聚合酶链反应-限制性片段长度多态性快速检测乙胺丁醇敏感性及广泛耐药结核临床分离株分子预测的性能评价

The West Indian medical journal Pub Date : 2015-06-12 DOI:10.7727/wimj.2014.022

M. Arjomandzadegan, R. Nazari, M. Zolfaghari, M. Taherahmadi, M. Sadrnia, L. Titov, A. Ahmadi, M. Shojapoor

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引用次数: 1

摘要

采用聚合酶链反应-限制性片段长度多态性(PCR-RFLP)方法快速检测结核分枝杆菌乙胺丁醇(EMB)耐药临床分离株。材料与方法从182株不同地区结核分枝杆菌临床分离株中抽取103株进行调查。采用Chelex 100法提取DNA，用特异性引物对embB基因进行PCR。用HaeIII和NlaII酶切酶切聚合酶链反应产物，分析酶切片段模式。对一些随机选择的样本进行测序。结果103株菌株中，52株对EMB耐药。继发性肺结核53例(51.50±1.77%)，原发肺结核50例(48.50±1.77%);P < 0.05)。63株广泛耐药(XDR)、XDR前耐药(pre-XDR)和多药耐药(MDR)分离株中，EMB耐药菌株分别为27株(87%)、18株(81.8%)和7株(70%)。结果PCR-RFLP方法显示，27R EMB XDR分离株中有13株(灵敏度48%，CI分别为0.307和0.66，特异性100%)，18R EMB XDR前分离株中有4株(灵敏度22%，CI分别为0.09和0.45，特异性100%)，7R EMB MDR分离株中有2株(灵敏度28%，CI分别为0.082和0.64，特异性100%)存在ATG-Met密码子306突变。测序结果与RFLP法一致。总体而言，分子方法的敏感性为36.5% (CI: 0.09, 0.45)，特异性为100%。40株全感毒株均为embB306突变株。广泛耐药菌株的embB306突变体比例(43%)高于前xdr和MDR分离株(优势比6.78;P < 0.001)。结论PCR-RFLP法可快速检测EMB药物的药敏。embB306位点是利用该方法快速预测耐多药和广泛耐药菌株对抗结核药物高耐药性的候选标记。

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Performance Assessment of the Polymerase Chain Reaction-Restriction Fragment Length Polymorphism Method for Rapid Detection of Susceptibility to Ethambutol and Molecular Prediction of Extensively Drug-resistant Tuberculosis in Clinical Isolates of Mycobacterium tuberculosis.

INTRODUCTION The polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) method was employed for rapid detection of ethambutol (EMB) resistant clinical isolates of Mycobacterium tuberculosis. MATERIALS AND METHODS From 182 clinical isolates of M tuberculosis collected from different regions, 103 strains were entered in the investigation. DNA was extracted by Chelex 100 method and PCR was performed using specific primers for embB gene. Polymerase chain reaction products were digested with HaeIII and NlaII restriction endonucleases and the patterns of restriction fragments were analysed. Some randomly selected samples were sequenced. RESULTS Out of 103 studied strains, 52 were resistant to EMB. The cases of secondary tuberculosis were 53 (51.50 ± 1.77%), and primary cases 50 (48.50 ± 1.77%; p > 0.05). From 63 extensively drug-resistant (XDR), pre-XDR and multidrug-resistant (MDR) isolates, 27 (87%), 18 (81.8%) and 7 (70%) strains were resistant to EMB, respectively. Results of PCR-RFLP method showed that from 27R EMB XDR isolates, 13 (sensitivity 48% with CI: 0.307, 0.66 and specificity 100%), from 18R EMB pre-XDR strains, 4 (sensitivity 22% with CI: 0.09, 0.45 and specificity 100%) and of 7R EMB MDR, 2 (sensitivity 28% with CI: 0.082, 0.64 and specificity 100%) had mutation in ATG-Met codon 306. Results of sequencing were concordant with RFLP method. Overall, sensitivity of the molecular method was 36.5% (CI: 0.09, 0.45) and specificity 100%. None of the 40 pansusceptible strains was embB306 mutants. Extensively drug-resistant strains had a higher proportion of embB306 mutants (43%) than pre-XDR and MDR isolates (odds ratio 6.78; p < 0.001). CONCLUSION Fast detection of susceptibility to EMB drug is possible by PCR-RFLP. The embB306 locus is a candidate marker for rapid prediction of high resistance consisting of MDR and XDR forms to anti-tuberculosis drugs using this method.

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The West Indian medical journal

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