WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro

Hearing loss affects over 460 million people worldwide and is a major socioeconomic burden. Both genetic and environmental factors (i.e., noise overexposure, ototoxic drug treatment and ageing), promote the irreversible degeneration of cochlear hair cells and associated auditory neurons, leading to...

Descripción completa

Detalles Bibliográficos
Autores principales: Rousset, Francis, Schilardi, Giulia, Sgroi, Stéphanie, Nacher-Soler, German, Sipione, Rebecca, Kleinlogel, Sonja, Senn, Pascal
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2022
Materias:
Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9367963/
https://www.ncbi.nlm.nih.gov/pubmed/35954276
http://dx.doi.org/10.3390/cells11152431
_version_ 1784765973263286272
author Rousset, Francis
Schilardi, Giulia
Sgroi, Stéphanie
Nacher-Soler, German
Sipione, Rebecca
Kleinlogel, Sonja
Senn, Pascal
author_facet Rousset, Francis
Schilardi, Giulia
Sgroi, Stéphanie
Nacher-Soler, German
Sipione, Rebecca
Kleinlogel, Sonja
Senn, Pascal
author_sort Rousset, Francis
collection PubMed
description Hearing loss affects over 460 million people worldwide and is a major socioeconomic burden. Both genetic and environmental factors (i.e., noise overexposure, ototoxic drug treatment and ageing), promote the irreversible degeneration of cochlear hair cells and associated auditory neurons, leading to sensorineural hearing loss. In contrast to birds, fish and amphibians, the mammalian inner ear is virtually unable to regenerate due to the limited stemness of auditory progenitors, and no causal treatment is able to prevent or reverse hearing loss. As of today, a main limitation for the development of otoprotective or otoregenerative therapies is the lack of efficient preclinical models compatible with high-throughput screening of drug candidates. Currently, the research field mainly relies on primary organotypic inner ear cultures, resulting in high variability, low throughput, high associated costs and ethical concerns. We previously identified and characterized the phoenix auditory neuroprogenitors (ANPGs) as highly proliferative progenitor cells isolated from the A/J mouse cochlea. In the present study, we aim at identifying the signaling pathways responsible for the intrinsic high stemness of phoenix ANPGs. A transcriptomic comparison of traditionally low-stemness ANPGs, isolated from C57Bl/6 and A/J mice at early passages, and high-stemness phoenix ANPGs was performed, allowing the identification of several differentially expressed pathways. Based on differentially regulated pathways, we developed a reprogramming protocol to induce high stemness in presenescent ANPGs (i.e., from C57Bl6 mouse). The pharmacological combination of the WNT agonist (CHIR99021) and TGFβ/Smad inhibitors (LDN193189 and SB431542) resulted in a dramatic increase in presenescent neurosphere growth, and the possibility to expand ANPGs is virtually limitless. As with the phoenix ANPGs, stemness-induced ANPGs could be frozen and thawed, enabling distribution to other laboratories. Importantly, even after 20 passages, stemness-induced ANPGs retained their ability to differentiate into electrophysiologically mature type I auditory neurons. Both stemness-induced and phoenix ANPGs resolve a main bottleneck in the field, allowing efficient, high-throughput, low-cost and 3R-compatible in vitro screening of otoprotective and otoregenerative drug candidates. This study may also add new perspectives to the field of inner ear regeneration.
format Online
Article
Text
id pubmed-9367963
institution National Center for Biotechnology Information
language English
publishDate 2022
publisher MDPI
record_format MEDLINE/PubMed
spelling pubmed-93679632022-08-12 WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro Rousset, Francis Schilardi, Giulia Sgroi, Stéphanie Nacher-Soler, German Sipione, Rebecca Kleinlogel, Sonja Senn, Pascal Cells Article Hearing loss affects over 460 million people worldwide and is a major socioeconomic burden. Both genetic and environmental factors (i.e., noise overexposure, ototoxic drug treatment and ageing), promote the irreversible degeneration of cochlear hair cells and associated auditory neurons, leading to sensorineural hearing loss. In contrast to birds, fish and amphibians, the mammalian inner ear is virtually unable to regenerate due to the limited stemness of auditory progenitors, and no causal treatment is able to prevent or reverse hearing loss. As of today, a main limitation for the development of otoprotective or otoregenerative therapies is the lack of efficient preclinical models compatible with high-throughput screening of drug candidates. Currently, the research field mainly relies on primary organotypic inner ear cultures, resulting in high variability, low throughput, high associated costs and ethical concerns. We previously identified and characterized the phoenix auditory neuroprogenitors (ANPGs) as highly proliferative progenitor cells isolated from the A/J mouse cochlea. In the present study, we aim at identifying the signaling pathways responsible for the intrinsic high stemness of phoenix ANPGs. A transcriptomic comparison of traditionally low-stemness ANPGs, isolated from C57Bl/6 and A/J mice at early passages, and high-stemness phoenix ANPGs was performed, allowing the identification of several differentially expressed pathways. Based on differentially regulated pathways, we developed a reprogramming protocol to induce high stemness in presenescent ANPGs (i.e., from C57Bl6 mouse). The pharmacological combination of the WNT agonist (CHIR99021) and TGFβ/Smad inhibitors (LDN193189 and SB431542) resulted in a dramatic increase in presenescent neurosphere growth, and the possibility to expand ANPGs is virtually limitless. As with the phoenix ANPGs, stemness-induced ANPGs could be frozen and thawed, enabling distribution to other laboratories. Importantly, even after 20 passages, stemness-induced ANPGs retained their ability to differentiate into electrophysiologically mature type I auditory neurons. Both stemness-induced and phoenix ANPGs resolve a main bottleneck in the field, allowing efficient, high-throughput, low-cost and 3R-compatible in vitro screening of otoprotective and otoregenerative drug candidates. This study may also add new perspectives to the field of inner ear regeneration. MDPI 2022-08-05 /pmc/articles/PMC9367963/ /pubmed/35954276 http://dx.doi.org/10.3390/cells11152431 Text en © 2022 by the authors. https://creativecommons.org/licenses/by/4.0/Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Rousset, Francis
Schilardi, Giulia
Sgroi, Stéphanie
Nacher-Soler, German
Sipione, Rebecca
Kleinlogel, Sonja
Senn, Pascal
WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro
title WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro
title_full WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro
title_fullStr WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro
title_full_unstemmed WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro
title_short WNT Activation and TGFβ-Smad Inhibition Potentiate Stemness of Mammalian Auditory Neuroprogenitors for High-Throughput Generation of Functional Auditory Neurons In Vitro
title_sort wnt activation and tgfβ-smad inhibition potentiate stemness of mammalian auditory neuroprogenitors for high-throughput generation of functional auditory neurons in vitro
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9367963/
https://www.ncbi.nlm.nih.gov/pubmed/35954276
http://dx.doi.org/10.3390/cells11152431
work_keys_str_mv AT roussetfrancis wntactivationandtgfbsmadinhibitionpotentiatestemnessofmammalianauditoryneuroprogenitorsforhighthroughputgenerationoffunctionalauditoryneuronsinvitro
AT schilardigiulia wntactivationandtgfbsmadinhibitionpotentiatestemnessofmammalianauditoryneuroprogenitorsforhighthroughputgenerationoffunctionalauditoryneuronsinvitro
AT sgroistephanie wntactivationandtgfbsmadinhibitionpotentiatestemnessofmammalianauditoryneuroprogenitorsforhighthroughputgenerationoffunctionalauditoryneuronsinvitro
AT nachersolergerman wntactivationandtgfbsmadinhibitionpotentiatestemnessofmammalianauditoryneuroprogenitorsforhighthroughputgenerationoffunctionalauditoryneuronsinvitro
AT sipionerebecca wntactivationandtgfbsmadinhibitionpotentiatestemnessofmammalianauditoryneuroprogenitorsforhighthroughputgenerationoffunctionalauditoryneuronsinvitro
AT kleinlogelsonja wntactivationandtgfbsmadinhibitionpotentiatestemnessofmammalianauditoryneuroprogenitorsforhighthroughputgenerationoffunctionalauditoryneuronsinvitro
AT sennpascal wntactivationandtgfbsmadinhibitionpotentiatestemnessofmammalianauditoryneuroprogenitorsforhighthroughputgenerationoffunctionalauditoryneuronsinvitro

Ejemplares similares