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Reflectivity and topography of cells grown on glass-coverslips measured with phase-shifted laser feedback interference microscopy

机译:相移激光反馈干涉显微镜测量玻璃盖玻片上生长的细胞的反射率和形貌

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In spite of the advantages associated with the molecular specificity of fluorescence imaging, there is still a significant need to augment these approaches with label-free imaging. Therefore, we have implemented a form of interference microscopy based upon phase-shifted, laser-feedback interferometry and developed an algorithm that can be used to separate the contribution of the elastically scattered light by sub-cellular structures from the reflection at the coverslip-buffer interface. The method offers an opportunity to probe protein aggregation, index of refraction variations and structure. We measure the topography and reflection from calibration spheres and from stress fibers and adhesions in both fixed and motile cells. Unlike the data acquired with reflection interference contrast microscopy, where the reflection from adhesions can appear dark, our approach demonstrates that these regions have high reflectivity. The data acquired from fixed and live cells show the presence of a dense actin layer located ≈ 100 nm above the coverslip interface. Finally, the measured dynamics of filopodia and the lamella in a live cell supports retrograde flow as the dominate mechanism responsible for filopodia retraction.
机译:尽管与荧光成像的分子特异性相关联的优势,但仍然非常需要使用无标记成像来增强这些方法。因此,我们已经实现了一种基于相移,激光反馈干涉术的干涉显微镜形式,并开发了一种算法,该算法可用于将亚细胞结构的弹性散射光的贡献与盖玻片缓冲液的反射分开接口。该方法提供了探查蛋白质聚集,折射率变化和结构的机会。我们从定标球以及固定和活动细胞中的应力纤维和粘附力测量地形和反射。与通过反射干涉对比显微镜获得的数据不同,在这种情况下,来自粘连的反射可能会显得很暗,我们的方法表明这些区域具有高反射率。从固定细胞和活细胞获得的数据表明,在盖玻片界面上方约100 nm处有密集的肌动蛋白层。最后,在活细胞中测得的丝状伪足和片状动力学支持逆行流动,这是造成丝状伪足缩回的主要机制。

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