4.6 Article

Fast volume-scanning light sheet microscopy reveals transient neuronal events

Journal

BIOMEDICAL OPTICS EXPRESS
Volume 9, Issue 5, Pages 2154-2167

Publisher

OPTICAL SOC AMER
DOI: 10.1364/BOE.9.002154

Keywords

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Funding

  1. UK Engineering and Physical Sciences Research Council (EPSRC) [EP/P030017/1]
  2. Biotechnology and Biological Sciences Research Council (BBSRC)
  3. Wellcome Trust
  4. BBSRC [BB/J018724/1] Funding Source: UKRI
  5. EPSRC [EP/P030017/1] Funding Source: UKRI

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Light sheet fluorescence microscopy offers considerable potential to the cellular neuroscience community as it makes it possible to image extensive areas of neuronal structures, such as axons or dendrites, with a low light budget, thereby minimizing phototoxicity. However, the shallow depth of a light sheet, which is critical for achieving high contrast, well resolved images, adds a significant challenge if fast functional imaging is also required, as multiple images need to be collected across several image planes. Consequently, fast functional imaging of neurons is typically restricted to a small tissue volume where part of the neuronal structure lies within the plane of a single image. Here we describe a method by which fast functional imaging can be achieved across a much larger tissue volume; a custom-built light sheet microscope is presented that includes a synchronized galvo mirror and electrically tunable lens, enabling high speed acquisition of images across a configurable depth. We assess the utility of this technique by acquiring fast functional Ca2+ imaging data across a neuron's dendritic arbour in mammalian brain tissue. Published by The Optical Society under the terms of the Creative Commons Attribution 4.0 License.

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