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利用光学不变量分析设计大视场双光子显微镜。

Designing a large field-of-view two-photon microscope using optical invariant analysis.

作者信息

Bumstead Jonathan R, Park Jasmine J, Rosen Isaac A, Kraft Andrew W, Wright Patrick W, Reisman Matthew D, Côté Daniel C, Culver Joseph P

机构信息

Washington University in Saint Louis, Department of Biomedical Engineering, St. Louis, Missouri, United States.

Washington University School of Medicine, Department of Radiology, St. Louis, Missouri, United States.

出版信息

Neurophotonics. 2018 Apr;5(2):025001. doi: 10.1117/1.NPh.5.2.025001. Epub 2018 Feb 19.

DOI:10.1117/1.NPh.5.2.025001
PMID:29487876
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5818100/
Abstract

Conventional two-photon microscopy (TPM) is capable of imaging neural dynamics with subcellular resolution, but it is limited to a field-of-view (FOV) diameter [Formula: see text]. Although there has been recent progress in extending the FOV in TPM, a principled design approach for developing large FOV TPM (LF-TPM) with off-the-shelf components has yet to be established. Therefore, we present a design strategy that depends on analyzing the optical invariant of commercially available objectives, relay lenses, mirror scanners, and emission collection systems in isolation. Components are then selected to maximize the space-bandwidth product of the integrated microscope. In comparison with other LF-TPM systems, our strategy simplifies the sequence of design decisions and is applicable to extending the FOV in any microscope with an optical relay. The microscope we constructed with this design approach can image [Formula: see text] lateral and [Formula: see text] axial resolution over a 7-mm diameter FOV, which is a 100-fold increase in FOV compared with conventional TPM. As a demonstration of the potential that LF-TPM has on understanding the microarchitecture of the mouse brain across interhemispheric regions, we performed imaging of both the cerebral vasculature and microglia cell bodies over the mouse cortex.

摘要

传统的双光子显微镜(TPM)能够以亚细胞分辨率对神经动力学进行成像,但它的视野(FOV)直径有限[公式:见原文]。尽管最近在扩展TPM的视野方面取得了进展,但尚未建立一种使用现成组件开发大视野TPM(LF-TPM)的原则性设计方法。因此,我们提出了一种设计策略,该策略依赖于单独分析市售物镜、中继透镜、镜扫描器和发射收集系统的光学不变量。然后选择组件以最大化集成显微镜的空间带宽积。与其他LF-TPM系统相比,我们的策略简化了设计决策的顺序,并且适用于扩展任何具有光学中继的显微镜的视野。我们用这种设计方法构建的显微镜可以在直径7毫米的视野上以[公式:见原文]横向和[公式:见原文]轴向分辨率进行成像,与传统TPM相比,视野增加了100倍。作为LF-TPM在理解跨半球区域小鼠脑微结构方面潜力的一个例证,我们对小鼠皮质的脑血管和小胶质细胞体进行了成像。

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