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Deletion of EphA4 enhances deafferentation-induced ipsilateral sprouting in auditory brainstem projections

✍ Scribed by Candace Y. Hsieh; Cindy T. Hong; Karina S. Cramer


Publisher
John Wiley and Sons
Year
2007
Tongue
English
Weight
905 KB
Volume
504
Category
Article
ISSN
0021-9967

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✦ Synopsis


Abstract

Axonal selection of ipsilateral and/or contralateral targets is essential for integrating bilateral sensory information and for coordinated movement. The molecular processes that determine ipsilateral and contralateral target choice are not fully understood. We examined this target selection in the developing auditory brainstem. Ventral cochlear nucleus (VCN) axons normally project to the medial nucleus of the trapezoid body (MNTB) only on the contralateral side. However, after unilateral removal of cochlear input in neonates, we found that axons from the unoperated VCN sprout and project to MNTB bilaterally. We found that EphA4 is expressed in the mouse auditory brainstem during development and during a sensitive period for ipsilateral sprouting, so we hypothesized that deletion of the Eph receptor EphA4 would impair target selection in these auditory pathways. Lipophilic dyes were used to evaluate quantitatively the brainstem projections in wild‐type and EphA4‐null mice. VCN‐MNTB projections in EphA4‐null mice were strictly contralateral, as in wild‐type mice. However, after deafferentation, EphA4‐null mice had a significant, threefold increase in the proportion of axons from the intact VCN that sprouted into ipsilateral MNTB compared with wild‐type mice. Heterozygous mice had a twofold increase in these projections. These results demonstrate that EphA4 influences auditory brainstem circuitry selectively in response to deafferentation. Although this axon guidance molecule is not by itself necessary for appropriate target choice during normal development, it is a strong determinant of ipsilateral vs. contralateral target choice during deafferentation‐induced plasticity. J. Comp. Neurol. 504:508–518, 2007. © 2007 Wiley‐Liss, Inc.