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Time-resolved polarization imaging by pump-probe (stimulated emission) fluorescence microscopy.

机译:时间分辨偏振成像通过泵浦探针(受激发射)荧光显微镜观察。

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摘要

We report the application of pump-probe fluorescence microscopy in time-resolved polarization imaging. We derived the equations governing the pump-probe stimulated emission process and characterized the pump and probe laser power levels for signal saturation. Our emphasis is to use this novel methodology to image polarization properties of fluorophores across entire cells. As a feasibility study, we imaged a 15-microm orange latex sphere and found that there is depolarization that is possibly due to energy transfer among fluorescent molecules inside the sphere. We also imaged a mouse fibroblast labeled with CellTracker Orange CMTMR (5-(and-6)-(((4-chloromethyl)benzoyl)amino)tetramethyl-rhodamine). We observed that Orange CMTMR complexed with gluthathione rotates fast, indicating the relatively low fluid-phase viscosity of the cytoplasmic microenvironment as seen by Orange CMTMR. The measured rotational correlation time ranged from approximately 30 to approximately 150 ps. This work demonstrates the effectiveness of stimulated emission measurements in acquiring high-resolution, time-resolved polarization information across the entire cell.
机译:我们报告了泵浦探针荧光显微镜在时间分辨偏振成像中的应用。我们推导了控制泵浦探针激发发射过程的方程式,并表征了泵浦和探针激光功率水平以实现信号饱和。我们的重点是使用这种新颖的方法对整个细胞上的荧光团的偏振特性进行成像。作为一项可行性研究,我们对15微米的橙色乳胶球成像,发现存在去极化,这可能是由于球内荧光分子之间的能量转移所致。我们还成像了用CellTracker Orange CMTMR(5-(and-6)-((((4-chloromethyl)benzoyl)amino)tetramethyl-rhodamine)标记的小鼠成纤维细胞。我们观察到与谷胱甘肽复合的Orange CMTMR旋转速度很快,表明Orange CMTMR所见的细胞质微环境的液相粘度相对较低。测得的旋转相关时间在大约30 ps至大约150 ps的范围内。这项工作证明了受激发射测量在获取整个电池上的高分辨率,时间分辨极化信息方面的有效性。

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