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Optimization of a Nucleic Acid-Based Reporter System To Detect Mycobacterium tuberculosis Antibiotic Sensitivity

机译:基于核酸的报告基因系统检测结核分枝杆菌抗生素敏感性的优化

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摘要

We previously reported the development of a prototype antibiotic sensitivity assay to detect drug-resistant Mycobacterium tuberculosis using infection by mycobacteriophage to create a novel nucleic acid transcript, a surrogate marker of mycobacterial viability, detected by reverse transcriptase PCR (M. C. Mulvey et al., mBio >3:e00312-11, 2012). This assay detects antibiotic resistance to all drugs, even drugs for which the resistance mechanism is unknown or complex: it is a phenotypic readout using nucleic acid detection. In this report, we describe development and characteristics of an optimized reporter system that directed expression of the RNA cyclase ribozyme, which generated circular RNA through an intramolecular splicing reaction and led to accumulation of a new nucleic acid sequence in phage-infected bacteria. These modifications simplified the assay, increased the limit of detection from 104 to <102 M. tuberculosis cells, and correctly identified the susceptibility profile of M. tuberculosis strains exposed for 16 h to either first-line or second-line antitubercular drugs. In addition to phenotypic drug resistance or susceptibility, the assay reported streptomycin MICs and clearly detected 10% drug-resistant cells in an otherwise drug-susceptible population.
机译:我们之前曾报道过使用抗生素分枝杆菌感染来创建耐药性结核分枝杆菌的抗生素敏感性试验原型的开发方法,该技术可通过逆转录酶PCR(MC Mulvey等人,mBio)检测到一种新的核酸转录物,即分枝杆菌生存力的替代标记。 > 3: e00312-11,2012)。该测定法可检测对所有药物的抗生素耐药性,即使耐药机制未知或复杂的药物也是如此:这是使用核酸检测的表型读数。在本报告中,我们描述了定向RNA环化酶核酶的表达的优化报告系统的发展和特征,该酶通过分子内剪接反应产生环状RNA,并在噬菌体感染的细菌中积累了新的核酸序列。这些修饰简化了测定过程,将检出限从10 4 增加到<10 2 结核分枝杆菌细胞,并正确鉴定了暴露于结核分枝杆菌的结核分枝杆菌菌株的敏感性。一线或二线抗结核药物治疗16小时。除表型耐药或易感性外,该检测方法还报告了链霉素MIC,并清楚地检测出在其他易感人群中的10%耐药细胞。

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