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16S rRNA gene pyrosequencing of reference and clinical samples and investigation of the temperature stability of microbiome profiles

机译:参考和临床样品的16S rRNA基因焦磷酸测序以及微生物组谱的温度稳定性研究

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摘要

BackgroundSample storage conditions, extraction methods, PCR primers, and parameters are major factors that affect metagenomics analysis based on microbial 16S rRNA gene sequencing. Most published studies were limited to the comparison of only one or two types of these factors. Systematic multi-factor explorations are needed to evaluate the conditions that may impact validity of a microbiome analysis. This study was aimed to improve methodological options to facilitate the best technical approaches in the design of a microbiome study. Three readily available mock bacterial community materials and two commercial extraction techniques, Qiagen DNeasy and MO BIO PowerSoil DNA purification methods, were used to assess procedures for 16S ribosomal DNA amplification and pyrosequencing-based analysis. Primers were chosen for 16S rDNA quantitative PCR and amplification of region V3 to V1. Swabs spiked with mock bacterial community cells and clinical oropharyngeal swabs were incubated at respective temperatures of -80°C, -20°C, 4°C, and 37°C for 4 weeks, then extracted with the two methods, and subjected to pyrosequencing and taxonomic and statistical analyses to investigate microbiome profile stability.
机译:背景样品的储存条件,提取方法,PCR引物和参数是影响基于微生物16S rRNA基因测序的宏基因组学分析的主要因素。大多数发表的研究仅限于比较这些因素中的一种或两种。需要系统的多因素探索来评估可能影响微生物组分析有效性的条件。这项研究旨在改善方法选择,以促进微生物组研究设计中的最佳技术方法。三种容易获得的模拟细菌群落材料和两种商业提取技术,Qiagen DNeasy和MO BIO PowerSoil DNA纯化方法,用于评估16S核糖体DNA扩增和基于焦磷酸测序的分析程序。选择引物用于16S rDNA定量PCR和扩增区域V3至V1。将掺有模拟细菌群落细胞的拭子和临床口咽拭子分别在-80°C,-20°C,4°C和37°C的温度下孵育4周,然后用两种方法提取并进行焦磷酸测序以及分类学和统计分析来研究微生物组谱的稳定性。

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