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使用共聚焦显微镜对完整肾小体中钙处理进行实时成像。

Real-time Imaging of Ca-handling in Intact Renal Glomeruli Using Confocal Microscopy.

作者信息

Ghayur Muhammad Nabeel, Janssen Luke Jeffrey

机构信息

Department of Medicine, McMaster University, St. Joseph's Hospital, Hamilton, Ontario, Canada.

出版信息

Med Hypotheses Res. 2009 Jul;5(1/2):47-56.

Abstract

Glomeruli are filtering units in the kidneys. Being multicellular and complex in structure, many aspects of glomerular function are yet to be elucidated. Most studies use glomerular cells in culture, which may exhibit altered physiology compared to native cells. Confocal microscopy has opened new avenues in exploring in situ glomerular function and physiology. In this report, we propose experimenting with glomerular cells in renal cortical slices and isolated intact glomeruli for Ca(2+)-handling studies. Cortical slices (100 μm thick) were obtained from mice while intact glomeruli were isolated from rats using the sieving method. These were loaded with fluo-4 and then placed in a confocal microscope. Fluo-4 was excited using a 488 nm photodiode laser and images were collected at 1 frame/sec. Changes in average fluorescence intensity (AFI) were interpreted as changes in Ca(2+). AFI increased to 37.1 ± 6.7% and 84.3 ± 20.9% with Ang II (0.01 and 0.1 μM respectively). Norepinephrine (10 μM), arginine vasopressin (0.1 μM) and K(+) (30 mM) also elevated AFI by 26.5 ± 6.8%, 22.3 ± 1.0% and 39.8 ± 10.3% respectively in the glomerular cells. Likewise in isolated glomeruli, Ang II (0.1-10 μM), K(+) (30-90 mM) and endothelin-1 (0.01-1 μM), all showed elevation in Ca(2+). These results give an impetus for future studies examining Ca(2+)-handling by confocal microscopy in glomerular cells using renal cortical slices and isolated intact glomeruli. The results support the utility of this system for study of glomerular physiology and pharmacology.

摘要

肾小球是肾脏中的滤过单位。由于其结构多细胞且复杂,肾小球功能的许多方面仍有待阐明。大多数研究使用培养的肾小球细胞,与天然细胞相比,这些细胞可能表现出生理变化。共聚焦显微镜为探索原位肾小球功能和生理学开辟了新途径。在本报告中,我们建议对肾皮质切片中的肾小球细胞和分离的完整肾小球进行实验,以研究钙离子处理。从小鼠获取皮质切片(100μm厚),同时使用筛分法从大鼠分离完整肾小球。将这些组织装载荧光素-4,然后置于共聚焦显微镜下。使用488nm光电二极管激光激发荧光素-4,并以每秒1帧的速度采集图像。平均荧光强度(AFI)的变化被解释为细胞内钙离子浓度(Ca(2+))的变化。使用血管紧张素II(分别为0.01和0.1μM)时,AFI分别增加到37.1±6.7%和84.3±20.9%。去甲肾上腺素(10μM)、精氨酸加压素(0.1μM)和钾离子(30mM)也分别使肾小球细胞中的AFI升高26.5±6.8%、22.3±1.0%和39.8±10.3%。同样,在分离的肾小球中,血管紧张素II(0.1 - 10μM)、钾离子(30 - 90mM)和内皮素-1(0.01 - 1μM)均显示细胞内钙离子浓度升高。这些结果为未来使用肾皮质切片和分离的完整肾小球通过共聚焦显微镜研究肾小球细胞钙离子处理的研究提供了动力。结果支持该系统在肾小球生理学和药理学研究中的实用性。

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