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J Neurophysiol 94: 1636-1644, 2005. First published April 20, 2005; doi:10.1152/jn.01013.2004
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INNOVATIVE METHODOLOGY

In Vivo Calcium Imaging of Circuit Activity in Cerebellar Cortex

Megan R. Sullivan1,3, Axel Nimmerjahn4, Dmitry V. Sarkisov2,3, Fritjof Helmchen4 and Samuel S.-H. Wang1,3

1Departments of Molecular Biology and 2Physics and 3Program in Neuroscience, Princeton University, Princeton, New Jersey; and 4Abteilung Zellphysiologie, Max-Planck-Institut für Medizinische Forschung, Heidelberg, Germany

Submitted 27 September 2004; accepted in final form 9 April 2005

In vivo two-photon calcium imaging provides the opportunity to monitor activity in multiple components of neural circuitry at once. Here we report the use of bulk-loading of fluorescent calcium indicators to record from axons, dendrites, and neuronal cell bodies in cerebellar cortex in vivo. In cerebellar folium crus IIa of anesthetized rats, we imaged the labeled molecular layer and identified all major cellular structures: Purkinje cells, interneurons, parallel fibers, and Bergmann glia. Using extracellular stimuli we evoked calcium transients corresponding to parallel fiber beam activity. This beam activity triggered prolonged calcium transients in interneurons, consistent with in vitro evidence for synaptic activation of N-methyl-D-aspartate receptors via glutamate spillover. We also observed spontaneous calcium transients in Purkinje cell dendrites that were identified as climbing-fiber-evoked calcium spikes by their size, time course, and sensitivity to AMPA receptor antagonist. Two-photon calcium imaging of bulk-loaded cerebellar cortex is thus well suited to optically monitor synaptic processing in the intact cerebellum.


Address for reprint requests and other correspondence: S. Wang, Dept. of Molecular Biology, Lewis Thomas Lab., Princeton University, Washington Road, Princeton, NJ 08544 (E-mail: sswang{at}princeton.edu)




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