Imaging Large-Scale Neural Activity with Cellular Resolution in Awake, Mobile Mice

We report a technique for two-photon fluorescence imaging with cellular resolution in awake, behaving mice with minimal motion artifact. The apparatus combines an upright, table-mounted two-photon microscope with a spherical treadmill consisting of a large, air-supported Styrofoam ball. Mice, with i...

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Published inNeuron (Cambridge, Mass.) Vol. 56; no. 1; pp. 43 - 57
Main Authors Dombeck, Daniel A., Khabbaz, Anton N., Collman, Forrest, Adelman, Thomas L., Tank, David W.
Format Journal Article
LanguageEnglish
Published United States Elsevier Inc 04.10.2007
Elsevier Limited
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ISSN0896-6273
1097-4199
1097-4199
DOI10.1016/j.neuron.2007.08.003

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Summary:We report a technique for two-photon fluorescence imaging with cellular resolution in awake, behaving mice with minimal motion artifact. The apparatus combines an upright, table-mounted two-photon microscope with a spherical treadmill consisting of a large, air-supported Styrofoam ball. Mice, with implanted cranial windows, are head restrained under the objective while their limbs rest on the ball's upper surface. Following adaptation to head restraint, mice maneuver on the spherical treadmill as their heads remain motionless. Image sequences demonstrate that running-associated brain motion is limited to ∼2-5 μm. In addition, motion is predominantly in the focal plane, with little out-of-plane motion, making the application of a custom-designed Hidden-Markov-Model-based motion correction algorithm useful for postprocessing. Behaviorally correlated calcium transients from large neuronal and astrocytic populations were routinely measured, with an estimated motion-induced false positive error rate of <5%.
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Authors contributed equally to this work.
ISSN:0896-6273
1097-4199
1097-4199
DOI:10.1016/j.neuron.2007.08.003