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线扫描拉曼显微镜用于细胞群体高通量化学成像的性能

Performance of line-scan Raman microscopy for high-throughput chemical imaging of cell population.

作者信息

Qi Ji, Shih Wei-Chuan

出版信息

Appl Opt. 2014 May 1;53(13):2881-5. doi: 10.1364/AO.53.002881.

Abstract

We evaluate the performance of line-scan Raman microscopy (LSRM), a versatile label-free technique, for high-throughput chemical imaging of cell population. We provide detailed design and configuration of a home-built LSRM system developed in our laboratory. By exploiting parallel acquisition, the LSRM system achieves a significant throughput advantage over conventional point-scan Raman microscopy by projecting a laser line onto the sample and imaging the Raman scattered light from the entire line using a grating spectrograph and a charge-coupled device (CCD) camera. Two-dimensional chemical maps can be generated by scanning the projected line in the transverse direction. The resolution in the x and y direction has been characterized to be ~600-800 nm for 785 nm laser excitation. Our system enables rapid classification of microparticles with similar shape, size, and refractive index based on their chemical composition. An equivalent imaging throughput of 100 microparticles/s for 1 μm polystyrene beads has been achieved. We demonstrate the application of LSRM to imaging bacterial spores by identifying endogenous calcium dipicolinate. We also demonstrate that LSRM enables the study of intact microalgal cells at the colonial level and the identification of intra- and extracellular chemical constituents and metabolites, such as chlorophyll, carotenoids, lipids, and hydrocarbons. We conclude that LSRM can be an effective and practical tool for obtaining endogenous microscopic chemical and molecular information from cell population.

摘要

我们评估了线扫描拉曼显微镜(LSRM)这种通用的无标记技术在细胞群体高通量化学成像方面的性能。我们详细介绍了在我们实验室开发的自制LSRM系统的设计和配置。通过利用并行采集,LSRM系统通过将激光线投射到样品上,并使用光栅光谱仪和电荷耦合器件(CCD)相机对来自整条线的拉曼散射光进行成像,从而比传统的点扫描拉曼显微镜具有显著的通量优势。通过在横向扫描投射的线可以生成二维化学图谱。对于785 nm激光激发,x和y方向的分辨率已被表征为约600 - 800 nm。我们的系统能够根据微粒的化学成分对形状、大小和折射率相似的微粒进行快速分类。对于1μm的聚苯乙烯珠,已实现了100个微粒/秒的等效成像通量。我们通过鉴定内源性吡啶二羧酸钙证明了LSRM在细菌孢子成像中的应用。我们还证明了LSRM能够在群体水平上研究完整的微藻细胞,并鉴定细胞内和细胞外的化学成分和代谢物,如叶绿素、类胡萝卜素、脂质和碳氢化合物。我们得出结论,LSRM可以成为从细胞群体中获取内源性微观化学和分子信息的有效且实用的工具。

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