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在体内通过光学切片对神经元结构和功能进行快速宽视场成像。

Fast widefield imaging of neuronal structure and function with optical sectioning in vivo.

作者信息

Li Ziwei, Zhang Qinrong, Chou Shih-Wei, Newman Zachary, Turcotte Raphaël, Natan Ryan, Dai Qionghai, Isacoff Ehud Y, Ji Na

机构信息

Department of Physics, University of California, Berkeley, Berkeley, CA 94720, USA.

Department of Automation, Tsinghua University, Beijing 100084, China.

出版信息

Sci Adv. 2020 May 8;6(19):eaaz3870. doi: 10.1126/sciadv.aaz3870. eCollection 2020 May.

Abstract

Optical microscopy, owing to its noninvasiveness and subcellular resolution, enables in vivo visualization of neuronal structure and function in the physiological context. Optical-sectioning structured illumination microscopy (OS-SIM) is a widefield fluorescence imaging technique that uses structured illumination patterns to encode in-focus structures and optically sections 3D samples. However, its application to in vivo imaging has been limited. In this study, we optimized OS-SIM for in vivo neural imaging. We modified OS-SIM reconstruction algorithms to improve signal-to-noise ratio and correct motion-induced artifacts in live samples. Incorporating an adaptive optics (AO) module to OS-SIM, we found that correcting sample-induced optical aberrations was essential for achieving accurate structural and functional characterizations in vivo. With AO OS-SIM, we demonstrated fast, high-resolution in vivo imaging with optical sectioning for structural imaging of mouse cortical neurons and zebrafish larval motor neurons, and functional imaging of quantal synaptic transmission at larval neuromuscular junctions.

摘要

光学显微镜因其非侵入性和亚细胞分辨率,能够在生理环境中对神经元结构和功能进行体内可视化。光学切片结构照明显微镜(OS-SIM)是一种宽场荧光成像技术,它使用结构化照明图案对焦内结构进行编码,并对三维样本进行光学切片。然而,其在体内成像中的应用一直受到限制。在本研究中,我们对OS-SIM进行了优化以用于体内神经成像。我们修改了OS-SIM重建算法,以提高信噪比并校正活样本中由运动引起的伪影。将自适应光学(AO)模块集成到OS-SIM中,我们发现校正样本引起的光学像差对于在体内实现准确的结构和功能表征至关重要。通过AO OS-SIM,我们展示了用于小鼠皮层神经元和斑马鱼幼虫运动神经元结构成像的快速、高分辨率体内光学切片成像,以及幼虫神经肌肉接头处量子突触传递的功能成像。

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