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Peptide nucleic acid probe detection of mutations in Mycobacterium tuberculosis genes associated with drug resistance

机译:肽核酸探针检测结核分枝杆菌基因中与耐药相关的突变

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The emergence of drug-resistant strains of Mycobacterium tuberculosis is a serious public health problem. Many of the specific gene mutations that cause drug resistance in M. tuberculosis are point mutations. We are developing a PCR-peptide nucleic acid (PNA)-based ELISA as a diagnostic method to recognize point mutations in genes associated with isoniazid and rifampin resistance in M. tuberculosis. Specific point mutation-containing sequences and wild-type sequences of cloned mycobacterial genes were PCR-amplified, denatured, and hybridized with PNA probes bound to microplate wells. Using 15-base PNA probes,, we established the hybridization temperatures (50degreesC-55degreesC) and other experimental conditions suitable for detecting clinically relevant point mutations in the katG and rpoB genes. Hybridization of PCR-amplified sequences that contained these point mutations with complementary mutation-specific PNAs resulted in significant increases in ELISA response compared with hybridization using wild-ope-specific PNAs. Conversely, PCR-amplified wild-type sequences hybridized much more efficiently with wildtype PNAs than with the mutation-specific PNAs. Using the M. tuberculosis cloned genes and PCR-PNA-ELISA format developed here, M. tuberculosis sequences containing point mutations associated with drug resistance can be identified in less than 24 h.
机译:结核分枝杆菌耐药菌株的出现是一个严重的公共卫生问题。在结核分枝杆菌中引起耐药性的许多特定基因突变是点突变。我们正在开发基于PCR肽核酸(PNA)的ELISA作为一种诊断方法,以识别结核分枝杆菌异烟肼和利福平耐药相关基因中的点突变。克隆的分枝杆菌基因的包含特定点突变的序列和野生型序列经过PCR扩增,变性并与与微孔板孔结合的PNA探针杂交。我们使用15个碱基的PNA探针,建立了适合检测katG和rpoB基因中临床相关点突变的杂交温度(50°C-55°C)和其他实验条件。与使用野生物特异性PNA杂交相比,包含这些点突变的PCR扩增序列与互补突变特异性PNA杂交导致ELISA反应显着增加。相反,PCR扩增的野生型序列与野生型PNA的杂交比与突变特异性PNA的杂交更有效。使用此处开发的结核分枝杆菌克隆基因和PCR-PNA-ELISA格式,可以在不到24小时的时间内鉴定出包含与耐药性相关的点突变的结核分枝杆菌序列。

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