Promoting molecular diagnostic equity: assessing in-house real-time PCR for Neisseria gonorrhoeae in anal samples from MSM recruited in an outpatient setting in Morocco.

Le infezioni in medicina Pub Date : 2024-09-01 eCollection Date: 2024-01-01 DOI:10.53854/liim-3203-9
Rokaya Aitlhaj-Mhand, Aicha Qasmaoui, Bahija Bellaji, Chaimae Remz, Reda Charof, Rachid El Jaoudi, Hanaa Abdelmoumen, Amina Hançali, Hicham Oumzil
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Abstract

Objectives: Gonorrhea is a prevalent sexually transmitted infection among men who have sex with men (MSM). In Morocco, the basic laboratory diagnosis of Neisseria gonorrhoeae (NG) is based on microscopy and, in some settings, on culture. However, no nucleic acid amplification test (NAAT) has been implemented for routine diagnosis of gonorrhoeae.The aim of this study is to assess the effectiveness of an in-house real-time PCR test for detecting N. gonorrhoeae DNA in anal swabs samples collected during an Integrated Behavioral and Biological survey.

Patients and methods: Samples from 245 MSM, recruited using a Respondent Driven Sampling, were collected and tested for NG infection using GeneXpert CT/NG assay (Cepheid, USA). An In-House real-time PCR technique targeting the pseudo gene porA was developed and used for a parallel investigation of the same infection. The reliability of the in-house RT-PCR was validated through tests of reproducibility, repeatability, limit of detection, and cross-reactivity with other bacteria. The intrinsic performance characteristics of the qRT-PCR were assessed, namely, the sensitivity, the specificity, the positive predictive value (PPV), and the negative predictive value (NPV). The GeneXpert CT/NG assay was adopted as a reference method.

Results: For N. gonorrhoeae detection, the in-house real-time PCR assay showed a sensitivity and specificity of 80% and 100%, respectively. The PPV of the assay was 100% and the NPV was 97.3%.

Conclusion: The in-house real-time PCR assay has high specificity and sensitivity, and it emerges as a promising approach for detecting N. gonorrhoeae in clinical specimens, particularly in decentralized settings such as regional laboratories.

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促进分子诊断公平:评估摩洛哥门诊男男性行为者肛门样本中淋病奈瑟菌的内部实时 PCR。
目的:淋病是男男性行为者(MSM)中一种普遍的性传播感染。在摩洛哥,淋病奈瑟菌(NG)的基本实验室诊断基于显微镜检查,在某些情况下还基于培养。本研究旨在评估一种内部实时 PCR 检测方法的有效性,该方法可用于检测在行为和生物综合调查中收集的肛拭子样本中的淋病奈瑟菌 DNA:采用受访者驱动抽样法收集了 245 名男男性行为者的样本,并使用 GeneXpert CT/NG 检测法(美国 Cepheid 公司)对样本进行了淋球菌感染检测。针对伪基因 porA 开发了一种内部实时 PCR 技术,用于对同一感染进行平行调查。通过对再现性、重复性、检测限以及与其他细菌的交叉反应进行测试,验证了内部 RT-PCR 技术的可靠性。还评估了 qRT-PCR 的内在性能特征,即灵敏度、特异性、阳性预测值 (PPV) 和阴性预测值 (NPV)。采用 GeneXpert CT/NG 检测法作为参照方法:结果:对于淋球菌的检测,内部实时 PCR 检测法的灵敏度和特异性分别为 80% 和 100%。结论:内部实时 PCR 检测的灵敏度和特异性分别为 80%和 100%,PPV 为 100%,NPV 为 97.3%:内部实时 PCR 检测法具有较高的特异性和灵敏度,是检测临床标本中淋球菌的有效方法,尤其是在地区实验室等分散环境中。
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