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Peptide Nucleic Acid Probe-Based Analysis as a New Detection Method for Clarithromycin Resistance in Helicobacter pylori

机译:基于肽核酸探针的分析法检测幽门螺杆菌对克拉霉素的耐药性

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Background/Aims Helicobacter pylori eradication rates are decreasing because of increases in clarithromycin resistance. Thus, finding an easy and accurate method of detecting clarithromycin resistance is important. Methods We evaluated 70 H. pylori isolates from Korean patients. Dual-labeled peptide nucleic acid (PNA) probes were designed to detect resistance associated with point mutations in 23S ribosomal ribonucleic acid gene domain V (A2142G, A2143G, and T2182C). Data were analyzed by probe-based fluorescence melting curve analysis based on probe-target dissociation temperatures and compared with Sanger sequencing. Results Among 70 H. pylori isolates, 0, 16, and 58 isolates contained A2142G, A2143G, and T2182C mutations, respectively. PNA probe-based analysis exhibited 100.0% positive predictive values for A2142G and A2143G and a 98.3% positive predictive value for T2182C. PNA probe-based analysis results correlated with 98.6% of Sanger sequencing results (κ-value=0.990; standard error, 0.010). Conclusions H. pylori clarithromycin resistance can be easily and accurately assessed by dual-labeled PNA probe-based melting curve analysis if probes are used based on the appropriate resistance-related mutations. This method is fast, simple, accurate, and adaptable for clinical samples. It may help clinicians choose a precise eradication regimen.
机译:背景/目的由于对克拉霉素的耐药性增加,幽门螺杆菌的根除率正在降低。因此,找到一种简便而准确的克拉霉素耐药性检测方法很重要。方法我们评估了来自韩国患者的70例幽门螺杆菌分离株。设计双标记肽核酸(PNA)探针以检测与23S核糖体核糖核酸基因域V(A2142G,A2143G和T2182C)中的点突变相关的抗性。通过基于探针目标解离温度的基于探针的荧光解链曲线分析来分析数据,并与Sanger测序进行比较。结果在70株幽门螺杆菌中,0、16和58株分别含有A2142G,A2143G和T2182C突变。基于PNA探针的分析显示A2142G和A2143G的阳性预测值为100.0%,T2182C的阳性预测值为98.3%。基于PNA探针的分析结果与Sanger测序结果的98.6%相关(κ值= 0.990;标准误,0.010)。结论如果使用基于适当耐药性相关突变的探针,可通过基于双标记PNA探针的解链曲线分析轻松而准确地评估幽门螺杆菌克拉霉素的耐药性。该方法快速,简单,准确,并且适​​用于临床样品。它可以帮助临床医生选择精确的根除方案。

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