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Looking inside the box: using Raman microspectroscopy to deconstruct microbial biomass stoichiometry one cell at a time.深入研究微生物细胞内物质组成:利用拉曼微光谱技术逐细胞解析微生物生物量化学计量。
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利用快速共振拉曼微光谱技术探测微生物群落中单细胞固定二氧化碳的情况。

Rapid resonance Raman microspectroscopy to probe carbon dioxide fixation by single cells in microbial communities.

机构信息

Department of Civil and Structural Engineering, Kroto Research Institute, University of Sheffield, Sheffield, UK.

出版信息

ISME J. 2012 Apr;6(4):875-85. doi: 10.1038/ismej.2011.150. Epub 2011 Nov 24.

DOI:10.1038/ismej.2011.150
PMID:22113377
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3309358/
Abstract

Photosynthetic microorganisms play crucial roles in aquatic ecosystems and are the major primary producers in global marine ecosystems. The discovery of new bacteria and microalgae that play key roles in CO(2) fixation is hampered by the lack of methods to identify hitherto-unculturable microorganisms. To overcome this problem we studied single microbial cells using stable-isotope probing (SIP) together with resonance Raman (RR) microspectroscopy of carotenoids, the light-absorbing pigments present in most photosynthetic microorganisms. We show that fixation of (13)CO(2) into carotenoids produces a red shift in single-cell RR (SCRR) spectra and that this SCRR-SIP technique is sufficiently sensitive to detect as little as 10% of (13)C incorporation. Mass spectrometry (MS) analysis of labelled cellular proteins verifies that the red shift in carotenoid SCRR spectra acts as a reporter of the (13)C content of single cells. Millisecond Raman imaging of cells in mixed cultures and natural seawater samples was used to identify cells actively fixing CO(2), demonstrating that the SCRR-SIP is a noninvasive method for the rapid and quantitative detection of CO(2) fixation at the single cell level in a microbial community. The SCRR-SIP technique may provide a direct method for screening environmental samples, and could help to reveal the ecophysiology of hitherto-unculturable microorganisms, linking microbial species to their ecological function in the natural environment.

摘要

光合微生物在水生生态系统中起着至关重要的作用,是全球海洋生态系统中主要的初级生产者。由于缺乏识别迄今无法培养的微生物的方法,新的在 CO(2)固定中起关键作用的细菌和微藻的发现受到了阻碍。为了解决这个问题,我们使用稳定同位素探测(SIP)和类胡萝卜素的共振拉曼(RR)微光谱学研究了单个微生物细胞,类胡萝卜素是大多数光合微生物中存在的吸光色素。我们表明,(13)CO(2)固定到类胡萝卜素中会导致单细胞 RR(SCRR)光谱发生红移,并且这种 SCRR-SIP 技术足够灵敏,可以检测到低至 10%的(13)C 掺入。对标记细胞蛋白的质谱(MS)分析验证了类胡萝卜素 SCRR 光谱的红移可以作为单个细胞(13)C 含量的报告器。混合培养物和天然海水样本中细胞的毫秒级拉曼成像用于鉴定正在积极固定 CO(2)的细胞,表明 SCRR-SIP 是一种在微生物群落中单细胞水平快速定量检测 CO(2)固定的非侵入性方法。SCRR-SIP 技术可能为筛选环境样本提供一种直接的方法,并有助于揭示迄今无法培养的微生物的生态生理学,将微生物物种与其在自然环境中的生态功能联系起来。