多重实时PCR检测脓肿分枝杆菌克拉霉素耐药基因的建立。

IF 2.4 4区 医学 Q3 MICROBIOLOGY
Carolina Salgado Pedace, Maria Gisele Gonçalves, Andréia Rodrigues Souza, Fernanda Cristina Dos Santos Simeão, Natalia Fernandes Garcia de Carvalho, Juliana Failde Gallo, Erica Chimara
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引用次数: 0

摘要

介绍。脓肿分枝杆菌分子鉴定及其耐药谱对选择正确的治疗方法具有重要意义。建立了多重实时荧光定量PCR (mqPCR)检测脓肿分枝杆菌群克拉霉素耐药基因的方法。采用Adolfo Lutz研究所2010 - 2012年接收的分离株,对hsp65基因片段(PRA-hsp65)进行PCR限制性内切酶分析,鉴定为脓肿分枝杆菌1型(n=135)和2型(n=71)。CLA药敏试验(DST)分别于第3天和第14天进行读数。采用hsp65和rpoB基因测序进行亚种鉴定,erm(41)和rrl基因进行突变检测和引物设计。常规PCR检测erm(41)基因缺失。引物和探针设计了五种检测方法:erm(41)基因全尺寸和缺失;erm(41)基因T28和C28;rrl基因a2058结果表明,191/206株(92.7%)分离株与所有方法一致,13/206株(6.3%)仅与分子方法一致。两个分离株(1.0%)与rrl基因测序结果不一致。mqPCR得到符合金标准的菌株204/206株(99.0%),考虑金标准法,灵敏度为98%,特异性为100%,考虑dst法,灵敏度为92%,特异性为93%。我们开发的mqPCR被证明是一种易于应用的工具,最大限度地减少了时间,错误和污染。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Development of multiplex real-time PCR for detection of clarithromycin resistance genes for the Mycobacterium abscessus group.

Introduction. The M. abscessus molecular identification and its drug-resistance profile are important to choose the correct therapy.Aim. This work developed a multiplex real-time PCR (mqPCR) for detection of clarithromycin resistance genes for the Mycobacterium abscessus group.Methodology. Isolates received by Adolfo Lutz Institute from 2010 to 2012, identified by PCR restriction enzyme analysis of a fragment of the hsp65 gene (PRA-hsp65) as M. abscessus type 1 (n=135) and 2 (n=71) were used. Drug susceptibility test (DST) for CLA were performed with reading on days 3 and 14. Subespecies identification by hsp65 and rpoB genes sequencing and erm(41) and rrl genes for mutation detection and primer design were performed. erm(41) gene deletion was detected by conventional PCR. Primers and probes were designed for five detections: erm(41) gene full size and with deletion; erm(41) gene T28 and C28; rrl gene A2058.Results. In total, 191/206 (92.7 %) isolates were concordant by all methods and 13/206 (6.3 %) were concordant only between molecular methods. Two isolates (1.0 %) were discordant by mqPCR compared to rrl gene sequencing. The mqPCR obtained 204/206 (99.0 %) isolates in agreement with the gold standard, with sensitivity and specificity of 98 and 100 %, respectively, considering the gold standard method and 92 and 93 % regarding DST.Conclusion. The mqPCR developed by us proved to be an easy-to-apply tool, minimizing time, errors and contamination.

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来源期刊
Journal of medical microbiology
Journal of medical microbiology 医学-微生物学
CiteScore
5.50
自引率
3.30%
发文量
143
审稿时长
4.5 months
期刊介绍: Journal of Medical Microbiology provides comprehensive coverage of medical, dental and veterinary microbiology, and infectious diseases. We welcome everything from laboratory research to clinical trials, including bacteriology, virology, mycology and parasitology. We publish articles under the following subject categories: Antimicrobial resistance; Clinical microbiology; Disease, diagnosis and diagnostics; Medical mycology; Molecular and microbial epidemiology; Microbiome and microbial ecology in health; One Health; Pathogenesis, virulence and host response; Prevention, therapy and therapeutics
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