Hair Cell Maturation is Differentially Regulated Along the Tonotopic Axis of the Mammalian Cochlea

Overview

Journal J Physiol

Specialty Physiology

Date 2019 Oct 30

PMID 31661723

Citations 25

Authors

Jing-Yi Jeng

Federico Ceriani

Aenea Hendry

Stuart L Johnson

Piece Yen

Dwayne D Simmons

Corne J Kros

Walter Marcotti

Affiliations

Soon will be listed here.

Abstract

Key Points: Outer hair cells (OHCs) enhance the sensitivity and the frequency tuning of the mammalian cochlea. Similar to the primary sensory receptor, the inner hair cells (IHCs), the mature functional characteristics of OHCs are acquired before hearing onset. We found that OHCs, like IHCs, fire spontaneous Ca -induced action potentials (APs) during immature stages of development, which are driven by Ca 1.3 Ca channels. We also showed that the development of low- and high-frequency hair cells is differentially regulated during pre-hearing stages, with the former cells being more strongly dependent on experience-independent Ca action potential activity.

Abstract: Sound amplification within the mammalian cochlea depends upon specialized hair cells, the outer hair cells (OHCs), which possess both sensory and motile capabilities. In various altricial rodents, OHCs become functionally competent from around postnatal day 7 (P7), before the primary sensory inner hair cells (IHCs), which become competent at about the onset of hearing (P12). The mechanisms responsible for the maturation of OHCs and their synaptic specialization remain poorly understood. We report that spontaneous Ca activity in the immature cochlea, which is generated by Ca 1.3 Ca channels, differentially regulates the maturation of hair cells along the cochlea. Under near-physiological recording conditions we found that, similar to IHCs, immature OHCs elicited spontaneous Ca action potentials (APs), but only during the first few postnatal days. Genetic ablation of these APs in vivo, using Ca 1.3 mice, prevented the normal developmental acquisition of mature-like basolateral membrane currents in low-frequency (apical) hair cells, such as I (carried by KCNQ4 channels), I and I (α9α10nAChRs) in OHCs and I and I (BK channels) in IHCs. Electromotility and prestin expression in OHCs were normal in Ca 1.3 mice. The maturation of high-frequency (basal) hair cells was also affected in Ca 1.3 mice, but to a much lesser extent than apical cells. However, a characteristic feature in Ca 1.3 mice was the reduced hair cell size irrespective of their cochlear location. We conclude that the development of low- and high-frequency hair cells is differentially regulated during development, with apical cells being more strongly dependent on experience-independent Ca APs.

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