Molecular detection of ceftriaxone resistance in Neisseria gonorrhoeae clinical specimens: a tool for public health control.

IF 3.6 3区医学 Q2 INFECTIOUS DISEASES Sexually Transmitted Infections Pub Date : 2024-07-25 DOI:10.1136/sextrans-2024-056132

Michaela Joanne Day, Dolcibella Boampong, Rachel Pitt, Aisha Bari, Monica Rebec, John Saunders, Helen Fifer, Jean Lutamyo Mbisa, Michelle Jayne Cole

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Abstract

Objectives: This study aimed to validate and implement a rapid screening assay for molecular detection of the penA-60 allele that is associated with ceftriaxone resistance in Neisseria gonorrhoeae for use on both isolate lysates and clinical specimen DNA extracts.

Methods: A N. gonorrhoeae penA real-time (RT)-PCR was adapted to include a species-specific pap confirmation target and a commercially available internal control to monitor for PCR inhibition.The modified assay was validated using N. gonorrhoeae-positive (n=24) and N. gonorrhoeae-negative (n=42) clinical specimens and isolate lysates. The panel included seven samples with resistance conferred by penA alleles targeted by the assay and four samples with different penA alleles. The feasibility of using the penA RT-PCR for molecular surveillance was assessed using clinical specimens from 54 individuals attending a London sexual health clinic who also had a N. gonorrhoeae isolate included in the 2020 Gonococcal Resistance to Antimicrobials Surveillance Programme (GRASP).

Results: The assay correctly identified N. gonorrhoeae specimens (n=7) with penA-60/64 alleles targeted by the assay. No penA false negatives/positives were detected, giving the penA target of the assay a sensitivity, specificity, positive and negative predicted values (PPV, NPV) of 100% (95% CIs; sensitivity; 56.1-100%, specificity; 93.6-100%, PPV; 56.1-100%, NPV; 93.6-100%).No cross-reactivity with other Neisseria species or other urogenital pathogens was detected. The N. gonorrhoeae target (pap) was detected in 73 out of 78 of the N. gonorrhoeae-positive specimens, resulting in 92.6% sensitivity (95% CI 83.0% to 97.3%), 100% specificity (95% CI 75.9% to 100%) and PPV, and a NPV of 89.4% (95% CI 52.5% to 90.9%). No penA-59/60/64 alleles were detected within the clinical specimens from the GRASP 2020 feasibility molecular surveillance study (n=54 individuals).

Conclusion: The implementation of this PCR assay for patient management, public health and surveillance purposes enables the rapid detection of gonococcal ceftriaxone resistance conferred by the most widely circulating penA alleles.

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淋病奈瑟菌临床样本中头孢曲松耐药性的分子检测：公共卫生控制工具。

研究目的本研究旨在验证和实施一种快速筛查检测方法，用于分子检测淋病奈瑟菌中与头孢曲松耐药性相关的 penA-60 等位基因，既可用于分离裂解物，也可用于临床标本 DNA 提取物：采用淋病奈瑟菌阳性（n=24）和淋病奈瑟菌阴性（n=42）临床标本和分离株裂解物对改进后的检测方法进行了验证。该检测组包括 7 份由该检测方法所针对的 penA 等位基因产生耐药性的样本和 4 份具有不同 penA 等位基因的样本。使用伦敦一家性健康诊所 54 名就诊者的临床标本评估了使用 penA RT-PCR 进行分子监测的可行性，这些就诊者的淋球菌分离物也被纳入了 2020 年淋球菌对抗菌药耐药性监测计划（GRASP）：结果：该检测方法正确鉴定出了具有该检测方法所针对的penA-60/64等位基因的淋球菌标本（n=7）。未发现 penA 假阴性/阳性，因此该检测方法的 penA 目标敏感性、特异性、阳性和阴性预测值（PPV、NPV）均为 100%（95% CIs；敏感性；56.1-100%，特异性；93.6-100%，PPV；56.1-100%，NPV；93.6-100%）。在 78 份淋球菌阳性标本中，有 73 份检测到了淋球菌靶标（pap），灵敏度为 92.6%（95% CI 83.0% 至 97.3%），特异性为 100%（95% CI 75.9% 至 100%），PPV 为 89.4%（95% CI 52.5% 至 90.9%）。在GRASP 2020可行性分子监测研究的临床样本（n=54人）中未检测到penA-59/60/64等位基因：结论：为患者管理、公共卫生和监测目的而实施的这一 PCR 检测可快速检测由最广泛流行的 penA 等位基因产生的淋球菌头孢曲松耐药性。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Sexually Transmitted Infections 医学-传染病学

CiteScore

5.70

自引率

8.30%

发文量

审稿时长

4-8 weeks

期刊介绍： Sexually Transmitted Infections is the world’s longest running international journal on sexual health. It aims to keep practitioners, trainees and researchers up to date in the prevention, diagnosis and treatment of all STIs and HIV. The journal publishes original research, descriptive epidemiology, evidence-based reviews and comment on the clinical, public health, sociological and laboratory aspects of sexual health from around the world. We also publish educational articles, letters and other material of interest to readers, along with podcasts and other online material. STI provides a high quality editorial service from submission to publication.