High-resolution structural and functional deep brain imaging using adaptive optics three-photon microscopy

被引:0
|
作者
Lina Streich
Juan Carlos Boffi
Ling Wang
Khaleel Alhalaseh
Matteo Barbieri
Ronja Rehm
Senthilkumar Deivasigamani
Cornelius T. Gross
Amit Agarwal
Robert Prevedel
机构
[1] European Molecular Biology Laboratory (EMBL),Cell Biology and Biophysics Unit
[2] Faculty of Biosciences,Collaboration for joint PhD degree between EMBL and Heidelberg University
[3] Heidelberg University,The Chica and Heinz Schaller Research Group, Institute for Anatomy and Cell Biology
[4] Heidelberg University,Epigenetics and Neurobiology Unit
[5] European Molecular Biology Laboratory,Interdisciplinary Center for Neurosciences
[6] Heidelberg University,Developmental Biology Unit
[7] European Molecular Biology Laboratory,Molecular Medicine Partnership Unit (MMPU)
[8] European Molecular Biology Laboratory,undefined
来源
Nature Methods | 2021年 / 18卷
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摘要
Multiphoton microscopy has become a powerful tool with which to visualize the morphology and function of neural cells and circuits in the intact mammalian brain. However, tissue scattering, optical aberrations and motion artifacts degrade the imaging performance at depth. Here we describe a minimally invasive intravital imaging methodology based on three-photon excitation, indirect adaptive optics (AO) and active electrocardiogram gating to advance deep-tissue imaging. Our modal-based, sensorless AO approach is robust to low signal-to-noise ratios as commonly encountered in deep scattering tissues such as the mouse brain, and permits AO correction over large axial fields of view. We demonstrate near-diffraction-limited imaging of deep cortical spines and (sub)cortical dendrites up to a depth of 1.4 mm (the edge of the mouse CA1 hippocampus). In addition, we show applications to deep-layer calcium imaging of astrocytes, including fibrous astrocytes that reside in the highly scattering corpus callosum.
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页码:1253 / 1258
页数:5
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