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Two-photon excitation endoscopy through a multimode optical fiber

机译:通过多模光纤的双光子激发内窥镜

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The vast number of propagating solutions to the wave equation in multimode optical fibers represents a larger information capacity than provided by fiber bundles of the same diameter. Therefore, in the field of imaging, multimode fibers potentially allow the transmission of images with higher resolution. However, image transmission through multimode fibers is not direct as in the fiber bundle case, in which each of the fiber cores can relay a portion of the distal image. In multimode fiber transmission, a distribution of intensity is scrambled in time and space by the propagating modes, leading to a speckle-like pattern that does not resemble the initial distribution. Here, we demonstrate two-photon excitation imaging of fluorescent beads through a multimode optical fiber. We show that our method maintains the advantages of two-photon excitation microscopy compared to single-photon excitation such as reduced photo-bleaching, deeper penetration depth and sectioning capability. Our method is based on time-gated digital phase conjugation, which allows the generation of focused pulses on the other side of a multimode fiber. To acquire an image, the focused femtosecond pulse is scanned in a three-dimensional mesh, producing two-photon excitation on each spatial location of the sample. By collecting the fluorescence through the fiber, a 3D two-photon image is reconstructed.
机译:与相同直径的光纤束相比,多模光纤中波动方程的大量传播解表示更大的信息容量。因此,在成像领域,多模光纤潜在地允许以更高的分辨率传输图像。然而,通过多模光纤的图像传输并不像在光纤束情况下那样直接,在光纤束情况下,每个光纤芯都可以中继一部分远端图像。在多模光纤传输中,传播模式会在时间和空间上扰乱强度分布,从而导致出现类似于初始分布的散斑状图案。在这里,我们演示了通过多模光纤的荧光珠的双光子激发成像。我们表明,与单光子激发相比,我们的方法保持了双光子激发显微镜的优势,例如减少了光漂白,更深的穿透深度和切片能力。我们的方法基于时间门控数字相位共轭,它允许在多模光纤的另一侧生成聚焦脉冲。为了获取图像,在三维网格中扫描聚焦的飞秒脉冲,在样本的每个空间位置上产生双光子激发。通过收集通过纤维的荧光,可以重建3D两光子图像。

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