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Impacts of Inter- and Intralaboratory Variations on the Reproducibility of Microbial Community Analyses

机译:实验室间和实验室内变异对微生物群落分析可重复性的影响

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摘要

With the advent of molecular biological techniques, especially next-generation sequencing and metagenomics, the number of microbial biogeography studies is rapidly increasing. However, these studies involve the synthesis of data generated by different laboratories using different protocols, chemicals, etc., all with inherent biases. The aim of this study was to assess inter- as well as intralaboratory variations in microbial community composition when standardized protocols are applied to a single soil sample. Aliquots from a homogenized soil sample from a rice field in Italy were sent to five participating laboratories. DNA was extracted by two investigators per laboratory using an identical protocol. All DNA samples were sent to one laboratory to perform DNA quantification, quantitative PCR (QPCR), and microarray and denaturing gradient gel electrophoresis (DGGE) analyses of methanotrophic communities. Yields, as well as purity of DNA, were significantly different between laboratories but in some cases also between investigators within the same laboratory. The differences in yield and quality of the extracted DNA were reflected in QPCR, microarray, and DGGE analysis results. Diversity indices (Shannon-Wiener, evenness, and richness) differed significantly between laboratories. The observed differences have implications for every project in which microbial communities are compared in different habitats, even if assessed within the same laboratory. To be able to make sensible comparisons leading to valid conclusions, intralaboratory variation should be assessed. Standardization of DNA extraction protocols and possible use of internal standards in interlaboratory comparisons may help in rendering a “quantifiable” bias.
机译:随着分子生物学技术的出现,特别是下一代测序和宏基因组学的发展,微生物生物地理学研究的数量正在迅速增加。但是,这些研究涉及由不同实验室使用不同的方案,化学药品等生成的数据的合成,所有这些都有固有的偏差。这项研究的目的是评估将标准化方案应用于单个土壤样品时微生物群落组成之间以及实验室内部的差异。来自意大利稻田的均质土壤样品的等分试样被送至五个参与实验室。每个实验室的两名研究人员使用相同的方案提取DNA。将所有DNA样品送至一间实验室进行甲烷营养化群落的DNA定量,定量PCR(QPCR)以及微阵列和变性梯度凝胶电泳(DGGE)分析。实验室之间的产量和DNA纯度均存在显着差异,但在某些情况下,同一实验室中的研究人员之间也存在显着差异。 QPCR,微阵列和DGGE分析结果反映了提取DNA的产量和质量的差异。实验室之间的多样性指数(Shannon-Wiener,均匀度和丰富度)差异很大。所观察到的差异对于在不同生境中比较微生物群落的每个项目都具有影响,即使在同一实验室进行评估也是如此。为了能够进行合理的比较以得出有效的结论,应评估实验室内的差异。 DNA提取方案的标准化以及在实验室间比较中可能使用内部标准可能有助于产生“可量化”的偏见。

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