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培养的少突胶质细胞的扫描近场光学显微镜成像的新方法。

Novel approaches for scanning near-field optical microscopy imaging of oligodendrocytes in culture.

机构信息

University of Trieste, Clinical Department of Biomedicine, Via Manzoni 16, Trieste, Italy.

出版信息

Neuroimage. 2010 Jan 1;49(1):517-24. doi: 10.1016/j.neuroimage.2009.07.035. Epub 2009 Jul 24.

Abstract

Newborn rat oligodendrocyte cultures were investigated by scanning near-field optical microscope (SNOM), a versatile new tool able to map cell membranes in 3D and simultaneously obtain images of the cytoplasm. Topography, error, transmission and reflection signals were acquired to describe cell morphology with nanometer-scale resolution. Oligodendrocytes were studied as a model because their extensive membrane processes (typical of their physiological role in myelination) made them particularly suitable to test the sensitivity of the new method. Furthermore, we combined a classical histochemical method with SNOM, to identify specific intracellular proteins at high definition. In particular, with this technique, cytoskeleton elements of oligodendrocytes, such as microtubules, were observed with tubulin antibodies. Images obtained with SNOM were also compared with those from conventional scanning electron microscopy (SEM) and optical microscopy. Our results showed that SNOM allowed to observe cell nanostructures otherwise undetectable all together with other microscopies. In conclusion, SNOM, combined with rapid and non-invasive methods of specimen preparation, appears to be a powerful tool that can offer new possibilities in the field of neuroscience imaging at nano-scale level.

摘要

新生大鼠少突胶质细胞培养物通过扫描近场光学显微镜(SNOM)进行研究,这是一种多功能的新工具,能够在 3D 中绘制细胞膜,并同时获得细胞质的图像。形貌、误差、传输和反射信号被获取,以纳米级分辨率描述细胞形态。少突胶质细胞被用作模型,因为它们广泛的膜过程(这是它们在髓鞘形成中的生理作用的典型特征)使它们特别适合测试新方法的灵敏度。此外,我们将经典的组织化学方法与 SNOM 相结合,以高清晰度识别特定的细胞内蛋白质。特别是,使用这种技术,可以用微管蛋白抗体观察到少突胶质细胞的细胞骨架元素,如微管。使用 SNOM 获得的图像也与传统的扫描电子显微镜(SEM)和光学显微镜获得的图像进行了比较。我们的结果表明,SNOM 允许观察到其他显微镜无法一起检测到的细胞纳米结构。总之,SNOM 与标本制备的快速和非侵入性方法相结合,似乎是一种强大的工具,可以在纳米尺度的神经科学成像领域提供新的可能性。

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