Simple, rapid, and inexpensive detection of Neisseria gonorrhoeae resistance mechanisms using heat-denatured isolates and SYBR green-based real-time PCR.

Kugelman G; Tapsall JW; Goire N

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Simple, rapid, and inexpensive detection of Neisseria gonorrhoeae resistance mechanisms using heat-denatured isolates and SYBR green-based real-time PCR.

机译：使用热变性分离物和基于SYBR Green的实时PCR简便，快速且廉价地检测淋病奈瑟菌。

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Neisseria gonorrhoeae has developed resistance to multiple classes of antimicrobials. There is now growing concern that without the availability of appropriate public health strategies to combat this problem, gonorrhea could become untreatable. For this reason, surveillance for gonococcal antimicrobial resistance must be optimal both in terms of obtaining a representative sample of gonococcal isolates and in terms of having the appropriate tools to identify resistance. To aid with this surveillance, molecular tools are increasingly being used. In the present study, we investigated the use of a simple heat denaturation protocol for isolate DNA preparation combined with SYBR green-based real-time PCR for the identification of mutations associated with N. gonorrhoeae antimicrobial resistance. A total of 109 clinical gonococcal isolates were tested by high-resolution melting (HRM) curve analysis for chromosomal mutations associated with gonococcal resistance to beta-lactam antibiotics: a penA 345A insertion, ponA L421P, mtrR G45D, substitutions at positions 120 and 121 in porB1b, and an adenine deletion in the mtrR promoter. An allele-specific PCR assay was also investigated for its ability to detect the adenine deletion in the mtrR promoter. The results were compared to those obtained by DNA sequencing. Our HRM assays provided the accurate discrimination of heat-treated isolates in which the sequence types differed in GC content, including isolates with the penA 345A insertion and the ponA L421P and mtrR G45D mutations. The allele-specific PCR assay accurately identified isolates with the adenine deletion in the mtrR promoter. Heat-denatured DNA combined with SYBR green-based real-time PCR offers a simple, rapid, and inexpensive means of detecting gonococcal resistance mechanisms. These methods may have broader application in the detection of polymorphisms associated with phenotypes of interest.

机译：淋病奈瑟氏球菌对多种抗菌素产生了抗药性。现在，人们越来越担心，如果没有适当的公共卫生策略来解决这个问题，淋病就可能变得无法治愈。因此，从获得代表性的淋球菌分离物样本和具有合适的工具识别耐药性方面，对淋球菌抗药性的监测必须是最佳的。为了帮助进行这种监视，越来越多地使用分子工具。在本研究中，我们调查了简单的热变性方案用于分离DNA制备与基于SYBR Green的实时PCR结合鉴定淋病奈瑟氏球菌抗药性相关突变的用途。通过高分辨率熔解（HRM）曲线分析测试了总共109个临床淋球菌分离株，以检测与淋球菌对β-内酰胺抗生素耐药相关的染色体突变：penA 345A插入，ponA L421P，mtrR G45D，在120和121位的替代porB1b和mtrR启动子中的腺嘌呤缺失。还研究了等位基因特异性PCR分析检测mtrR启动子中腺嘌呤缺失的能力。将结果与通过DNA测序获得的结果进行比较。我们的HRM分析可准确区分序列类型在GC含量上不同的热处理分离株，包括带有penA 345A插入序列以及ponA L421P和mtrR G45D突变的分离株。等位基因特异性PCR检测可准确鉴定出mtrR启动子中腺嘌呤缺失的分离株。热变性DNA与基于SYBR Green的实时PCR结合提供了一种检测淋球菌耐药机制的简单，快速且廉价的方法。这些方法在检测与目标表型相关的多态性方面可能具有更广泛的应用。

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《Antimicrobial agents and chemotherapy.》 |2009年第10期|共6页
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Kugelman G; Tapsall JW; Goire N;
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1. Simple, rapid, and inexpensive detection of Neisseria gonorrhoeae resistance mechanisms using heat-denatured isolates and SYBR green-based real-time PCR. [J] . Kugelman G, Tapsall JW, Goire N Antimicrobial agents and chemotherapy. . 2009,第10期

机译：使用热变性分离物和基于SYBR Green的实时PCR简便，快速且廉价地检测淋病奈瑟菌。
2. Development of a SYBR green-based real-time RT-PCR assay for rapid detection of the emerging swine acute diarrhea syndrome coronavirus [J] . Ma Lei, Zeng Fanwen, Cong Feng, Journal of Virological Methods . 2019,第期

机译：开发SYBR绿色实时RT-PCR测定，用于快速检测新出现的猪急性腹泻综合征冠状病毒
3. Rapid and Specific Detection of Acidovorax avenae subsp citrulli Using SYBR Green-Based Real-Time PCR Amplification of the YD-Repeat Protein Gene [J] . Cho Min Seok, Park Duck Hwan, Ahn Tae-Young, Journal of microbiology and biotechnology . 2015,第9期

机译：YD-重复蛋白基因的基于SYBR Green的实时PCR扩增可快速，特异地检测酸果蝇
4. Rapid detection of antibiotic resistance mechanisms and toxin screening: a new application of SRM/MRM for the clinical microbiology laboratory [C] . Y. Charretier, C. Franceschi, O. Dauwalder, American Society for Mass Spectrometry Conference on Mass Spectrometry and Allied Topics . 2012

机译：快速检测抗生素抗性机制和毒素筛选：SRM / MRM对临床微生物实验室的新应用
5. A rapid method for detecting single nucleotide polymorphisms using antimicrobial resistance in Neisseria gonorrhoeae as a model. [D] . Cullingham, Kyle J. G. 2005

机译：一种使用淋病奈瑟氏菌为模型的抗药性检测单核苷酸多态性的快速方法。
6. Simple Rapid and Inexpensive Detection of Neisseria gonorrhoeae Resistance Mechanisms Using Heat-Denatured Isolates and SYBR Green-Based Real-Time PCR [O] . Gayle Kugelman, John W. Tapsall, Namraj Goire, 2009

机译：使用热变性分离物和基于SYBR Green的实时PCR简便快速且廉价地检测淋病奈瑟菌
7. Simple, rapid, and inexpensive detection of Neisseria gonorrhoeae resistance mechanisms using heat-denatured isolates and SYBR green-based real-time PCR. [O] . Kugelman Gayle, Tapsall John W., Goire Namraj, 2009

机译：使用热变性分离物和基于SYBR Green的实时PCR简便，快速且廉价地检测淋病奈瑟菌。
8. Novel Mechanism of High-Level, Broad-Spectrum Antibiotic Resistance Caused by a Single Base Pair Change in Neisseria gonorrhoeae [R] . Ohneck, E. A., Zalucki, Y. M., Johnson, P. J., 2011

机译：淋病奈瑟菌单碱基对变化引起的高水平，广谱抗生素耐药的新机制

Simple, rapid, and inexpensive detection of Neisseria gonorrhoeae resistance mechanisms using heat-denatured isolates and SYBR green-based real-time PCR.

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