Development and performance evaluation of a clinical metagenomics approach for identifying pathogens in the whole blood from patients with undifferentiated fever.

IF 4.8 2区医学 Q2 IMMUNOLOGY

Frontiers in Cellular and Infection Microbiology Pub Date : 2025-09-15 eCollection Date: 2025-01-01 DOI:10.3389/fcimb.2025.1667422

Jan Slunečko, Rok Kogoj, Samo Zakotnik, Alen Suljič, Nataša Knap, Martin Bosilj, Franc Strle, Tatjana Avšič-Županc, Petra Bogovič, Miša Korva

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引用次数: 0

Abstract

Introduction: Blood culture is the cornerstone of microbiological diagnostics for patients with acute undifferentiated fever and no obvious localization of infection; however, up to 50% of cases remain undiagnosed. Infections caused by arboviruses, fastidious or even uncultivable bacteria, or parasites often go undiagnosed without the use of target-specific molecular methods. These are typically performed in a stepwise manner, increasing cost and delaying results. Metagenomic next-generation sequencing (mNGS) has recently gained recognition as a potential universal pathogen detection tool for such cases. Our study aimed to develop a streamlined mNGS workflow for simultaneous detection of intracellular and cell-free pathogens within a single sequencing library.

Methods: Total nucleic acid was isolated separately from 200 EDTA blood samples. The plasma isolate was processed with DNase, followed by the depletion of host ribosomal and messenger RNA, reverse transcription, and sequence-independent single primer amplification (SISPA). The whole blood isolate was only reverse transcribed, with no other pre-processing manipulation. Finally, the two fractions were combined prior to library preparation and sequencing using either Oxford Nanopore Technologies or Illumina. Following established bioinformatics analysis, we developed a mathematical ranking approach (ClinSeq score) that enabled quick identification of relevant pathogens in approximately one hour.

Results: The mNGS workflow reached 79.5% (159/200) overall sensitivity. For bacteria the sensitivity was 88.6% (70/79), DNA viruses, 66.7% (10/15) and for RNA viruses 73.8% (76/103). Pathogen detections by individual sequencing methods showed overall sensitivity of Illumina and ONT to be 80.0% (76/95) and 79.1% (83/105) respectively. The ClinSeq score correctly highlighted the pathogen in 126/200 (63.0%) samples effectively with a Cohen's kappa (κ) agreement of 0.61 with manual analysis.

Conclusion: Developed comprehensive mNGS workflow detects a wide range of pathogens in patients with acute undifferentiated fever. The unified workflow improves sensitivity for intracellular bacteria and RNA viruses, reduces time, cost and complexity by eliminating the need for separate library preparations, enabling faster turnaround suitable for clinical settings. The ClinSeq score effectively differentiates true pathogen signals from background noise, reducing false positives and manual interpretation time. Overall, the workflow demonstrates flexible, and efficient pathogen detection, supporting its potential for clinical diagnostics and improved patient management.

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用于鉴定未分化发热患者全血病原体的临床宏基因组学方法的开发和性能评估。

简介：血培养是急性未分化发热且感染无明显局限性患者微生物学诊断的基础；然而，高达50%的病例仍未得到诊断。由虫媒病毒、挑剔的甚至不可培养的细菌或寄生虫引起的感染，如果不使用靶向分子方法，往往无法诊断。这些通常以逐步的方式进行，增加了成本并延迟了结果。元基因组下一代测序（mNGS）最近被认为是一种潜在的通用病原体检测工具。我们的研究旨在开发一种简化的mNGS工作流程，用于在单个测序文库中同时检测细胞内和细胞外病原体。方法：从200份EDTA血样中分离总核酸。血浆分离物经dna酶处理，然后进行宿主核糖体和信使RNA的消耗，逆转录和序列独立单引物扩增（SISPA）。全血分离株仅进行逆转录，未进行其他预处理操作。最后，在文库制备和测序之前，使用Oxford Nanopore Technologies或Illumina将两个部分结合起来。根据已建立的生物信息学分析，我们开发了一种数学排序方法（ClinSeq评分），可以在大约一小时内快速识别相关病原体。结果：mNGS工作流程的总灵敏度达到79.5%（159/200）。细菌的敏感性为88.6% (70/79)，DNA病毒为66.7% (10/15)，RNA病毒为73.8%（76/103）。不同测序方法的病原菌检测结果显示，Illumina和ONT的总灵敏度分别为80.0%（76/95）和79.1%（83/105）。ClinSeq评分正确地突出了126/200（63.0%）样品中的病原体，人工分析的科恩kappa （κ）一致性为0.61。结论：开发的综合mNGS工作流程可检测急性未分化热患者的多种病原体。统一的工作流程提高了对细胞内细菌和RNA病毒的敏感性，通过消除对单独文库准备的需要，减少了时间、成本和复杂性，实现了适合临床环境的更快周转。ClinSeq评分有效地从背景噪声中区分真实的病原体信号，减少假阳性和人工解释时间。总体而言，该工作流程展示了灵活、高效的病原体检测，支持其在临床诊断和改善患者管理方面的潜力。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Frontiers in Cellular and Infection Microbiology IMMUNOLOGY-MICROBIOLOGY

CiteScore

7.90

自引率

7.00%

发文量

1817

审稿时长

14 weeks

期刊介绍： Frontiers in Cellular and Infection Microbiology is a leading specialty journal, publishing rigorously peer-reviewed research across all pathogenic microorganisms and their interaction with their hosts. Chief Editor Yousef Abu Kwaik, University of Louisville is supported by an outstanding Editorial Board of international experts. This multidisciplinary open-access journal is at the forefront of disseminating and communicating scientific knowledge and impactful discoveries to researchers, academics, clinicians and the public worldwide. Frontiers in Cellular and Infection Microbiology includes research on bacteria, fungi, parasites, viruses, endosymbionts, prions and all microbial pathogens as well as the microbiota and its effect on health and disease in various hosts. The research approaches include molecular microbiology, cellular microbiology, gene regulation, proteomics, signal transduction, pathogenic evolution, genomics, structural biology, and virulence factors as well as model hosts. Areas of research to counteract infectious agents by the host include the host innate and adaptive immune responses as well as metabolic restrictions to various pathogenic microorganisms, vaccine design and development against various pathogenic microorganisms, and the mechanisms of antibiotic resistance and its countermeasures.