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Soil Sample Preservation Strategy Affects the Microbial Community Structure

机译:土壤样品保存策略影响微生物群落结构

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摘要

Sample preservation is a critical procedure in any research that relies on molecular tools and is conducted in remote areas. Sample preservation options include low and room temperature storage, which require freezing equipment and specific buffering solutions, respectively. The aim of the present study was to investigate whether DNA/RNA Shield 1x from Zymo Research and DESS (Dimethyl sulfoxide, Ethylenediamine tetraacetic acid, Saturated Salt) solution performed similarly to snap freezing in liquid nitrogen. Soil samples were stored for 1 month in each of the buffers and without any solution at a range of temperatures: –20, +4, and +23°C. All treatments were compared to the “optimal treatment”, namely, snap freezing in liquid nitrogen. The quality and quantity of DNA were analyzed, and the microbial community structure was investigated in all samples. The results obtained indicated that the quantity and integrity of DNA was preserved well in all samples; however, the taxonomic distribution was skewed in samples stored without any solution at ambient temperatures, particularly when analyses were performed at lower taxonomic levels. Although both solutions performed equally well, sequencing output and OTU numbers in DESS-treated samples were closer to those snap frozen with liquid nitrogen. Furthermore, DNA/RNA Shield-stored samples performed better for the preservation of rare taxa.
机译:样品保存是在任何依赖于分子工具的研究中的一个关键程序,并在偏远地区进行。样品保存选项包括较低和室温存储,其需要分别需要冷冻设备和特定的缓冲溶液。本研究的目的是研究与Zymo研究和DES(二甲基亚砜,乙二胺四乙酸,饱和盐)溶液类似的DNA / RNA屏蔽1X是否与液氮中的冷冻混合。在每个缓冲液中储存1个月的土壤样品,并且在温度范围内没有任何溶液:-20,+ 4和+ 23℃。将所有治疗与“最佳处理”进行比较,即液氮中的冻结。分析DNA的质量和量,并在所有样品中研究了微生物群落结构。得到的结果表明,在所有样品中,DNA的数量和完整性良好;然而,在没有任何溶液在环境温度下储存的样品中的样品中偏离分类物分布,特别是当分析在较低的分类水平下进行。尽管在DESS处理样品中同样良好地进行的溶液,测序输出和OTU数更接近液氮冷冻的那些。此外,DNA / RNA屏蔽存储的样品更好地进行了稀有出征的保存。

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