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从土壤和沉积物中的细菌芽孢中灵敏定量分析二吡咯羧酸。

Sensitive quantification of dipicolinic acid from bacterial endospores in soils and sediments.

机构信息

Department of Biological Sciences, University of Calgary, Calgary, T2N 1N4, Canada.

Department of Geoscience, University of Calgary, Calgary, T2N 1N4, Canada.

出版信息

Environ Microbiol. 2021 Mar;23(3):1397-1406. doi: 10.1111/1462-2920.15343. Epub 2020 Dec 21.

Abstract

Endospore-forming bacteria make up an important and numerically significant component of microbial communities in a range of settings including soils, industry, hospitals and marine sediments extending into the deep subsurface. Bacterial endospores are non-reproductive structures that protect DNA and improve cell survival during periods unfavourable for bacterial growth. An important determinant of endospores withstanding extreme environmental conditions is 2,6-pyridine dicarboxylic acid (i.e. dipicolinic acid, or DPA), which contributes heat resistance. This study presents an improved HPLC-fluorescence method for DPA quantification using a single 10-min run with pre-column Tb chelation. Relative to existing DPA quantification methods, specific improvements pertain to sensitivity, detection limit and range, as well as the development of new free DPA and spore-specific DPA proxies. The method distinguishes DPA from intact and recently germinated spores, enabling responses to germinants in natural samples or experiments to be assessed in a new way. DPA-based endospore quantification depends on accurate spore-specific DPA contents, in particular, thermophilic spores are shown to have a higher DPA content, meaning that marine sediments with plentiful thermophilic spores may require spore number estimates to be revisited. This method has a wide range of potential applications for more accurately quantifying bacterial endospores in diverse environmental samples.

摘要

形成芽孢的细菌在包括土壤、工业、医院和海洋沉积物在内的一系列环境中,是微生物群落的重要且数量众多的组成部分,并延伸到深部地下。细菌芽孢是一种非繁殖结构,可在不利于细菌生长的时期保护 DNA 并提高细胞存活率。芽孢能耐受极端环境条件的一个重要决定因素是 2,6-吡啶二羧酸(即吡啶二羧酸,或 DPA),它有助于提高耐热性。本研究提出了一种使用Tb 螯合的单个 10 分钟预柱运行进行 DPA 定量的改进 HPLC-荧光方法。与现有的 DPA 定量方法相比,该方法在灵敏度、检测限和范围方面都有具体的改进,并且开发了新的游离 DPA 和芽孢特异性 DPA 探针。该方法可区分 DPA 与完整和最近发芽的芽孢,从而可以以新的方式评估天然样品或实验中的发芽剂的响应。基于 DPA 的芽孢定量取决于准确的芽孢特异性 DPA 含量,特别是嗜热芽孢的 DPA 含量较高,这意味着富含嗜热芽孢的海洋沉积物可能需要重新估算芽孢数量。该方法具有广泛的潜在应用,可更准确地定量不同环境样品中的细菌芽孢。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8311/8048543/f1a8e4ad4356/EMI-23-1397-g003.jpg

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