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Multimodal multiphoton microscopy

机译:多峰多光子显微镜

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摘要

Multiphoton microscopy is a powerful technique for high spatial resolution thick tissue imaging. In its simple version, it uses a high repetition rate femtosecond oscillator laser source focussed and scanned across biological sample that contains fluorophores. However, not every biological structure is inherently fluorescent or can be stained without causing biochemical changes. To circumvent these limitations, other non-invasive nonlinear optical imaging approaches are currently being developed and investigated with regard to different applications. These techniques are: (1) second harmonic generation (SHG), (2) third harmonic generation (THG), and (3) coherent anti-Stokes Raman scattering (CARS) microscopy. The main advantage of the above mentioned techniques is that they derive their imaging contrast from optical nonlinearities that do not involve fluorescence process. As a particular application example we investigated collagen arrays. We show that combining SHG-THG-CARS onto a single imaging platform provides complementary information about the sub-micron architecture of the tissue. SHG microscopy reveals the fibrillar architecture of collagen arrays and confirm a rather high degree of heterogeneity of χ~((2)) within the focal volume, THG highlights the boundaries between the collagen sheets, and CH_2 spectroscopic contrast with CARS.
机译:多光子显微镜技术是用于高空间分辨率厚组织成像的强大技术。在其简单版本中,它使用高重复率的飞秒振荡器激光源聚焦并扫描包含荧光团的生物样品。但是,并非每个生物结构都具有固有的荧光性或可以染色而不会引起生化变化。为了克服这些限制,目前正在针对不同的应用开发和研究其他非侵入性非线性光学成像方法。这些技术是:(1)二次谐波生成(SHG),(2)三次谐波生成(THG)和(3)相干抗斯托克斯拉曼散射(CARS)显微镜。上述技术的主要优点是它们从不涉及荧光过程的光学非线性中获得了它们的成像对比度。作为一个特殊的应用实例,我们研究了胶原蛋白阵列。我们显示,将SHG-THG-CARS组合到单个成像平台上可提供有关组织亚微米结构的补充信息。 SHG显微镜检查揭示了胶原蛋白阵列的原纤维结构,并证实了焦点体积内χ〜((2))的异质性相当高,THG突出显示了胶原蛋白薄片之间的边界,CH_2与CARS的光谱对比。

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