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拉曼镊子对单个微生物细胞的分选。

Raman tweezers sorting of single microbial cells.

机构信息

Molecular Microbial Ecology, CEH-Oxford, Mansfield Road, Oxford OX1 3SR, UK. Science and Technology Facilities Council, Rutherford Appleton Laboratory, Harwell Science and Innovation Campus, Didcot OX11 0QX, UK.

出版信息

Environ Microbiol Rep. 2009 Feb;1(1):44-9. doi: 10.1111/j.1758-2229.2008.00002.x.

DOI:10.1111/j.1758-2229.2008.00002.x
PMID:23765719
Abstract

We have selectively isolated microbial cells by identifying and then manipulating cells using a combination of Raman microspectroscopy and optical trapping. The criterion for cell discrimination is based on spectral peak shifts within the Raman spectrum of individual cells. A specific shift in the phenylalanine peak position from 1001 rel. cm(-1) to 965 rel. cm(-1) is utilized to indicate the uptake of (13) C within the cell that utilized (13) C-substrate. Cells were captured and manipulated using an infrared (1064 nm) laser while Raman spectra were acquired over shorter timescales (30 s) using a co-aligned 514.5 nm laser beam. Selected cells were manoeuvred to a clean part of a capillary tube and the tubes were cleaved to physically separate the cells. The technique was tested for cell viability and cross-contamination effects using 70 single yeast cells (Saccharomyces cerevisia). Following these tests, 58 single bacterial cells (Escherichia coli DH5α, and Pseudomonas fluorescens SBW25::Km-RFP) that exhibited (13) C uptake were sorted from bacterial populations. Among those isolated cells, 11 out of 18 yeast cells and 7 out of 18 single SBW25::Km-RFP cells were recovered by incubation; 2 out of 7 sorted yeast cells and 3 out of 8 sorted bacterial cells (single SBW25::Km-RFP) were genome amplified correctly. We show that the Raman tweezers approach has the potential to open a new frontier to study unculturable microorganisms, which account for more than 99% microbes in natural environment.

摘要

我们通过结合使用拉曼微光谱和光学捕获技术,选择性地分离微生物细胞,通过识别和操作细胞。细胞鉴别标准基于单个细胞的拉曼光谱中的谱峰位移。细胞内利用 (13)C 底物时苯丙氨酸峰位置从 1001 rel. cm(-1) 到 965 rel. cm(-1) 的特定位移被用来指示这一情况。细胞通过红外 (1064 nm) 激光捕获和操作,而拉曼光谱在更短的时间尺度(30 秒)内通过共准直的 514.5 nm 激光束获得。选择的细胞被操纵到毛细管的干净部分,然后将管子切割以物理分离细胞。该技术使用 70 个单个酵母细胞(酿酒酵母)进行了细胞活力和交叉污染影响的测试。进行这些测试后,从细菌群体中分拣出 58 个表现出 (13)C 摄取的单个细菌细胞(大肠杆菌 DH5α 和荧光假单胞菌 SBW25::Km-RFP)。在这些分离的细胞中,18 个酵母细胞中有 11 个,18 个 SBW25::Km-RFP 细胞中有 7 个通过孵育回收;7 个分选酵母细胞中有 2 个,8 个分选细菌细胞(单个 SBW25::Km-RFP)中有 3 个正确进行了基因组扩增。我们表明,拉曼镊子方法有可能开创一个研究不可培养微生物的新领域,这些微生物在自然环境中占 99%以上的微生物。

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