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In vivo Conf ocal Laser Scanning Microscopy and Micropuncture in Intact Rat

机译:完整大鼠体内活体激光扫描显微镜和显微穿刺

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Background: Intravital microscopy theoretically provides the optimal conditions for studying specific organ functions. However, the application of microscopy in intact organs in vivo has been limited so far due to technical difficulties. The purpose of this study was to establish a method of in vivo confocal laser scanning microscopy (CLSM) for the study of endocytosis in proximal tubules of intact kidney. Methods: The left kidney of rats placed on a modified microscope stage was exposed and stabilized in a thermostatically controlled cup. The stage was then attached to an upright confocal microscope. Surface proximal tubules were microinfused with fluorescent albumin or transferrin. Single or time-series images of microinfused proximal tubules were recorded in reflection and/or fluorescence mode. Results: The stability of the kidney and the resolution of images were sufficient to visualize intracellular vesicles. Albumin and transferrin were initially observed at the brush border, then later internalized by proximal tubules and accumulated in lysosomes over a time period of 15 min. Furthermore, fusion of vesicles was observed in time-lapse images. Conclusion: These results show that in vivo CLSM in intact kidney may be an excellent method to evaluate proximal tubular endocytosis and ligand trafficking.
机译:背景:玻璃体内显微镜理论上为研究特定器官功能提供了最佳条件。然而,由于技术上的困难,迄今为止在活体完整器官中显微术的应用受到限制。这项研究的目的是建立一种体内共聚焦激光扫描显微镜(CLSM)的方法,用于研究完整肾脏近端小管的内吞作用。方法:将大鼠置于改良显微镜下的左肾暴露于恒温杯中并稳定。然后将载物台连接到直立共聚焦显微镜上。将表面近端小管微注入荧光白蛋白或转铁蛋白。显微注射近端小管的单次或时序图像以反射和/或荧光模式记录。结果:肾脏的稳定性和图像的分辨率足以可视化细胞内囊泡。最初在刷状缘观察到白蛋白和转铁蛋白,然后在近端小管内化,并在15分钟的时间内积聚在溶酶体中。此外,在延时图像中观察到囊泡融合。结论:这些结果表明完整肾脏中的体内CLSM可能是评估近端肾小管内吞作用和配体运输的极好方法。

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