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用于对与不同环境样本相关的微生物群落进行非培养分析的DNA提取方法的统计评估。

Statistical assessment of DNA extraction methodology for culture-independent analysis of microbial community associated with diverse environmental samples.

作者信息

Mahajan Rishi, Attri Sampan, Sharma Kavita, Singh Niharika, Sharma Deepika, Goel Gunjan

机构信息

Department of Biotechnology and Bioinformatics, Jaypee University of Information Technology, Waknaghat, Solan, 173234, India.

出版信息

Mol Biol Rep. 2018 Jun;45(3):297-308. doi: 10.1007/s11033-018-4162-3. Epub 2018 Feb 16.

DOI:10.1007/s11033-018-4162-3
PMID:29453765
Abstract

Cost-effectiveness, quality, time-effectiveness and ease of the methodology are the most crucial factors in isolating quality DNA from wide variety of samples. Thus, research efforts focusing on the development of an efficient DNA extraction protocol is the need of the hour. The present study therefore, focuses on development of an efficient, rapid and free of inhibitory substances based methodology for extracting metagenomic DNA from diverse environmental samples viz. anaerobic biogas digesta, ruminant stomach, human feces, soil, and microbial starter cultures used for preparation of fermented food. PCR-DGGE based analysis and quality metagenomic library preparation, using DNA extraction methodology, validates the developed protocol. The developed protocol is cost effective, capable of isolating DNA from small sample size (100-1000 µl), time efficient (1.5-2.0 h protocol) and results in significantly higher DNA yield (4-8 times increased yield) when compared to previously available DNA extraction method and a commercial DNA extraction kit. The DNA extracted from the samples using different protocols was evaluated based on its ability to identify diverse microbial species using PCR-DGGE profiles targeting variable region within the 16S rRNA gene. The results of microbial community analysis revealed comparability of the developed protocol to commercial kits, in effectively identifying dominant representatives of the microbial community in different samples. Using the DNA extracted from the presented methodology, metagenomic libraries were prepared, which were found suitable for sequencing on Illumina platform.

摘要

成本效益、质量、时间效益以及方法的简便性是从各种样本中分离高质量DNA的最关键因素。因此,当下迫切需要致力于开发一种高效的DNA提取方案。所以,本研究着重于开发一种高效、快速且不含抑制性物质的方法,用于从不同环境样本中提取宏基因组DNA,这些样本包括厌氧沼气消化池、反刍动物胃、人类粪便、土壤以及用于制备发酵食品的微生物发酵剂培养物。基于PCR-DGGE的分析以及使用DNA提取方法制备高质量宏基因组文库,验证了所开发的方案。与先前可用的DNA提取方法和商业DNA提取试剂盒相比,所开发的方案具有成本效益,能够从小样本量(100 - 1000微升)中分离DNA,时间效率高(1.5 - 2.0小时的方案),并且DNA产量显著更高(产量提高4 - 8倍)。基于利用靶向16S rRNA基因可变区域的PCR-DGGE图谱鉴定不同微生物物种的能力,对使用不同方案从样本中提取的DNA进行了评估。微生物群落分析结果表明,所开发的方案在有效鉴定不同样本中微生物群落的优势代表方面与商业试剂盒具有可比性。使用从所提出的方法中提取的DNA制备了宏基因组文库,发现其适合在Illumina平台上进行测序。

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Using environmental DNA to assess population-wide spatiotemporal reserve use.利用环境DNA评估全种群的时空保护区利用情况。
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The effect of DNA extraction methodology on gut microbiota research applications.DNA提取方法对肠道微生物群研究应用的影响。
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Protocols for metagenomic DNA extraction and Illumina amplicon library preparation for faecal and swab samples.粪便和拭子样本的宏基因组DNA提取及Illumina扩增子文库制备方案。
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