Impact of Sample Type and DNA Isolation Procedure on Genomic Inference of Microbiome Composition

被引:168
作者
Knudsen, Berith E. [1 ]
Bergmark, Lasse [1 ,3 ]
Munk, Patrick [1 ]
Lukjancenko, Oksana [1 ]
Prieme, Anders [2 ]
Aarestrup, Frank M. [1 ]
Pamp, Sunje J. [1 ]
机构
[1] Tech Univ Denmark, Natl Food Inst, Lyngby, Denmark
[2] Univ Copenhagen, Dept Biol, Copenhagen, Denmark
[3] Novo Nordisk, Bagsvaerd, Denmark
关键词
16S rRNA gene profiling; DNA isolation; metagenomics; microbial ecology; microbiome; next-generation sequencing; BACTERIAL; RICHNESS;
D O I
10.1128/mSystems.00095-16
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Explorations of complex microbiomes using genomics greatly enhance our understanding about their diversity, biogeography, and function. The isolation of DNA from microbiome specimens is a key prerequisite for such examinations, but challenges remain in obtaining sufficient DNA quantities required for certain sequencing approaches, achieving accurate genomic inference of microbiome composition, and facilitating comparability of findings across specimen types and sequencing projects. These aspects are particularly relevant for the genomics-based global surveillance of infectious agents and antimicrobial resistance from different reservoirs. Here, we compare in a stepwise approach a total of eight commercially available DNA extraction kits and 16 procedures based on these for three specimen types (human feces, pig feces, and hospital sewage). We assess DNA extraction using spike-in controls and different types of beads for bead beating, facilitating cell lysis. We evaluate DNA concentration, purity, and stability and microbial community composition using 16S rRNA gene sequencing and for selected samples using shotgun metagenomic sequencing. Our results suggest that inferred community composition was dependent on inherent specimen properties as well as DNA extraction method. We further show that bead beating or enzymatic treatment can increase the extraction of DNA from Gram-positive bacteria. Final DNA quantities could be increased by isolating DNA from a larger volume of cell lysate than that in standard protocols. Based on this insight, we designed an improved DNA isolation procedure optimized for microbiome genomics that can be used for the three examined specimen types and potentially also for other biological specimens. A standard operating procedure is available from https://dx.doi.org/10.6084/m9.figshare.3475406. IMPORTANCE Sequencing-based analyses of microbiomes may lead to a breakthrough in our understanding of the microbial worlds associated with humans, animals, and the environment. Such insight could further the development of innovative ecosystem management approaches for the protection of our natural resources and the design of more effective and sustainable solutions to prevent and control infectious diseases. Genome sequence information is an organism (pathogen)independent language that can be used across sectors, space, and time. Harmonized standards, protocols, and workflows for sample processing and analysis can facilitate the generation of such actionable information. In this study, we assessed several procedures for the isolation of DNA for next-generation sequencing. Our study highlights several important aspects to consider in the design and conduct of sequence-based analysis of microbiomes. We provide a standard operating procedure for the isolation of DNA from a range of biological specimens particularly relevant in clinical diagnostics and epidemiology.
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页数:15
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