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使用SOLiD 16S rRNA基因测序和SOLiD鸟枪法测序对肠道微生物群进行分析。

Analysis of the intestinal microbiota using SOLiD 16S rRNA gene sequencing and SOLiD shotgun sequencing.

作者信息

Mitra Suparna, Förster-Fromme Karin, Damms-Machado Antje, Scheurenbrand Tim, Biskup Saskia, Huson Daniel H, Bischoff Stephan C

出版信息

BMC Genomics. 2013;14 Suppl 5(Suppl 5):S16. doi: 10.1186/1471-2164-14-S5-S16. Epub 2013 Oct 16.

Abstract

BACKGROUND

Metagenomics seeks to understand microbial communities and assemblages by DNA sequencing. Technological advances in next generation sequencing technologies are fuelling a rapid growth in the number and scope of projects aiming to analyze complex microbial environments such as marine, soil or the gut. Recent improvements in longer read lengths and paired-sequencing allow better resolution in profiling microbial communities. While both 454 sequencing and Illumina sequencing have been used in numerous metagenomic studies, SOLiD sequencing is not commonly used in this area, as it is believed to be more suitable in the context of reference-guided projects.

RESULTS

To investigate the performance of SOLiD sequencing in a metagenomic context, we compared taxonomic profiles of SOLiD mate-pair sequencing reads with Sanger paired reads and 454 single reads. All sequences were obtained from the bacterial 16S rRNA gene, which was amplified from microbial DNA extracted from a human fecal sample. Additionally, from the same fecal sample, complete genomic microbial DNA was extracted and shotgun sequenced using SOLiD sequencing to study the composition of the intestinal microbiota and the existing microbial metabolism. We found that the microbiota composition of 16S rRNA gene sequences obtained using Sanger, 454 and SOLiD sequencing provide results comparable to the result based on shotgun sequencing. Moreover, with SOLiD sequences we obtained more resolution down to the species level. In addition, the shotgun data allowed us to determine a functional profile using the databases SEED and KEGG.

CONCLUSIONS

This study shows that SOLiD mate-pair sequencing is a viable and cost-efficient option for analyzing a complex microbiome. To the best of our knowledge, this is the first time that SOLiD sequencing has been used in a human sample.

摘要

背景

宏基因组学旨在通过DNA测序来了解微生物群落和组合。新一代测序技术的技术进步推动了旨在分析复杂微生物环境(如海洋、土壤或肠道)的项目数量和范围的快速增长。近期在更长读长和配对测序方面的改进使得在分析微生物群落时具有更高的分辨率。虽然454测序和Illumina测序已在众多宏基因组学研究中得到应用,但SOLiD测序在该领域并不常用,因为人们认为它更适用于参考引导的项目。

结果

为了研究SOLiD测序在宏基因组背景下的性能,我们将SOLiD配对末端测序读数的分类学图谱与桑格配对读数和454单端读数进行了比较。所有序列均来自细菌16S rRNA基因,该基因从人类粪便样本中提取的微生物DNA中扩增得到。此外,从同一粪便样本中提取了完整的基因组微生物DNA,并使用SOLiD测序进行鸟枪法测序,以研究肠道微生物群的组成和现有的微生物代谢。我们发现,使用桑格、454和SOLiD测序获得的16S rRNA基因序列的微生物群组成提供了与基于鸟枪法测序结果相当的结果。此外,利用SOLiD序列,我们在物种水平上获得了更高的分辨率。此外,鸟枪法数据使我们能够使用SEED和KEGG数据库确定功能图谱。

结论

本研究表明,SOLiD配对末端测序是分析复杂微生物组的一种可行且经济高效的选择。据我们所知,这是SOLiD测序首次用于人类样本。

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