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组织样本直接 PCR 检测结核分枝杆菌复合群:一种替代细菌培养的方法。

Direct PCR on Tissue Samples To Detect Mycobacterium tuberculosis Complex: an Alternative to the Bacteriological Culture.

机构信息

VISAVET Health Surveillance Center, Complutense University of Madrid, Madrid, Spain.

Veterinary Faculty, Animal Health Department, Complutense University of Madrid, Madrid, Spain.

出版信息

J Clin Microbiol. 2021 Jan 21;59(2). doi: 10.1128/JCM.01404-20.

Abstract

Bovine tuberculosis (bTB) is an ongoing issue in several countries within the European Union. Microbiological culture is the official confirmation technique for the presence of complex (MTBC) members in bovine tissues, but several methodological issues, such as moderate sensitivity and long incubation times, require the development of more sensitive and rapid techniques. This study evaluates the analytical and diagnostic performance, comparative to culture, of a real-time PCR targeting the MTBC-specific IS transposon using a panel of bovine tissue samples sourced from the Spanish bTB eradication campaign. Robustness and repeatability were evaluated in an interlaboratory trial between European Union National Reference Laboratories. The limit of detection with 95% confidence was established at 65 fg/reaction of purified genomic equivalents. Diagnostic sensitivity (Se) and specificity (Sp) were, respectively, 96.45% and 93.66%, and the overall agreement (κ) was 0.88. Cross-reactivity was detected against two mycobacterial isolates identified as and " subsp. ," and whole-genome sequencing (WGS) analysis of the latter isolate revealed an IS-like sequence with 83% identity. An identical IS-like element was found in other complex species in the NCBI nucleotide and WGS databases. Despite this finding, this methodology is considered a valuable alternative to culture, and the strategy of use should be defined depending on the control or eradication programs.

摘要

牛结核病(bTB)是欧盟几个国家持续存在的问题。微生物培养是确认牛组织中复杂分枝杆菌(MTBC)成员存在的官方确认技术,但一些方法学问题,如中度敏感性和较长的孵育时间,需要开发更敏感和快速的技术。本研究使用来自西班牙牛结核病根除运动的牛组织样本进行了一项分析,评估了针对 MTBC 特异性 IS 转座子的实时 PCR 技术的分析和诊断性能,与培养方法相比。在欧盟国家参考实验室之间的实验室间试验中评估了稳健性和可重复性。用 95%置信区间建立的检测限为 65 fg/反应的纯化基因组当量。诊断灵敏度(Se)和特异性(Sp)分别为 96.45%和 93.66%,总体一致性(κ)为 0.88。针对两种鉴定为 和“ 亚种”的分枝杆菌分离株检测到交叉反应,对后者分离株的全基因组测序(WGS)分析显示存在与 83%同源性的 IS 样序列。在 NCBI 核苷酸和 WGS 数据库中其他复杂种属中发现了相同的 IS 样元件。尽管有此发现,但该方法被认为是培养的一种有价值的替代方法,并且应根据控制或根除计划定义使用策略。

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