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Integrated one- and two-photon scanned oblique plane illumination (SOPi) microscopy for rapid volumetric imaging

机译:集成的一光子和二光子扫描斜面照明(SOPi)显微镜用于快速体积成像

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摘要

Versatile, sterically accessible imaging systems capable of in vivo rapid volumetric functional and structural imaging deep in the brain continue to be a limiting factor in neuroscience research. Towards overcoming this obstacle, we present integrated one- and two-photon scanned oblique plane illumination (SOPi, /sōpī/) microscopy which uses a single front-facing microscope objective to provide light-sheet scanning based rapid volumetric imaging capability at subcellular resolution. Our planar scan-mirror based optimized light-sheet architecture allows for non-distorted scanning of volume samples, simplifying accurate reconstruction of the imaged volume. Integration of both one-photon (1P) and two-photon (2P) light-sheet microscopy in the same system allows for easy selection between rapid volumetric imaging and higher resolution imaging in scattering media. Using SOPi, we demonstrate deep, large volume imaging capability inside scattering mouse brain sections and rapid imaging speeds up to 10 volumes per second in zebrafish larvae expressing genetically encoded fluorescent proteins GFP or GCaMP6s. SOPi’s flexibility and steric access makes it adaptable for numerous imaging applications and broadly compatible with orthogonal techniques for actuating or interrogating neuronal structure and activity.
机译:能够在大脑深处进行体内快速体积功能和结构成像的多功能,空间可访问的成像系统继续成为神经科学研究的限制因素。为了克服这一障碍,我们提出了集成的单光子和双光子扫描斜面照明(SOPi,/sōpī/)显微镜,该显微镜使用单个正面显微镜物镜在亚细胞分辨率下提供基于光片扫描的快速体积成像功能。我们基于平面扫描镜的优化光片架构允许对体积样本进行不失真的扫描,从而简化了成像体积的精确重建。在同一系统中将单光子(1P)和双光子(2P)光学片显微镜集成在一起,可以轻松地在散射介质中的快速体积成像和高分辨率成像之间进行选择。使用SOPi,我们证明了在散布的小鼠脑部区域内的深层大体积成像能力以及在表达遗传编码的荧光蛋白GFP或GCaMP6s的斑马鱼幼虫中的快速成像速度高达每秒10卷。 SOPi的灵活性和空间访问能力使其适用于多种成像应用,并与用于驱动或询问神经元结构和活动的正交技术广泛兼容。

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