State-of-the-art approaches in the investigation of human seminal bacteriome using metagenomic methods.

IF 2.3 Q2 PUBLIC, ENVIRONMENTAL & OCCUPATIONAL HEALTH
Frontiers in reproductive health Pub Date : 2025-06-05 eCollection Date: 2025-01-01 DOI:10.3389/frph.2025.1557912
Jan Hofman, Petra Brenerova, Petra Borilova Linhartova
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引用次数: 0

Abstract

Although the understanding of the causes of infertility is the key to its successful treatment, recent studies have shown that as many as 50% of male-caused infertility cases are considered idiopathic. The microbial colonization of the male reproductive system was shown to be associated with reduced male reproductive fitness. Investigation of the seminal microbiome, however, remains challenging. This article aimed to improve this situation by creating the first comprehensive review of literature on the metagenomic methods (including the pre-analytical and analytical approaches) used in the research on human seminal bacteriome (total bacterial DNA in the matrix), published in 2018-2024. A total of 29 studies addressing the analysis of the human seminal bacteriome were identified. The analysis typically involved DNA extraction from the supernatant using commercial kits, amplification of the gene for 16S rRNA, and sequencing of amplicons. Where the separation of seminal plasma was performed, centrifugation was the dominant method used for this purpose. The significant heterogeneity in individual steps of methodological approaches in the analysis of the human seminal bacteriome complicates the comparison of results among studies and the establishment of standard procedures, hindering clinical advancements. For this reason, a protocol for the analysis of the human seminal plasma bacteriome is proposed here, which could lead to improved comparability of results among studies and make future research more efficient. This protocol is founded on rigorous quality control measures, compliance with the WHO laboratory manual for sample collection, extensive pretreatment involving mechanical and enzymatic lysis, DNA extraction using the QIAamp DNA Mini Kit (Qiagen), and short-read sequencing conducted on the MiSeq platform (Illumina).

使用宏基因组方法研究人类精液细菌组的最新方法。
虽然了解不育的原因是成功治疗的关键,但最近的研究表明,多达50%的男性引起的不育病例被认为是特发性的。男性生殖系统的微生物定植被证明与男性生殖适应性降低有关。然而,对精液微生物组的研究仍然具有挑战性。本文旨在通过对2018-2024年发表的关于人类精液细菌组(基质中总细菌DNA)研究中使用的宏基因组方法(包括前分析方法和分析方法)的文献进行首次全面综述,从而改善这种情况。共有29项研究涉及人类精液细菌群的分析。分析通常包括使用商业试剂盒从上清中提取DNA,扩增16S rRNA基因,并对扩增子进行测序。在进行精浆分离的地方,离心是用于此目的的主要方法。在分析人类精液细菌组的方法学方法中,各个步骤的显著异质性使研究结果的比较和标准程序的建立复杂化,阻碍了临床进步。因此,本文提出了一种分析人类精浆细菌组的方案,可以提高研究结果之间的可比性,提高未来研究的效率。本方案建立在严格的质量控制措施的基础上,符合世卫组织样本采集实验室手册,包括机械和酶解的广泛预处理,使用QIAamp DNA Mini Kit (Qiagen)提取DNA,并在MiSeq平台(Illumina)上进行短读测序。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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CiteScore
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审稿时长
13 weeks
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