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Highly Reproducible 16S Sequencing Facilitates Measurement of Host Genetic Influences on the Stickleback Gut Microbiome

机译:高度可重复的16s测序有助于测量载体肠道微生物组上的宿主遗传影响

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Multicellular organisms interact with resident microbes in important ways, and a better understanding of host-microbe interactions is aided by tools such as high-throughput 16S sequencing. However, rigorous evaluation of the veracity of these tools in a different context from which they were developed has often lagged behind. Our goal was to perform one such critical test by examining how variation in tissue preparation and DNA isolation could affect inferences about gut microbiome variation between two genetically divergent lines of threespine stickleback fish maintained in the same laboratory environment. Using careful experimental design and intensive sampling of individuals, we addressed technical and biological sources of variation in 16S-based estimates of microbial diversity. After employing a two-tiered bead beating approach that comprised tissue homogenization followed by microbial lysis in subsamples, we found an extremely minor effect of DNA isolation protocol relative to among-host microbial diversity differences. Abundance estimates for rare operational taxonomic units (OTUs), however, showed much lower reproducibility. Gut microbiome composition was highly variable across fish—even among cohoused siblings—relative to technical replicates, but a subtle effect of host genotype (stickleback line) was nevertheless detected for some microbial taxa. IMPORTANCE Our findings demonstrate the importance of appropriately quantifying biological and technical variance components when attempting to understand major influences on high-throughput microbiome data. Our focus was on understanding among-host (biological) variance in community metrics and its magnitude in relation to within-host (technical) variance, because meaningful comparisons among individuals are necessary in addressing major questions in host-microbe ecology and evolution, such as heritability of the microbiome. Our study design and insights should provide a useful example for others desiring to quantify microbiome variation at biological levels in the face of various technical factors in a variety of systems.
机译:多细胞生物以重要的方式与常规微生物相互作用,并且通过诸如高通量16s测序的工具来帮助更好地理解宿主微生物相互作用。然而,严格评估这些工具的真实性在他们开发的不同背景下经常落后。我们的目标是通过检查组织制剂和DNA分离的变化如何影响关于在同一实验室环境中维护的两个遗传分歧的血管内汗鱼鱼之间的肠道微生物变化的推论。利用仔细的实验​​设计和密集采样的个人,我们解决了16S基微生物多样性估计的技术和生物学来源。在采用具有组织均质化的双层珠子跳动方法之后,随后是亚样品中的微生物裂解,我们发现DNA分离方案相对于宿主微生物多样性差异的极小效果。然而,对罕见运营分类单位(OTUS)的丰富估计表现出更低的再现性。肠道微生物组合物在鱼类中具有高度变化 - 甚至在舒适的兄弟姐妹中 - 相对于技术复制,但对于一些微生物分类群来说,仍然检测到宿主基因型(棘爪线)的微妙效果。重要性我们的调查结果表明,在试图了解对高通量微生物组数据的主要影响时适当地定量生物和技术方差分量的重要性。我们的重点是在社区度量的主持人(生物)方差以及主机内(技术)方差的幅度的理解,因为个人在主持人微生物生态和进化中的主要问题中有意义地进行了有意义的比较微生物组的遗传性。我们的研究设计和见解应为他人提供一种有用的示例,以便在面对各种系统中的各种技术因素面对各种技术因素来量化生物水平的微生物组变化。

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