MiR-210 promotes sensory hair cell formation in the organ of corti.

Sabrina Riccardi,Juliet Leighton-Davies,Frederic Sigoillot,Bernd Kinzel,Guglielmo Roma,Martin Beibel,Christian N Parker,Sebastian Bergling,Judith Knehr,Tewis Bouwmeester,Annick Werner

doi:10.1186/s12864-016-2620-7

Sabrina Riccardi, Juliet Leighton-Davies + Show 9 more

Open Access

https://doi.org/10.1186/s12864-016-2620-7

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Abstract

BackgroundHearing loss is the most common sensory defect afflicting several hundred million people worldwide. In most cases, regardless of the original cause, hearing loss is related to the degeneration and death of hair cells and their associated spiral ganglion neurons. Despite this knowledge, relatively few studies have reported regeneration of the auditory system. Significant gaps remain in our understanding of the molecular mechanisms underpinning auditory function, including the factors required for sensory cell regeneration. Recently, the identification of transcriptional activators and repressors of hair cell fate has been augmented by the discovery of microRNAs (miRNAs) associated with hearing loss. As miRNAs are central players of differentiation and cell fate, identification of miRNAs and their gene targets may reveal new pathways for hair cell regeneration, thereby providing new avenues for the treatment of hearing loss.ResultsIn order to identify new genetic elements enabling regeneration of inner ear sensory hair cells, next-generation miRNA sequencing (miRSeq) was used to identify the most prominent miRNAs expressed in the mouse embryonic inner ear cell line UB/OC-1 during differentiation towards a hair cell like phenotype. Based on these miRSeq results eight most differentially expressed miRNAs were selected for further characterization. In UB/OC-1, miR-210 silencing in vitro resulted in hair cell marker expression, whereas ectopic expression of miR-210 resulted in new hair cell formation in cochlear explants. Using a lineage tracing mouse model, transdifferentiation of supporting epithelial cells was identified as the likely mechanism for this new hair cell formation. Potential miR-210 targets were predicted in silico and validated experimentally using a miR-trap approach.ConclusionMiRSeq followed by ex vivo validation revealed miR-210 as a novel factor driving transdifferentiation of supporting epithelial cells to sensory hair cells suggesting that miR-210 might be a potential new factor for hearing loss therapy. In addition, identification of inner ear pathways regulated by miR-210 identified potential new drug targets for the treatment of hearing loss.Electronic supplementary materialThe online version of this article (doi:10.1186/s12864-016-2620-7) contains supplementary material, which is available to authorized users.

Highlights

Hearing loss is the most common sensory defect afflicting several hundred million people worldwide
Ninety-nine miRNAs are differentially expressed during UB/OC-1 differentiation To investigate the potential role of microRNAs in sensory hair cell formation, we performed generation small RNA sequencing of UB/OC-1 cells, comparing the non-sensory epithelial precursor cell stage with cells at an early stage of differentiation towards a sensory haircell-like phenotype
For miRNA sequencing (miRSeq) we collected five samples of UB/OC-1 cells at precursor stage grown at 33 °C and three samples of differentiating UB/OC-1 cells collected 1 day after temperature shift to 39 °C (Additional file 1)

Summary

Introduction

Hearing loss is the most common sensory defect afflicting several hundred million people worldwide. Regardless of the original cause, hearing loss is related to the degeneration and death of hair cells and their associated spiral ganglion neurons Despite this knowledge, relatively few studies have reported regeneration of the auditory system. Significant gaps remain in our understanding of the molecular mechanisms underpinning auditory function, including the factors required for sensory cell regeneration. In mammals, supporting cells can be forced to transdifferentiate into new auditory hair cells given the right stimulus, namely over-expression of Atoh, which is normally only expressed during fetal development [7] This suggests that the molecular systems required for inducing inner ear hair cell fate are still present and functional in adult mammalian supporting cells, and their fate may be altered if the cells receive the appropriate signals [8, 9]

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