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Design and application of a novel two-amplicon approach for defining eukaryotic microbiota

机译:一种微生物微生物的新型二扩增子方法的设计与应用

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摘要

Abstract Background Due to a lack of systematic diagnostics, our understanding of the diversity and role of eukaryotic microbiota in human health is limited. While studies have shown fungal communities to be significant modulators of human health, information on the prevalence of taxa such as protozoa and helminths has been limited to a small number of species for which targeted molecular diagnostics are available. To probe the diversity of eukaryotic microbes and their relationships with other members of the microbiota, we applied in silico and experimental approaches to design a novel two-amplicon surveillance tool, based on sequencing regions of ribosomal RNA genes and their internal transcribed spacers. We subsequently demonstrated the utility of our approach by characterizing the eukaryotic microbiota of 46 hospitalized Malawian children suffering from Severe Acute Malnutrition (SAM). Results Through in silico analysis and validation on a diverse panel of eukaryotes, we identified 18S rRNA variable genetic regions 4 and 5 (18S V4 V5), together with a region encoding 28S rRNA variable genetic region 2 and the internal transcribed spacers (transITS), as optimal for the systematic classification of eukaryotes. Sequencing of these regions revealed protozoa in all stool samples from children with SAM and helminths in most, including several eukaryotes previously implicated in malnutrition and diarrheal disease. Clinical comparisons revealed no association between protozoan parasites and diarrhea or HIV reactivity. However, the presence of Blastocystis correlated with bacterial alpha diversity and increased abundance of specific taxa, including Sporobacter, Cellulosibacter, Oscillibacter, and Roseburia. Conclusion We suggest this novel two-amplicon based strategy will prove an effective tool to deliver new insights into the role of eukaryotic microbiota in health and disease.
机译:摘要背景由于缺乏系统诊断,我们对人类健康中真核微生物群的多样性和作用的理解有限。虽然研究表明了真菌社区是人类健康的重要调节剂,但有关原生动物和蠕虫等分类率的普遍性的信息仅限于少量可获得靶标分子诊断的物种。为了探讨真核微生物的多样性及其与微生物群的其他成员的关系,我们应用于基于核糖体RNA基因的测序区域及其内部转录间隔物设计一种设计一种新型双扩增子监测工具的实验方法。随后,我们通过表征了46名住院的马拉维儿童患有严重急性营养不良(SAM)的真核微生物群的方法来证明了我们的方法的效用。结果通过在真核生物面板上的硅分析和验证中,我们鉴定了18S rRNA可变遗传区域4和5(18s V4 V5),以及编码28s rRNA可变遗传区域2和内部转录间隔物(转运)的区域,作为真核生物的系统分类的最佳选择。这些区域的测序显示了来自SAM和Helminths的儿童的所有粪便样本中的原生动物,包括若干以前涉及营养不良和腹泻病的真核生物。临床比较揭示了原生动物寄生虫和腹泻或静脉反应性之间的关联。然而,胚泡的存在与细菌α多样性相关和增加的特定分类群,包括猪杆菌,纤维素,振动杆菌和Roseburia。结论我们建议这种基于两种的基于两个扩增子的策略将证明是一种有效的工具,以便为真核微生物群在健康和疾病中提供新的洞察力。

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