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Massively parallel sequencing of single cells by epicPCR links functional genes with phylogenetic markers

机译:通过epicPCR大规模并行测序单个细胞将功能基因与系统发生标记联系起来

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摘要

Many microbial communities are characterized by high genetic diversity. 16S ribosomal RNA sequencing can determine community members, and metagenomics can determine the functional diversity, but resolving the functional role of individual cells in high throughput remains an unsolved challenge. Here, we describe epicPCR (Emulsion, Paired Isolation and Concatenation PCR), a new technique that links functional genes and phylogenetic markers in uncultured single cells, providing a throughput of hundreds of thousands of cells with costs comparable to one genomic library preparation. We demonstrate the utility of our technique in a natural environment by profiling a sulfate-reducing community in a freshwater lake, revealing both known sulfate reducers and discovering new putative sulfate reducers. Our method is adaptable to any conserved genetic trait and translates genetic associations from diverse microbial samples into a sequencing library that answers targeted ecological questions. Potential applications include identifying functional community members, tracing horizontal gene transfer networks and mapping ecological interactions between microbial cells.
机译:许多微生物群落的特征是遗传多样性高。 16S核糖体RNA测序可以确定社区成员,宏基因组学可以确定功能多样性,但是在高通量下解析单个细胞的功能仍然是一项尚未解决的挑战。在这里,我们描述了epicPCR(乳液,配对分离和串联PCR),这是一种在未培养的单细胞中连接功能基因和系统发生标记的新技术,可提供成千上万个细胞的通量,其成本可与一个基因组文库制备相媲美。我们通过对淡水湖中的硫酸盐还原群落进行分析,揭示已知的硫酸盐还原剂并发现新的假定的硫酸盐还原剂,证明了我们技术在自然环境中的实用性。我们的方法适用于任何保守的遗传性状,并将来自各种微生物样品的遗传关联转化为可回答目标生态问题的测序文库。潜在的应用包括识别功能性社区成员,追踪水平基因转移网络以及绘制微生物细胞之间的生态相互作用。

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