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利用高分辨率熔解曲线PCR分析通过rpoB基因扫描快速鉴定耐多药结核分枝杆菌分离株

Rapid identification of multidrug-resistant Mycobacterium tuberculosis isolates by rpoB gene scanning using high-resolution melting curve PCR analysis.

作者信息

Pietzka Ariane T, Indra Alexander, Stöger Anna, Zeinzinger Josef, Konrad Miriam, Hasenberger Petra, Allerberger Franz, Ruppitsch Werner

机构信息

Austrian Agency for Health and Food Safety, Vienna, Austria.

出版信息

J Antimicrob Chemother. 2009 Jun;63(6):1121-7. doi: 10.1093/jac/dkp124. Epub 2009 Apr 15.

Abstract

BACKGROUND

Multidrug-resistant (MDR) Mycobacterium tuberculosis poses a serious threat to the control of tuberculosis (TB) and constitutes an increasing public health problem. The availability of rapid in vitro susceptibility tests is a prerequisite for optimal patient treatment. Rifampicin resistance caused by diverse mutations in the rpoB gene is an established and widely used surrogate marker for MDR-TB. We used a high-resolution melting (HRM) curve analysis approach to scan for mutations in the rpoB gene.

METHODS

A total of 49 MDR-TB and 19 fully susceptible non-MDR-TB isolates, as determined by conventional drug susceptibility testing using the BACTEC-MGIT960 system, were used to evaluate the suitability of HRM curve analysis as a rapid and accurate screening system for rifampicin resistance.

RESULTS

HRM analysis of the rpoB cluster I site allowed the correct allocation of 44 of the 49 MDR-TB isolates and all non-MDR-TB isolates. Three of the five MDR-TB isolates (60%) falsely identified as non-MDR-TB harboured the V176F mutation that could be specifically detected by an additional HRM assay. The combined HRM analysis of all strains and isolates exhibited 95.9% sensitivity and 100% specificity.

CONCLUSIONS

With a positive predictive value of 100% and a negative predictive value of at least 99.9%, this combined HRM curve analysis is an ideal screening method for the TB laboratory, with minimal requirements of cost and time. The method is a closed-tube assay that can be performed in an interchangeable 96- or 384-well microplate format enabling a rapid, reliable, simple and cost-effective handling of even large sample numbers.

摘要

背景

耐多药结核分枝杆菌对结核病的控制构成严重威胁,且公共卫生问题日益严峻。开展快速体外药敏试验是实现患者最佳治疗的前提条件。rpoB基因的多种突变导致的利福平耐药是耐多药结核病公认且广泛应用的替代标志物。我们采用高分辨率熔解(HRM)曲线分析方法筛查rpoB基因中的突变。

方法

使用BACTEC-MGIT960系统通过常规药敏试验确定的49株耐多药结核菌株和19株完全敏感的非耐多药结核菌株,用于评估HRM曲线分析作为利福平耐药快速准确筛查系统的适用性。

结果

对rpoB基因簇I位点进行HRM分析,可正确区分49株耐多药结核菌株中的44株以及所有非耐多药结核菌株。5株被误判为非耐多药结核的耐多药结核菌株中有3株(60%)携带V176F突变,可通过额外的HRM检测特异性检出。对所有菌株和分离株进行的联合HRM分析显示敏感性为95.9%,特异性为100%。

结论

这种联合HRM曲线分析的阳性预测值为100%,阴性预测值至少为99.9%,是结核病实验室理想的筛查方法,成本和时间要求极低。该方法为闭管检测,可在96孔或384孔微孔板中进行,即使样本数量众多也能实现快速、可靠、简便且经济高效的处理。

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