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Two-photon excited fluorescence microscopy combined with spectral and time-resolved measurements for fluorophore identification

机译:双光子激发荧光显微镜结合荧光团鉴定的光谱和时间分辨测量

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Two-photon excited fluorescence microscopy was used to study unstained tissue and paper samples. As an excitation source a mode-locked Ti:Sapphire laser was utilized. In the experiments we used a conventional fluorescence microscope with a scanning board. The incoming laser pulses were focused onto the sample and the epifluorescence observed. In the spectroscopic measurements the fluorescence light was projected either on the slit of an polychromator with a CCD camera or, in some experiments, on a streak camera connected to the polychromator. The signal was then detected by a 2D-CCD camera. Fluorescence images were scanned by recording the fluorescence light pixel by pixel with a photomultiplier tube. Signal filtering and image processing were performed on a personal computer. Tissue samples from animals treated with photodynamic therapy were examined. The tissue contained protoporphyrin IX as a photosensitizer.
机译:双光子激发荧光显微镜用于研究未染色的组织和纸样品。作为激励源,使用模式锁定的Ti:使用蓝宝石激光。在实验中,我们使用具有扫描板的常规荧光显微镜。进入的激光脉冲聚焦到样品上并观察到ePiforegence。在光谱测量中,荧光灯在具有CCD摄像机的多色仪的狭缝上突出,或者在一些实验中,在连接到多色机的条纹相机上。然后通过2D-CCD相机检测信号。通过用光电倍增管通过像素记录荧光光像素来扫描荧光图像。在个人计算机上执行信号滤波和图像处理。检查了用光动力疗法治疗的动物的组织样品。组织含有原子卟啉IX作为光敏剂。

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