Mycobacterium tuberculosis pseudo-outbreak due to laboratory cross-contamination: A molecular epidemiology outbreak investigation.

Nayla Léveillé, Floriane Point, Josée Houde, Michael Hall, Hafid Souhaline, Marie-Andrée Leblanc, Pierre-Marie Akochy, Simon Grandjean Lapierre
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Abstract

Background: Mycobacterial culture is routinely performed to diagnose tuberculosis (TB) in Canada. Globally, meta-analyses suggest that up to 2% of positive cultures are falsely positive for Mycobacterium tuberculosis due to laboratory cross-contamination. Five patients from distinct clinical institutions in Montréal were diagnosed with culture-positive TB as their clinical samples were processed in a centralized mycobacteria laboratory. Cross-contamination was suspected due to culture positivity in an organ donor with low TB pre-test probability. We describe a TB pseudo-outbreak due to laboratory cross-contamination and assess the role of conventional typing (i.e., mycobacterial interspersed repetitive unit variable number of tandem repeats [MIRU-VNTR]) and whole-genome sequencing (WGS) in supporting the investigation.

Methods: Patients' epidemiological risk factors and clinical presentations were reviewed. The trajectories of pre- and per-analytic samples were retraced to identify potential cross-contamination events. Tuberculosis isolates were characterized by MIRU-VNTR and WGS using Oxford Nanopore Technology (ONT). The bioinformatic pipeline tbpore (v0.7.1) cluster was used for phylogenetic analyses.

Results: Two patients had previous exposure to endemic settings and clinical symptoms compatible with TB. Culture media inoculation overlapped in time for four patients, including one with suspected pulmonary cavitary disease and an organ donor whose organs had been transplanted in three different receivers. The MIRU-VNTR and WGS typing confirmed isolates from those four patients to be identical.

Conclusion: Clinical, laboratory and molecular typing data, including results from ONT sequencing, were considered sufficiently robust to confirm laboratory cross-contamination and TB therapy was discontinued including in all organ transplant recipients.

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实验室交叉污染引起的结核分枝杆菌伪暴发:一次分子流行病学暴发调查。
背景:在加拿大,分枝杆菌培养是诊断结核病的常规方法。在全球范围内,荟萃分析表明,由于实验室交叉污染,高达2%的阳性培养物为结核分枝杆菌假阳性。在集中的分枝杆菌实验室处理临床样本时,来自montracimal不同临床机构的5名患者被诊断为培养阳性结核。由于一名器官供体培养阳性,且结核病检测前概率低,因此怀疑存在交叉污染。我们描述了一起由实验室交叉污染引起的结核病伪暴发,并评估了传统分型(即分枝杆菌穿插重复单位可变数目串联重复序列[MIRU-VNTR])和全基因组测序(WGS)在支持调查中的作用。方法:回顾性分析患者的流行病学危险因素及临床表现。分析前和分析后样品的轨迹被追溯,以确定潜在的交叉污染事件。采用牛津纳米孔技术(ONT)对结核分离株进行MIRU-VNTR和WGS鉴定。采用生物信息学管道tbpore (v0.7.1)聚类进行系统发育分析。结果:两名患者曾接触过地方性环境,临床症状与结核病相符。四名患者的培养基接种时间重叠,包括一名疑似肺腔疾病患者和一名器官捐赠者,他的器官被移植给了三个不同的接受者。MIRU-VNTR和WGS分型证实这4例患者的分离株是相同的。结论:临床、实验室和分子分型数据,包括ONT测序结果,被认为足够可靠,可以确认实验室交叉污染,并停止结核病治疗,包括所有器官移植受者。
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