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The Journal of Neurophysiology Vol. 86 No. 2 August 2001, pp. 1037-1042
Copyright ©2001 by the American Physiological Society
California Institute of Technology, Pasadena, California 91125
D'Apuzzo, Massimo,
Georgia Mandolesi,
Gerald Reis, and
Erin M. Schuman.
Abundant GFP Expression and LTP in Hippocampal Acute Slices by In
Vivo Injection of Sindbis Virus. J. Neurophysiol. 86: 1037-1042, 2001. Virus-mediated gene transfer into
neurons is a powerful tool for the analysis of neuronal structure and
function. Recombinant sindbis virus has been previously used to study
protein function in hippocampal neuron cultures as well as in
hippocampal organotypic slice cultures. Nevertheless, some concern
still exists about the physiological relevance of these cultured
preparations. Acute hippocampal slices are a widely used preparation
for the study of synaptic transmission, but currently recombinant gene
delivery is usually achieved only through time-consuming transgenic
techniques. In this study, we show that a subregion of the CA1 area in
acute hippocampal slices can be specifically altered to express a gene of interest. A sindbis virus vector carrying an enhanced green fluorescent protein (EGFP) reporter was injected in vivo into the
hippocampus of adult rats. After 18 h, rats were killed, and acute
hippocampal slices, infected in the CA1 field, were analyzed morphologically and electrophysiologically. Infected slices showed healthy and stable electrophysiological responses as well as long-term potentiation. In addition, infected pyramidal cells were readily recognized in living slices by two-photon imaging. Specifically, the
introduction of an EGFP-Actin fusion protein greatly enhanced the
detection of fine processes and dendritic spines. We propose this
technique as an efficient tool for studying gene function in adult
hippocampal neurons.
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