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Rapid volumetric imaging with Bessel-Beam three-photon microscopy

机译:贝塞尔光束三光子显微镜快速体积成像

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摘要

Owing to its tissue-penetration ability, multi-photon fluorescence microscopy allows for the high-resolution, non-invasive imaging of deep tissue in vivo; the recently developed three-photon microscopy (3PM) has extended the depth of high-resolution, non-invasive functional imaging of mouse brains to beyond 1.0 mm. However, the low repetition rate of femtosecond lasers that are normally used in 3PM limits the temporal resolution of point-scanning three-photon microscopy. To increase the volumetric imaging speed of 3PM, we propose a combination of an axially elongated needle-like Bessel-beam with three-photon excitation (3PE) to image biological samples with an extended depth of focus. We demonstrate the higher signal-to-background ratio (SBR) of the Bessel-beam 3PM compared to the two-photon version both theoretically and experimentally. Finally, we perform simultaneous calcium imaging of brain regions at different axial locations in live fruit flies and rapid volumetric imaging of neuronal structures in live mouse brains. These results highlight the unique advantage of conducting rapid volumetric imaging with a high SBR in the deep brain in vivo using scanning Bessel-3PM.
机译:由于具有组织穿透能力,因此多光子荧光显微镜可以对体内深层组织进行高分辨率,无创成像。最近开发的三光子显微镜(3PM)将鼠标脑的高分辨率,非侵入性功能成像的深度扩展到1.0毫米以上。但是,通常在3PM中使用的飞秒激光器的低重复率限制了点扫描三光子显微镜的时间分辨率。为了提高3PM的体积成像速度,我们建议将轴向细长的针状贝塞尔光束与三光子激发(3PE)结合使用,以对具有扩展焦点深度的生物样品进行成像。我们在理论上和实验上都证明了与双光子版本相比,贝塞尔光束3PM具有更高的信噪比(SBR)。最后,我们对活果蝇在不同轴向位置的大脑区域进行同步钙成像,并在活老鼠大脑中对神经元结构进行快速体积成像。这些结果凸显了使用Bessel-3PM扫描在体内深脑中以高SBR进行快速体积成像的独特优势。

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