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Detection by Denaturing Gradient Gel Electrophoresis of pncA Mutations Associated with Pyrazinamide Resistance in Mycobacterium tuberculosis Isolates from the United States-Mexico Border Region

机译:通过变性梯度凝胶电泳检测与美国-墨西哥边境地区分离的结核分枝杆菌中与吡嗪酰胺抗性相关的pncA突变

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摘要

Denaturing gradient gel electrophoresis (DGGE) was used to probe for mutations associated with pyrazinamide (PZA) resistance in the pncA gene of Mycobacterium tuberculosis. DGGE scans for mutations across large regions of DNA and rivals sequencing in its ability to detect DNA alterations. Specific mutations can often be recognized by their characteristic denaturation pattern, which serves as a molecular fingerprint. Five PCR target fragments were designed to scan for DNA alterations across 600 bp of pncA in 181 M. tuberculosis isolates from patients residing in the U.S-Mexico border states of Texas and Tamaulipas, respectively. A region of pncA was observed with a high GC content and a melting temperature approaching 90°C that was initially refractory to denaturation, and a DGGE target fragment was specifically designed to detect mutations in this region. DGGE detected pncA mutations in 82 of 83 PZA-resistant isolates. By contrast, only 1 of 98 PZA-susceptible isolates harbored a detectable DNA alteration. The pncA gene was sequenced from 41 isolates, and 32 DNA alterations in 32 PZA-resistant isolates were identified, including 11 new mutations. DGGE also detected nine isolates whose susceptibility to PZA appeared to be incorrect, and DNA sequencing confirmed these apparent errors in drug susceptibility testing. These results demonstrate the power and usefulness of DGGE in detecting mutations associated with PZA resistance in M. tuberculosis.
机译:变性梯度凝胶电泳(DGGE)用于检测结核分枝杆菌pncA基因中与吡嗪酰胺(PZA)抗性相关的突变。 DGGE扫描大范围DNA的突变,并在检测DNA改变的能力方面与测序相匹敌。特定突变通常可以通过其特征性的变性模式来识别,这种变性模式可以用作分子指纹。设计了五个PCR目标片段,以扫描分别来自美国德克萨斯州和塔毛利帕斯州墨西哥边境地区患者的181个结核分枝杆菌中600 bp pncA的DNA改变。观察到pncA区域具有较高的GC含量和接近90°C的熔化温度,该温度最初难以变性,并且专门设计了DGGE目标片段来检测该区域的突变。 DGGE在83个耐PZA的分离株中的82个中检测到pncA突变。相比之下,在98种PZA易感菌株中,只有1种具有可检测到的DNA改变。从41个分离株中测序出pncA基因,并鉴定了32个PZA抗性分离株中的32个DNA改变,包括11个新突变。 DGGE还检测了九种对PZA敏感性不正确的分离株,DNA测序证实了这些在药物敏感性测试中的明显错误。这些结果证明了DGGE在检测结核分枝杆菌中与PZA抗性相关的突变中的作用和实用性。

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