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获取土壤宏基因组以研究微生物多样性。

Accessing the soil metagenome for studies of microbial diversity.

机构信息

Environmental Microbial Genomics, Laboratoire Ampere, Ecole Centrale de Lyon, Université de Lyon, 36 Avenue Guy de Collongue, 69134 Ecully, France.

出版信息

Appl Environ Microbiol. 2011 Feb;77(4):1315-24. doi: 10.1128/AEM.01526-10. Epub 2010 Dec 23.

Abstract

Soil microbial communities contain the highest level of prokaryotic diversity of any environment, and metagenomic approaches involving the extraction of DNA from soil can improve our access to these communities. Most analyses of soil biodiversity and function assume that the DNA extracted represents the microbial community in the soil, but subsequent interpretations are limited by the DNA recovered from the soil. Unfortunately, extraction methods do not provide a uniform and unbiased subsample of metagenomic DNA, and as a consequence, accurate species distributions cannot be determined. Moreover, any bias will propagate errors in estimations of overall microbial diversity and may exclude some microbial classes from study and exploitation. To improve metagenomic approaches, investigate DNA extraction biases, and provide tools for assessing the relative abundances of different groups, we explored the biodiversity of the accessible community DNA by fractioning the metagenomic DNA as a function of (i) vertical soil sampling, (ii) density gradients (cell separation), (iii) cell lysis stringency, and (iv) DNA fragment size distribution. Each fraction had a unique genetic diversity, with different predominant and rare species (based on ribosomal intergenic spacer analysis [RISA] fingerprinting and phylochips). All fractions contributed to the number of bacterial groups uncovered in the metagenome, thus increasing the DNA pool for further applications. Indeed, we were able to access a more genetically diverse proportion of the metagenome (a gain of more than 80% compared to the best single extraction method), limit the predominance of a few genomes, and increase the species richness per sequencing effort. This work stresses the difference between extracted DNA pools and the currently inaccessible complete soil metagenome.

摘要

土壤微生物群落拥有所有环境中最高水平的原核生物多样性,而涉及从土壤中提取 DNA 的宏基因组方法可以提高我们对这些群落的了解。大多数对土壤生物多样性和功能的分析都假设从土壤中提取的 DNA 代表了土壤中的微生物群落,但随后的解释受到从土壤中回收的 DNA 的限制。不幸的是,提取方法并不能为宏基因组 DNA 提供均匀且无偏的样本,因此无法准确确定物种的分布情况。此外,任何偏差都会导致对整体微生物多样性的估计产生误差,并可能使某些微生物类群无法进行研究和利用。为了改进宏基因组方法、研究 DNA 提取偏差并提供评估不同群体相对丰度的工具,我们通过将宏基因组 DNA 按以下方式进行分组,来研究可及社区 DNA 的生物多样性:(i)垂直土壤采样,(ii)密度梯度(细胞分离),(iii)细胞裂解严格性,和(iv)DNA 片段大小分布。每个部分都具有独特的遗传多样性,具有不同的主要和稀有物种(基于核糖体基因间 spacer 分析 [RISA] 指纹图谱和 phylochips)。所有部分都有助于发现宏基因组中更多的细菌群体,从而增加了用于进一步应用的 DNA 池。事实上,我们能够访问宏基因组中更多具有遗传多样性的部分(与最佳的单一提取方法相比,增加了 80%以上),限制了少数基因组的优势,并增加了每个测序工作的物种丰富度。这项工作强调了提取的 DNA 池与当前无法访问的完整土壤宏基因组之间的差异。

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