Neural Regeneration Research ›› 2013, Vol. 8 ›› Issue (17): 1541-1550.doi: 10.3969/j.issn.1673-5374.2013.17.001

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Neurotrophins differentially stimulate the growth of cochlear neurites on collagen surfaces and in gels

Joanna Xie1, Kwang Pak1, Amaretta Evans1, Andy Kamgar-Parsi1, Stephen Fausti2, Lina Mullen1, Allen Frederic Ryan1, 3   

  1. 1 Department of Surgery/Otolaryngology, School of Medicine and Veterans Administration Medical Center, University of California, San Diego, CA 92093-0666, USA
    2 National Center for Research on Auditory Rehabilitation, Portland VA Medical Center, Portland, OR, USA
    3 Department of Neurosciences, School of Medicine and Veterans Administration Medical Center, University of California, San Diego, CA 92093-0666, USA
  • Received:2012-12-21 Revised:2013-02-07 Online:2013-06-15 Published:2013-06-15
  • Contact: Allen Frederic Ryan, Ph.D., Professor, Division of Otolaryngology, School of Medicine, 0666 University of California, San Diego, 9500 Gilman Drive, La Jolla, CA 92093-0666, USA, afryan@ucsd.edu.
  • About author:Joanna Xie☆, Studying for doctorate.

Abstract:

The electrodes of a cochlear implant are located far from the surviving neurons of the spiral ganglion, which results in decreased precision of neural activation compared to the normal ear. If the neurons could be induced to extend neurites toward the implant, it might be possible to stimulate more discrete subpopulations of neurons, and to increase the resolution of the device. However, a major barrier to neurite growth toward a cochlear implant is the fluid filling the scala tympani, which separates the neurons from the electrodes. The goal of this study was to evaluate the growth of cochlear neurites in three-dimensional extracellular matrix molecule gels, and to increase biocompatibility by using fibroblasts stably transfected to produce neurotrophin-3 and brain-derived neurotrophic factor. Spiral ganglion explants from neonatal rats were evaluated in cultures. They were exposed to soluble neurotrophins, cells transfected to secrete neurotrophins, and/or collagen gels. We found that cochlear neurites grew readily on collagen surfaces and in three-dimensional collagen gels. Co-culture with cells producing neurotrophin-3 resulted in increased numbers of neurites, and neurites that were longer than when explants were cultured with control fibroblasts stably transfected with green fluorescent protein. Brain-derived neurotrophic factor-producing cells resulted in a more dramatic increase in the number of neurites, but there was no significant effect on neurite length. It is suggested that extracellular matrix molecule gels and cells transfected to produce neurotrophins offer an opportunity to attract spiral ganglion neurites toward a cochlear implant.

Key words: neural regeneration, peripheral nerve injury, cochlear implant, inner ear, neuron, neurite guidance, neurotrophin, extracellular matrix, collagen gel, grants-supported paper, neuroregeneration