验的常规培养方法带来的延迟。

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