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Fluorescence lifetime microscopy: a stimulated emission a

机译:荧光寿命显微镜:受激发射

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Abstract: The stimulated emission process has been rarely exploited in spectroscopy and microscopy. Instead, a spectroscopy method based on the pump-probe principle has been frequently used to observe picosecond and femtosecond processes. This common approach has not been applied to microscopy due to the relatively slow acquisition time and the lack of 3D information. We have exploited an idea originally proposed by F. Lytle group in which two pulsed lasers are simultaneously focused on the sample. One laser is used to excite a population of molecules and the second laser to induce stimulated emission. The stimulated radiation is carried away in the same direction of the stimulating laser beam. By collecting the fluorescence emission in other directions, we observe a modulation of the fluorescence signal as a function of the delay between the two laser pulses. The repetition rate of the two lasers is slightly different producing a frequency beating at the laser overlapping volume. We have extended this method to achieve very high spatial and temporal resolution in the microscope environment. By recording only the beating frequency, we obtain a 3D sectional effect similar to two-photon excitation. The harmonic content of the beating signal is limited by the laser pulse width and by the sample frequency response. Information of picosecond processes are extracted by standard frequency-domain methods. Using this principle, we built a stimulated emission microscope that has 3D and fluorescence lifetime capabilities.!34
机译:摘要:受激发射过程在光谱学和显微镜学中很少被利用。取而代之的是,基于泵浦探针原理的光谱方法已被经常用于观察皮秒和飞秒过程。由于相对较慢的采集时间和缺少3D信息,因此该通用方法尚未应用于显微镜检查。我们已经利用了F. Lytle小组最初提出的想法,其中两个脉冲激光同时聚焦在样品上。一种激光用于激发分子的聚集,另一种激光用于激发受激发射。被激发的辐射在与被激发的激光束相同的方向上被带走。通过收集其他方向的荧光发射,我们观察到荧光信号作为两个激光脉冲之间的延迟的函数的调制。两个激光器的重复率略有不同,从而在激光器重叠体积处产生频率跳动。我们扩展了此方法,以在显微镜环境中实现很高的时空分辨率。通过仅记录跳动频率,我们获得了类似于双光子激发的3D截面效果。跳动信号的谐波含量受激光脉冲宽度和采样频率响应限制。皮秒过程的信息是通过标准频域方法提取的。使用此原理,我们构建了具有3D和荧光寿命功能的受激发射显微镜。34

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