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Metagenomics of Two Severe Foodborne Outbreaks Provides Diagnostic Signatures and Signs of Coinfection Not Attainable by Traditional Methods

机译:两次严重食源性暴发的宏基因组学提供了传统方法无法实现的合并感染的诊断特征和体征

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Diagnostic testing for foodborne pathogens relies on culture-based techniques that are not rapid enough for real-time disease surveillance and do not give a quantitative picture of pathogen abundance or the response of the natural microbiome. Powerful sequence-based culture-independent approaches, such as shotgun metagenomics, could sidestep these limitations and potentially reveal a pathogen-specific signature on the microbiome that would have implications not only for diagnostics but also for better understanding disease progression and pathogen ecology. However, metagenomics have not yet been validated for foodborne pathogen detection. Toward closing these gaps, we applied shotgun metagenomics to stool samples collected from two geographically isolated (Alabama and Colorado) foodborne outbreaks, where the etiologic agents were identified by culture-dependent methods as distinct strains of Salmonella enterica subsp. enterica serovar Heidelberg. Metagenomic investigations were consistent with the culture-based findings and revealed, in addition, the in situ abundance and level of intrapopulation diversity of the pathogen, the possibility of coinfections with Staphylococcus aureus, overgrowth of commensal Escherichia coli, and significant shifts in the gut microbiome during infection relative to reference healthy samples. Additionally, we designed our bioinformatics pipeline to deal with several challenges associated with the analysis of clinical samples, such as the high frequency of coeluting human DNA sequences and assessment of the virulence potential of pathogens. Comparisons of these results to those of other studies revealed that in several, but not all, cases of diarrheal outbreaks, the disease and healthy states of the gut microbial community might be distinguishable, opening new possibilities for diagnostics.
机译:食源性病原体的诊断检测依赖于基于培养的技术,这些技术对于实时疾病监测来说不够快速,并且不能定量地反映病原体丰度或天然微生物组的反应。强大的基于序列的培养非依赖性方法,如鸟枪法宏基因组学,可以回避这些局限性,并可能揭示微生物组上的病原体特异性特征,这不仅对诊断有影响,而且对更好地了解疾病进展和病原体生态学也有影响。然而,宏基因组学尚未被验证用于食源性病原体检测。为了缩小这些差距,我们将鸟枪法宏基因组学应用于从两个地理隔离(阿拉巴马州和科罗拉多州)食源性暴发中收集的粪便样本,其中病原体通过培养依赖性方法鉴定为海德堡肠道沙门氏菌亚种的不同菌株。宏基因组学研究与基于培养的结果一致,此外还揭示了病原体的原位丰度和种群内多样性水平、与金黄色葡萄球菌合并感染的可能性、共生大肠杆菌的过度生长以及感染期间肠道微生物组相对于参考健康样本的显着变化。此外,我们设计了生物信息学管道,以应对与临床样本分析相关的几个挑战,例如人类DNA序列共洗脱的高频率和病原体毒力潜力的评估。将这些结果与其他研究的结果进行比较表明,在几个(但不是全部)腹泻爆发病例中,肠道微生物群落的疾病和健康状态可能是可区分的,这为诊断开辟了新的可能性。

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