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细菌表面增强拉曼散射光谱中约 730cm(-1) 波段的起源:一种稳定同位素方法。

The origin of the band at around 730 cm(-1) in the SERS spectra of bacteria: a stable isotope approach.

机构信息

Technical University of Munich, Institute of Hydrochemistry, Chair of Analytical Chemistry, Marchioninistr. 17, 81377 Munich, Germany.

出版信息

Analyst. 2016 May 10;141(10):2874-8. doi: 10.1039/c6an00306k.

Abstract

Raman microspectroscopy is an emerging tool to analyze the molecular and isotopic composition of single microbial cells. It can be used to achieve an in situ understanding of metabolic processes. Due to the low sensitivity of the Raman effect, surface-enhanced Raman scattering (SERS) is utilized to enhance the Raman signal. The SERS spectra of bacteria are usually characterized by a pronounced band at around 730 cm(-1), which is assigned to glycosidic ring vibrations or to adenine or even to CH2 deformation in different studies. In order to clarify the origin of this band, we employed a stable isotope approach and performed a SERS analysis of Escherichia coli bacteria using in situ prepared Ag nanoparticles. The cells were grown on unlabeled ((12)C, (14)N) and labeled ((13)C, (15)N) carbon and nitrogen sources in different combinations. The SERS band of the stable isotope labeled microorganisms showed a characteristic red-shift in the SERS spectra, which solely depends on the isotopic composition. It was therefore possible to confidently assign this band to adenine-related compounds. Furthermore, by utilizing the fingerprint area of single-cell SERS spectra as the input for the principal component analysis, one can clearly differentiate between E. coli bacteria incorporating different stable isotopes.

摘要

拉曼微光谱学是一种新兴的工具,可用于分析单个微生物细胞的分子和同位素组成。它可以用于实现对代谢过程的原位理解。由于拉曼效应的灵敏度较低,因此利用表面增强拉曼散射(SERS)来增强拉曼信号。细菌的 SERS 光谱通常具有约 730 cm(-1) 处的明显带,在不同的研究中,该带被分配给糖苷环振动或腺嘌呤,甚至是 CH2 变形。为了澄清该带的起源,我们采用了稳定同位素方法,并使用原位制备的 Ag 纳米粒子对大肠杆菌进行了 SERS 分析。将细胞在未标记的((12)C,(14)N)和标记的((13)C,(15)N)碳和氮源的不同组合中生长。稳定同位素标记的微生物的 SERS 带在 SERS 光谱中显示出特征的红移,该红移仅取决于同位素组成。因此,可以将该带明确分配给与腺嘌呤有关的化合物。此外,通过将单细胞 SERS 光谱的指纹区域用作主成分分析的输入,可以清楚地区分吸收不同稳定同位素的大肠杆菌。

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