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利用单核苷酸多态性和核心基因组多位点序列分型结合纳米孔读取对肠炎沙门氏菌进行亚型评估。

Subtyping Evaluation of Enteritidis Using Single Nucleotide Polymorphism and Core Genome Multilocus Sequence Typing with Nanopore Reads.

机构信息

Center for Food Safety, University of Georgiagrid.213876.9, Griffin, Georgia, USA.

School of Biomedical and Pharmaceutical Sciences, Guangdong University of Technology, Guangzhou, China.

出版信息

Appl Environ Microbiol. 2022 Aug 9;88(15):e0078522. doi: 10.1128/aem.00785-22. Epub 2022 Jul 12.

Abstract

Whole-genome sequencing (WGS) for public health surveillance and epidemiological investigation of foodborne pathogens predominantly relies on sequencing platforms that generate short reads. Continuous improvement of long-read nanopore sequencing, such as Oxford nanopore technologies (ONT), presents a potential for leveraging multiple advantages of the technology in public health and food industry settings, including rapid turnaround and onsite applicability in addition to superior read length. Using an established cohort of Salmonella Enteritidis isolates for subtyping evaluation, we assessed the technical readiness of nanopore long read sequencing for single nucleotide polymorphism (SNP) analysis and core-genome multilocus sequence typing (cgMLST) of a major foodborne pathogen. By multiplexing three isolates per flow cell, we generated sufficient sequencing depths in <7 h of sequencing for robust subtyping. SNP calls by ONT and Illumina reads were highly concordant despite homopolymer errors in ONT reads (R9.4.1 chemistry). correction of such errors allowed accurate allelic calling for cgMLST and allelic difference measurements to facilitate heuristic detection of outbreak isolates. Evaluation, standardization, and implementation of the ONT approach to WGS-based, strain-level subtyping is challenging, in part due to its relatively high base-calling error rates and frequent iterations of sequencing chemistry and bioinformatic analytics. Our study established a baseline for the continuously evolving nanopore technology as a viable solution to high-quality subtyping of Salmonella, delivering comparable subtyping performance when used standalone or together with short-read platforms. This study paves the way for evaluating and optimizing the logistics of implementing the ONT approach for foodborne pathogen surveillance in specific settings.

摘要

全基因组测序(WGS)主要用于公共卫生监测和食源性病原体的流行病学调查,依赖于生成短读长的测序平台。Oxford nanopore technologies(ONT)等长读长纳米孔测序的不断改进,为在公共卫生和食品工业环境中利用该技术的多种优势提供了潜力,包括快速周转和现场适用性,以及优越的读长。我们使用建立的肠炎沙门氏菌分离株进行亚分型评估的队列,评估了纳米孔长读测序在单核苷酸多态性(SNP)分析和主要食源性病原体核心基因组多位点序列分型(cgMLST)中的技术准备情况。通过每个流动池混合三个分离株,我们在 <7 小时的测序时间内生成了足够的测序深度,以进行稳健的亚分型。尽管 ONT 读长中存在同源多聚体错误(R9.4.1 化学),但 ONT 和 Illumina 读长的 SNP 调用高度一致。通过纠正此类错误,允许对 cgMLST 进行准确的等位基因调用,并测量等位基因差异,以促进对暴发分离株的启发式检测。基于 WGS 的基于菌株水平的亚分型的 ONT 方法的评估、标准化和实施具有挑战性,部分原因是其相对较高的碱基调用错误率和频繁的测序化学和生物信息学分析迭代。我们的研究为不断发展的纳米孔技术建立了基线,作为沙门氏菌高质量亚分型的可行解决方案,当单独使用或与短读长平台一起使用时,提供可比的亚分型性能。本研究为评估和优化特定环境中实施 ONT 方法进行食源性病原体监测的物流铺平了道路。

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