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两阶段结核病诊断:在床边检测结核感染和 INH 和 RIF 耐药性时结合离心微流控技术,随后通过靶向 NGS 进行抗生素耐药性分析。

Two-stage tuberculosis diagnostics: combining centrifugal microfluidics to detect TB infection and Inh and Rif resistance at the point of care with subsequent antibiotic resistance profiling by targeted NGS.

机构信息

Hahn-Schickard, 79110 Freiburg, Germany.

SYNLAB Gauting SYNLAB Human Genetics Munich, 82131 Gauting, Germany.

出版信息

Lab Chip. 2023 Dec 20;24(1):74-84. doi: 10.1039/d3lc00783a.

DOI:10.1039/d3lc00783a
PMID:37999937
Abstract

Globally, tuberculosis (TB) remains the deadliest bacterial infectious disease, and spreading antibiotic resistances is the biggest challenge for combatting the disease. Rapid and comprehensive diagnostics including drug susceptibility testing (DST) would assure early treatment, reduction of morbidity and the interruption of transmission chains. To date, rapid genetic resistance testing addresses only one to four drug groups while complete DST is done phenotypically and takes several weeks. To overcome these limitations, we developed a two-stage workflow for rapid TB diagnostics including DST from a single sputum sample that can be completed within three days. The first stage is qPCR detection of complex (MTBC) including antibiotic resistance testing against the first-line antibiotics, isoniazid (Inh) and rifampicin (Rif). The test is automated by centrifugal microfluidics and designed for point of care (PoC). Furthermore, enriched MTBC DNA is provided in a detachable sample tube to enable the second stage: if the PCR detects MTBC and resistance to either Inh or Rif, the MTBC DNA is shipped to specialized facilities and analyzed by targeted next generation sequencing (tNGS) to assess the complete resistance profile. Proof-of-concept testing of the PoC test revealed an analytical sensitivity of 44.2 CFU ml, a diagnostic sensitivity of 96%, and a diagnostic specificity of 100% for MTBC detection. Coupled tNGS successfully provided resistance profiles, demonstrated for samples from 17 patients. To the best of our knowledge, the presented combination of PoC qPCR with tNGS allows for the fastest comprehensive TB diagnostics comprising decentralized pathogen detection with subsequent resistance profiling in a facility specialized in tNGS.

摘要

在全球范围内,结核病(TB)仍然是最致命的细菌性传染病,而抗生素耐药性的传播是对抗该疾病的最大挑战。快速和全面的诊断,包括药敏试验(DST),将确保早期治疗、降低发病率和中断传播链。迄今为止,快速基因耐药性检测仅针对一到四种药物组,而完整的 DST 是表型进行的,需要数周时间。为了克服这些限制,我们开发了一种两阶段的工作流程,用于从单个痰样本中进行快速结核病诊断和药敏试验,整个过程可在三天内完成。第一阶段是 qPCR 检测复杂的结核分枝杆菌(MTBC),包括针对一线抗生素异烟肼(Inh)和利福平(Rif)的耐药性检测。该测试通过离心微流控技术实现自动化,设计用于即时护理(PoC)。此外,提供了可分离的样本管中的富集 MTBC DNA,以实现第二阶段:如果 PCR 检测到 MTBC 以及对 Inh 或 Rif 的耐药性,则将 MTBC DNA 运送到专门的设施,并通过靶向下一代测序(tNGS)进行分析,以评估完整的耐药谱。该 PoC 测试的概念验证测试显示,MTBC 检测的分析灵敏度为 44.2 CFU ml,诊断灵敏度为 96%,特异性为 100%。耦合 tNGS 成功提供了耐药谱,为 17 名患者的样本提供了证明。据我们所知,这种即时检测 qPCR 与 tNGS 的组合允许进行最快的全面结核病诊断,包括在专门从事 tNGS 的设施中进行分散的病原体检测和随后的耐药性分析。

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