Divergent excitation two photon microscopy for 3D random access mesoscale imaging at single cell resolution

In neuroscience, diffraction limited two-photon (2P) microscopy is a cornerstone technique that permits minimally invasive optical monitoring of neuronal activity. However, most conventional 2P microscopes impose significant constraints on the size of the imaging field-of-view and the specific shape...

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Bibliographic Details
Published inbioRxiv
Main Authors Janiak, Filip K, Bartel, Philipp, Bale, Michael, Yoshimatsu, T, Komulainen, Emilia H, Zhou, Mingyi, Staras, Kevin, Prieto-Godino, Lucia L, Euler, Thomas, Maravall, Miguel, Baden, Tom
Format Paper
LanguageEnglish
Published Cold Spring Harbor Cold Spring Harbor Laboratory Press 29.10.2019
Subjects
Microscopes
Microscopy
Nervous system
Optics
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Summary:In neuroscience, diffraction limited two-photon (2P) microscopy is a cornerstone technique that permits minimally invasive optical monitoring of neuronal activity. However, most conventional 2P microscopes impose significant constraints on the size of the imaging field-of-view and the specific shape of the effective excitation volume, thus limiting the scope of biological questions that can be addressed and the information obtainable. Here, employing 'divergent beam optics' (DBO), we present an ultra-low-cost, easily implemented and flexible solution to address these limitations, offering a several-fold expanded three-dimensional field of view that also maintains single-cell resolution. We show that this implementation increases both the space-bandwidth product and effective excitation power, and allows for straight-forward tailoring of the point-spread-function. Moreover, rapid laser-focus control via an electrically tunable lens now allows near-simultaneous imaging of remote regions separated in three dimensions and permits the bending of imaging planes to follow natural curvatures in biological structures. Crucially, our core design is readily implemented (and reversed) within a matter of hours, and fully compatible with a wide range of existing 2P customizations, making it highly suitable as a base platform for further development. We demonstrate the application of our system for imaging neuronal activity in a variety of examples in mice, zebrafish and fruit flies. Footnotes * https://github.com/BadenLab/DBOscope
DOI:10.1101/821405