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急性心肌切片中的多点多光子Ca²⁺成像

Multispot multiphoton Ca²⁺ imaging in acute myocardial slices.

作者信息

Borile Giulia, de Mauro Claudio, Urbani Andrea, Alfieri Domenico, Pavone Francesco S, Mongillo Marco

机构信息

University of Padova, Department of Biomedical Science, Viale Colombo 3, Padova 35129, ItalybVenetian Institute of Molecular Medicine, Via Orus 2, Padova 35129, Italy.

Light4Tech Firenze s.r.l., Via Pisana 316, Scandicci 50018, Italy.

出版信息

J Biomed Opt. 2015 May;20(5):51016. doi: 10.1117/1.JBO.20.5.051016.

Abstract

Multiphoton microscopy has become essential for dynamic imaging in thick living tissues. High-rate, full-field image acquisition in multiphoton microscopy is achievable by parallelization of the excitation and detection pathways. We developed our approach via a diffractive optical element which splits a pulsed laser into 16 beamlets and exploits a descanned detection system consisting of an array of beamlet-associated photomultiplier tubes. The optical performance of the multiphoton multispot system (MCube) has been characterized in cardiac tissue sections and subsequently used for the first time for fluorescence imaging of cardiomyocyte Ca²⁺ dynamics in viable acute cardiac slices. Multispot multiphoton microscopy (MMM) has never been used before to monitor Ca²⁺ dynamics in thick, viable tissue samples. Acute heart slices are a powerful close-to-in vivo model of Ca²⁺ imaging allowing the simultaneous observation of several cells in their own tissue environment, exploiting the multiphoton excitation ability to penetrate scattering tissues. Moreover, we show that the concurrent high spatial and temporal resolutions afforded by the parallel scanning in MMM can be exploited to simultaneously assess subcellular Ca²⁺ dynamics in different cells in the tissue. We recorded local Ca²⁺ release events including macrosparks, travelling waves, and rotors.

摘要

多光子显微镜已成为厚层活组织动态成像的关键技术。通过激发和检测路径的并行化,多光子显微镜可实现高速、全场图像采集。我们通过一种衍射光学元件开发了我们的方法,该元件将脉冲激光分成16个小光束,并采用了一种由与小光束相关的光电倍增管阵列组成的去扫描检测系统。多光子多点系统(MCube)的光学性能已在心脏组织切片中得到表征,并随后首次用于在存活的急性心脏切片中对心肌细胞Ca²⁺动力学进行荧光成像。多点多光子显微镜(MMM)以前从未用于监测厚层、存活组织样本中的Ca²⁺动力学。急性心脏切片是一种强大的近乎体内的Ca²⁺成像模型,利用多光子激发穿透散射组织的能力,可在其自身组织环境中同时观察多个细胞。此外,我们表明,MMM中的并行扫描所提供的同时高空间和时间分辨率可用于同时评估组织中不同细胞的亚细胞Ca²⁺动力学。我们记录了局部Ca²⁺释放事件,包括大钙火花、行波和转子。

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