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

微生物 生物 固碳 稳定同位素探测 光合作用 显微拉曼光谱 莱茵衣藻 微生物种群生物学 微生物生态学 类胡萝卜素 细菌 环境化学 拉曼光谱 植物 生物化学 化学 突变体 物理 光学 基因 遗传学
作者
Mengqiu Li,Daniel P. Canniffe,Philip Jackson,Paul A. Davison,Simon FitzGerald,Mark J. Dickman,J. Grant Burgess,C. Neil Hunter,Wei E. Huang
出处
期刊:The ISME Journal [Springer Nature]
卷期号:6 (4): 875-885 被引量:99
标识
DOI:10.1038/ismej.2011.150
摘要

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.
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