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影响淋病奈瑟菌分子检测阳性确认的因素。

Factors That Influence Confirmation of Neisseria gonorrhoeae Positivity by Molecular Methods.

机构信息

Department of Laboratory Medicine, Royal Infirmary of Edinburgh, NHS Lothian, Edinburgh, United Kingdom

Department of Laboratory Medicine, Royal Infirmary of Edinburgh, NHS Lothian, Edinburgh, United Kingdom.

出版信息

J Clin Microbiol. 2019 May 24;57(6). doi: 10.1128/JCM.02068-18. Print 2019 Jun.

Abstract

Several nucleic acid amplification tests (NAATs) with high sensitivity exist. However, the specificity of NAATs may be suboptimal, particularly for extragenital biospecimens. Consequently, confirmation with a second NAAT is common, although this represents a burden on resources. Furthermore, the rationale for confirmation is contentious. The objective of this work was to assess confirmation in over 13,000 screen-positive samples representing various biospecimens and three separate screening assays, the Abbott RealTime CT/NG (Abbott Molecular, Inc., Des Plaines, IL), the Cobas CT/NG test (Roche Molecular Systems Inc., Alameda, CA), and the BD ProbeTec ET CT/GC amplified DNA assay (BD Diagnostics, Sparks, MD). Factors predictive of confirmation were determined via logistic regression involving sex, year, whether the sample was formally validated, and sample site. Level of confirmation varied according to screening assay (96.2%, 86.0%, and 73.9% for the Abbott, Roche, and BD tests, respectively) in sample types formally included according to the manufacturers' instructions (i.e., validated). Sex did not affect confirmation for 2/3 assays, and the likelihood of confirmation of samples not formally included in manufacturer instructions (i.e., nonvalidated) was 89.1%, 82.1%, and 59.2% for the Abbott, Roche, and BD tests, respectively. Rectal swabs, which are nonvalidated samples, confirmed in 91.5%, 90.1%, and 87.4% of samples initially tested with the respective assays. The requirement to confirm in validated samples is not required for all NAATs, although initial assay-specific evaluation is justified given observed variability. Rectal samples represent robust biospecimens for NAAT testing and may not require confirmation when screened with the assays described.

摘要

有几种高灵敏度的核酸扩增检测(NAAT)。然而,NAAT 的特异性可能不够理想,特别是对于外生殖器生物标本。因此,常用第二种 NAAT 进行确认,尽管这对资源构成了负担。此外,确认的基本原理存在争议。本研究的目的是评估在代表各种生物标本和三种单独筛查检测的 13000 多个筛查阳性样本中进行确认的情况,这三种检测分别是 Abbott RealTime CT/NG(雅培分子公司,德斯普兰斯,IL)、Cobas CT/NG 检测(罗氏分子系统公司,阿拉米达,CA)和 BD ProbeTec ET CT/GC 扩增 DNA 检测(BD 诊断公司,斯帕克斯,MD)。通过涉及性别的逻辑回归确定了预测确认的因素,以及年份、样本是否经过正式验证以及样本部位。根据制造商的说明正式包含的样本类型(即经过验证的样本)的筛查检测,确认率有所不同(Abbott、Roche 和 BD 检测的分别为 96.2%、86.0%和 73.9%)。对于 2/3 的检测,性别的影响不影响确认,对于制造商说明中未正式包含的样本(即未经确认的样本)的确认可能性分别为 Abbott、Roche 和 BD 检测的 89.1%、82.1%和 59.2%。直肠拭子是非经确认的样本,在最初用各自的检测方法检测的样本中,有 91.5%、90.1%和 87.4%的样本得到了确认。并非所有的 NAAT 都需要对验证样本进行确认,尽管鉴于观察到的变异性,初始的特定检测方法的评估是合理的。直肠样本是用于 NAAT 检测的强有力的生物标本,在用所述检测方法筛查时可能不需要确认。

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