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Chemically Resolved Imaging of Biological Cells and Thin Films by Infrared Scanning Near-Field Optical Microscopy

机译:化学分辨成像的生物细胞和薄膜的红外扫描近场光学显微镜。

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摘要

The infrared (IR) absorption of a biological system can potentially report on fundamentally important microchemical properties. For example, molecular IR profiles are known to change during increases in metabolic flux, protein phosphorylation, or proteolytic cleavage. However, practical implementation of intracellular IR imaging has been problematic because the diffraction limit of conventional infrared microscopy results in low spatial resolution. We have overcome this limitation by using an IR spectroscopic version of scanning near-field optical microscopy (SNOM), in conjunction with a tunable free-electron laser source. The results presented here clearly reveal different chemical constituents in thin films and biological cells. The space distribution of specific chemical species was obtained by taking SNOM images at IR wavelengths (λ) corresponding to stretch absorption bands of common biochemical bonds, such as the amide bond. In our SNOM implementation, this chemical sensitivity is combined with a lateral resolution of 0.1 μm (≈λ/70), well below the diffraction limit of standard infrared microscopy. The potential applications of this approach touch virtually every aspect of the life sciences and medical research, as well as problems in materials science, chemistry, physics, and environmental research.
机译:生物系统的红外(IR)吸收可能会报告根本上重要的微化学性质。例如,已知分子IR分布在代谢通量增加,蛋白质磷酸化或蛋白水解裂解过程中发生变化。然而,由于常规红外显微镜的衍射极限导致低的空间分辨率,因此细胞内IR成像的实际实施存在问题。我们通过使用红外光谱版本的扫描近场光学显微镜(SNOM)以及可调谐的自由电子激光源,克服了这一限制。此处呈现的结果清楚地揭示了薄膜和生物细胞中的不同化学成分。通过在对应于常见生物化学键(如酰胺键)的拉伸吸收带的IR波长(λ)上拍摄SNOM图像,可以获得特定化学物质的空间分布。在我们的SNOM实施中,这种化学敏感性与0.1μm(≈λ/ 70)的横向分辨率相结合,远低于标准红外显微镜的衍射极限。这种方法的潜在应用几乎涉及生命科学和医学研究的各个方面,以及材料科学,化学,物理和环境研究中的问题。

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