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建立用于微生物组研究的标准化舌涂层采集方法。

Establishment of a Standard Tongue Coating Collection Method for Microbiome Studies.

机构信息

State Key Laboratory of Dampness Syndrome of Chinese Medicine, The Second Affiliated Hospital of Guangzhou University of Chinese Medicine, Guangzhou, China.

Medical Research Center, Huazhong University of Science and Technology Union Shenzhen Hospital, Shenzhen, China.

出版信息

Biopreserv Biobank. 2023 Dec;21(6):599-609. doi: 10.1089/bio.2022.0113. Epub 2023 Feb 2.

Abstract

Recently, researchers have been focusing on characterizing the tongue coating microbiome from patients with digestive tract disease. However, to the best of our knowledge, the tongue coating collection methods have not been standardized until now. This article focuses on bridging this gap by exploring and validating the conditions suitable for the collection of tongue coating samples. One hundred forty-one healthy subjects were involved in the standardization of the tongue coating collection method. We conducted our standardization experiment by comparing different sampling tools, different preservation solutions, different scraping times, and different storage days with preservation at room temperature. The tongue coating samples from 59 normal individuals were analyzed using 16S ribosomal RNA (rRNA) gene-sequencing technology. The assessment of the quality of extracted DNA was used to verify our established method. We separated the 59 subjects into two groups (aged and younger), and the sequencing results were used to explore the age-related changes in microbiome. Sterile oral swab B is suitable for the collection of tongue coating samples. To obtain a sufficient amount of DNA from a tongue coating sample, we recommend 30 times of tongue coating scraping. Normal saline, phosphate-buffered saline, and commercial preservation solution are all suitable for short-term sample storage (<1 hour). The commercial long-term preservation solution, which stores samples at room temperature (0 hour to 7 days) and can provide for fast commercial transportation, ensures the integrity of the sample DNA as well as the stability of the DNA quality. By using the established method, extracted DNA from all the 59 normal individuals' tongue coating samples passed an appropriate quality bar for microbiome studies. The average value of OD 260/280 is 1.72 ± 0.10; the average total DNA amount is 334.92 ng (±183.81 ng). The bacterial diversity of the tongue coating is increased and the bacterial community composition changes greatly in the NC group (aged normal subjects). Fusobacteriota is found as the dominant bacteria phyla in aged normal subjects with the 16S rRNA gene-sequencing technology. At the genus level, the relative abundance of Fusobacterium, Haemophilus, and Leptotrichia are significantly higher in aged individuals (all  < 0.05), and Neisseria, Streptococcus, and Porphyromonas are significantly higher in younger individuals (all  < 0.05). A participant-friendly tongue coating collection method for microbiome analyses can be established with good reliability and reproducibility. By taking advantage of our established method and 16S rRNA gene sequencing, significant differences were found in diversity and composition of tongue coating microbiota between aged and younger individuals, which contributes to a better understanding of the age-related composition of tongue coating microbiota.

摘要

最近,研究人员一直专注于描述消化道疾病患者的舌涂层微生物组。然而,据我们所知,到目前为止,还没有标准化的舌涂层采集方法。本文通过探索和验证适合采集舌涂层样本的条件来解决这一差距。

141 名健康受试者参与了舌涂层采集方法的标准化。我们通过比较不同的采样工具、不同的保存溶液、不同的刮擦次数和不同的储存天数(在室温下保存)来进行标准化实验。使用 16S 核糖体 RNA(rRNA)基因测序技术分析了 59 名正常个体的舌涂层样本。提取 DNA 的质量评估用于验证我们建立的方法。我们将 59 名受试者分为两组(年龄较大和年龄较小),并使用测序结果探索微生物组与年龄相关的变化。

无菌口腔拭子 B 适合采集舌涂层样本。为了从舌涂层样本中获得足够量的 DNA,我们建议进行 30 次舌涂层刮擦。生理盐水、磷酸盐缓冲盐水和商业保存溶液都适合短期样本储存(<1 小时)。商业长期保存溶液可在室温下储存样本(0 小时至 7 天),并可提供快速商业运输,确保样本 DNA 的完整性和 DNA 质量的稳定性。使用建立的方法,所有 59 名正常个体的舌涂层样本的提取 DNA 都通过了微生物组研究的适当质量标准。OD260/280 的平均值为 1.72±0.10;总 DNA 量的平均值为 334.92ng(±183.81ng)。使用 16S rRNA 基因测序技术发现,NC 组(年龄较大的正常受试者)中舌涂层的细菌多样性增加,细菌群落组成发生了很大变化。厚壁菌门被发现是年龄较大的正常受试者的优势细菌门。在属水平上,变形菌属、嗜血杆菌属和勒特氏菌属的相对丰度在年龄较大的个体中显著较高(均<0.05),而奈瑟菌属、链球菌属和卟啉单胞菌属在年龄较小的个体中显著较高(均<0.05)。

可以建立一种参与者友好的用于微生物组分析的舌涂层采集方法,具有良好的可靠性和可重复性。利用我们建立的方法和 16S rRNA 基因测序,发现年龄较大和年龄较小个体之间的舌涂层微生物组多样性和组成存在显著差异,这有助于更好地了解年龄相关的舌涂层微生物组组成。

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