Maturation of Ribbon Synapses in Hair Cells Is Driven by Thyroid Hormone

doi:10.1523/JNEUROSCI.3974-06.2007

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The Journal of Neuroscience, March 21, 2007, 27(12):3163-3173; doi:10.1523/JNEUROSCI.3974-06.2007

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Cellular/Molecular
Maturation of Ribbon Synapses in Hair Cells Is Driven by Thyroid Hormone
Gaston Sendin,¹ Anna V. Bulankina,¹ Dietmar Riedel,² and Tobias Moser¹
¹InnerEarLab, Department of Otolaryngology and Center for Molecular Physiology of the Brain, Göttingen University Medical School, 37075 Göttingen, Germany, and ²Electron Microscopy Group, Department of Neurobiology, Max Planck Institute for Biophysical Chemistry, 37077 Göttingen, Germany
Correspondence should be addressed to Tobias Moser, InnerEarLab, Department of Otolaryngology, University of Göttingen, Center for Molecular Physiology of the Brain, Bernstein Center for Computational Neuroscience, 37099 Göttingen, Germany. Email: tmoser{at}gwdg.de
Ribbon synapses of inner hair cells (IHCs) undergo developmentalmaturation until after the onset of hearing. Here, we studiedwhether IHC synaptogenesis is regulated by thyroid hormone (TH).We performed perforated patch-clamp recordings of Ca²⁺ currentsand exocytic membrane capacitance changes in IHCs of athyroidand TH-substituted Pax8^–/– mice during postnataldevelopment. Ca²⁺ currents remained elevated in athyroid IHCsat the end of the second postnatal week, when it had developmentallydeclined in wild-type and TH-rescued mutant IHCs. The efficiencyof Ca²⁺ influx in triggering exocytosis of the readily releasablevesicle pool was reduced in athyroid IHCs. Ribbon synapses wereformed despite the TH deficiency. However, different from wildtype, in which synapse elimination takes place at approximatelythe onset of hearing, the number of ribbon synapses remainedelevated in 2-week-old athyroid IHCs. Moreover, the ultrastructureof these synapses appeared immature. Using quantitative reversetranscription-PCR, we found a TH-dependent developmental upregulationof the mRNAs for the neuronal SNARE (soluble N-ethylmaleimide-sensitivefactor attachment protein receptor) proteins, SNAP25 (synaptosomal-associatedprotein of 25 kDa) and synaptobrevin 1, in the organ of Corti.These molecular changes probably contribute to the improvementof exocytosis efficiency in mature IHCs. IHCs of 2-week-oldathyroid Pax8^–/– mice maintained the normally temporaryefferent innervation. Moreover, they lacked large-conductanceCa²⁺-activated K⁺ channels and KCNQ4 channels. This togetherwith the persistently increased Ca²⁺ influx permitted continuedaction potential generation. We conclude that TH regulates IHCdifferentiation and is essential for morphological and functionalmaturation of their ribbon synapses. We suggest that presynapticdysfunction of IHCs is a mechanism in congenital hypothyroiddeafness.

Key words: thyroid hormone; ion channel; ribbon synapse; exocytosis; hair cell; capacitance; Pax8

Received Sept. 12, 2006; revised Jan. 19, 2007; accepted Jan. 19, 2007.

Correspondence should be addressed to Tobias Moser, InnerEarLab, Department of Otolaryngology, University of Göttingen, Center for Molecular Physiology of the Brain, Bernstein Center for Computational Neuroscience, 37099 Göttingen, Germany. Email: tmoser{at}gwdg.de

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