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使用单叠氮碘化丙啶(PMA)排除无活性细菌DNA对首次排出胎粪中细菌微生物组进行表征。

Characterization of the bacterial microbiome in first-pass meconium using propidium monoazide (PMA) to exclude nonviable bacterial DNA.

作者信息

Stinson L F, Keelan J A, Payne M S

机构信息

Division of Obstetrics and Gynaecology, Faculty of Health & Medical Sciences, The University of Western Australia, Crawley, WA, Australia.

出版信息

Lett Appl Microbiol. 2019 May;68(5):378-385. doi: 10.1111/lam.13119. Epub 2019 Feb 15.

Abstract

Numerous studies have reported bacterial DNA in first-pass meconium samples, suggesting that the human gut microbiome is seeded prior to birth. However, these studies have not been able to discriminate between DNA from living bacterial cells, DNA from dead bacterial cells or cell-free DNA. Here we have used propidium monoazide (PMA) together with 16S rRNA gene sequencing to determine whether there are intact bacterial cells in the fetal gut. DNA was extracted from first-pass meconium (n = 5) and subjected to 16S rRNA gene sequencing with/without PMA treatment. All meconium samples, regardless of PMA treatment, contained detectable levels of bacterial DNA; however, treatment with PMA prior to DNA extraction decreased the DNA yield by approximately 20%. PMA-treated meconium samples did not differ significantly from untreated samples in terms of observed number of OTUs (P = 0·945); although they did differ taxonomically, with around one quarter of OTUs identified in untreated samples only, suggesting that they have originated from cell-free/nonviable DNA. The mean Sørensen coefficient for treated vs untreated samples was 0·527. Our findings suggest that the fetal gut is seeded with intact bacterial cells prior to birth. This is an important finding, as exposure to live bacteria during gestation might have a significant impact on the developing fetus. SIGNIFICANCE AND IMPACT OF THE STUDY: DNA-based microbiome studies performed using 16S rRNA gene sequencing are limited by their inability to discriminate between live bacterial cells, dead bacterial cells and cell-free DNA. Here we use propidium monoazide (PMA) to exclude nonviable bacteria from microbiome analysis of first-pass meconium samples and thereby reveal that the majority of the purported fetal gut microbiome is from intact bacterial cells. This work demonstrates the importance of excluding nonviable bacteria when analysing the microbial community in low-biomass samples such as meconium.

摘要

许多研究报告了首次排出的胎粪样本中存在细菌DNA,这表明人类肠道微生物群在出生前就已定植。然而,这些研究无法区分来自活细菌细胞的DNA、来自死细菌细胞的DNA或无细胞DNA。在这里,我们使用单叠氮碘化丙啶(PMA)结合16S rRNA基因测序来确定胎儿肠道中是否存在完整的细菌细胞。从首次排出的胎粪(n = 5)中提取DNA,并在有/无PMA处理的情况下进行16S rRNA基因测序。所有胎粪样本,无论是否经过PMA处理,都含有可检测水平的细菌DNA;然而,在DNA提取前用PMA处理会使DNA产量降低约20%。在观察到的OTU数量方面,PMA处理的胎粪样本与未处理的样本没有显著差异(P = 0·945);尽管它们在分类学上存在差异,约四分之一的OTU仅在未处理的样本中被鉴定出来,这表明它们源自无细胞/无活力的DNA。处理样本与未处理样本的平均索伦森系数为0·527。我们的研究结果表明,胎儿肠道在出生前就已接种了完整的细菌细胞。这是一项重要的发现,因为孕期接触活细菌可能会对发育中的胎儿产生重大影响。研究的意义和影响:使用16S rRNA基因测序进行的基于DNA的微生物组研究受到其无法区分活细菌细胞、死细菌细胞和无细胞DNA的限制。在这里,我们使用单叠氮碘化丙啶(PMA)从首次排出的胎粪样本的微生物组分析中排除无活力细菌,从而揭示所谓的胎儿肠道微生物群的大部分来自完整的细菌细胞。这项工作证明了在分析低生物量样本(如胎粪)中的微生物群落时排除无活力细菌的重要性。

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