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Vibrational imaging of lipid droplets in live fibroblast cells with coherent anti-Stokes Raman scattering microscopy

机译:具有相干抗风细胞的活性成纤维细胞脂肪液滴的振动成像,具有连贯的抗刺激拉曼散射显微镜

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摘要

A new vibrational imaging method based on coherent anti-Stokes Raman scattering (CARS) has been used for high-speed, selective imaging of neutral lipid droplets (LDs) in unstained live fibroblast cells. LDs have a high density of C-H bonds and show a high contrast in laser-scanning CARS images taken at 2,845 cm−1, the frequency for aliphatic C-H vibrations. The contrast from LDs was confirmed by comparing CARS and Oil Red O (ORO)-stained fluorescence images. The fluorescent labeling processes were examined with CARS microscopy. It was found that ORO staining of fixed cells caused aggregation of LDs, whereas fixing with formaldehyde or staining with Nile Red did not affect LDs. CARS microscopy was also used to monitor the 3T3-L1 cell differentiation process, revealing that there was an obvious clearance of LDs at the early stage of differentiation. After that, the cells started to differentiate and reaccumulate LDs in the cytoplasm in a largely unsynchronized manner. Differentiated cells formed small colonies surrounded by undifferentiated cells that were devoid of LDs.These observations demonstrate that CARS microscopy can follow dynamic changes in live cells with chemical selectivity and noninvasiveness. CARS microscopy, in tandem with other techniques, provides exciting possibilities for studying LD dynamics under physiological conditions without perturbation of cell functions.
机译:一种新的基于相干抗Stokes拉曼散射(汽车)的振动成像方法已被用于未染色的活成纤维细胞中中性脂液滴(LDS)的高速,选择性成像。 LDS具有高密度的C-H键,并在激光扫描汽车图像中显示出在2,845cm-1的激光扫描图像中的高对比度,脂肪族C-H振动的频率。通过比较汽车和油红O(ORO) - 染色的荧光图像来确认来自LDS的对比。用汽车显微镜检查荧光标记过程。结果发现固定细胞的ORO染色引起LD的聚集,而用甲醛或用尼罗红染色的固定不会影响LDS。汽车显微镜也用于监测3T3-L1细胞分化过程,揭示了分化早期的LDS清除。之后,细胞开始以极大的不同步方式在细胞质中分化和重新升温LD。分化的细胞形成了未分化的细胞包围的小菌落,这些细胞缺乏LDS。这些观察结果表明,汽车显微镜可以遵循具有化学选择性和非侵入性活细胞的动态变化。与其他技术的串联汽车显微镜提供了在没有细胞功能的情况下在没有扰乱的情况下在生理条件下学习LD动力学的激动令人兴奋的可能性。

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