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Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors

Numerous studies have shown the recovery of auditory function in mouse models of genetic hearing loss following AAV gene therapy, yet translation to the clinic has not yet been demonstrated. One limitation has been the lack of human inner ear cell lines or tissues for validating viral gene therapies...

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Autores principales: van Beelen, Edward S. A., van der Valk, Wouter H., Verhagen, Thijs O., de Groot, John C. M. J., Madison, Margot A., Shadmanfar, Wijs, Hensen, Erik F., Jansen, Jeroen C., van Benthem, Peter Paul G., Holt, Jeffrey R., Locher, Heiko
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2022
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9221426/
https://www.ncbi.nlm.nih.gov/pubmed/35740941
http://dx.doi.org/10.3390/biom12060816
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author van Beelen, Edward S. A.
van der Valk, Wouter H.
Verhagen, Thijs O.
de Groot, John C. M. J.
Madison, Margot A.
Shadmanfar, Wijs
Hensen, Erik F.
Jansen, Jeroen C.
van Benthem, Peter Paul G.
Holt, Jeffrey R.
Locher, Heiko
author_facet van Beelen, Edward S. A.
van der Valk, Wouter H.
Verhagen, Thijs O.
de Groot, John C. M. J.
Madison, Margot A.
Shadmanfar, Wijs
Hensen, Erik F.
Jansen, Jeroen C.
van Benthem, Peter Paul G.
Holt, Jeffrey R.
Locher, Heiko
author_sort van Beelen, Edward S. A.
collection PubMed
description Numerous studies have shown the recovery of auditory function in mouse models of genetic hearing loss following AAV gene therapy, yet translation to the clinic has not yet been demonstrated. One limitation has been the lack of human inner ear cell lines or tissues for validating viral gene therapies. Cultured human inner ear tissue could help confirm viral tropism and efficacy for driving exogenous gene expression in targeted cell types, establish promoter efficacy and perhaps selectivity for targeted cells, confirm the expression of therapeutic constructs and the subcellular localization of therapeutic proteins, and address the potential cellular toxicity of vectors or exogenous constructs. To begin to address these questions, we developed an explant culture method using native human inner ear tissue excised at either fetal or adult stages. Inner ear sensory epithelia were cultured for four days and exposed to vectors encoding enhanced green fluorescent protein (eGFP). We focused on the synthetic AAV9-PHP.B capsid, which has been demonstrated to be efficient for driving eGFP expression in the sensory hair cells of mouse and non-human primate inner ears. We report that AAV9-PHP.B also drives eGFP expression in fetal cochlear hair cells and in fetal and adult vestibular hair cells in explants of human inner ear sensory epithelia, which suggests that both the experimental paradigm and the viral capsid may be valuable for translation to clinical application.
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spelling pubmed-92214262022-06-24 Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors van Beelen, Edward S. A. van der Valk, Wouter H. Verhagen, Thijs O. de Groot, John C. M. J. Madison, Margot A. Shadmanfar, Wijs Hensen, Erik F. Jansen, Jeroen C. van Benthem, Peter Paul G. Holt, Jeffrey R. Locher, Heiko Biomolecules Article Numerous studies have shown the recovery of auditory function in mouse models of genetic hearing loss following AAV gene therapy, yet translation to the clinic has not yet been demonstrated. One limitation has been the lack of human inner ear cell lines or tissues for validating viral gene therapies. Cultured human inner ear tissue could help confirm viral tropism and efficacy for driving exogenous gene expression in targeted cell types, establish promoter efficacy and perhaps selectivity for targeted cells, confirm the expression of therapeutic constructs and the subcellular localization of therapeutic proteins, and address the potential cellular toxicity of vectors or exogenous constructs. To begin to address these questions, we developed an explant culture method using native human inner ear tissue excised at either fetal or adult stages. Inner ear sensory epithelia were cultured for four days and exposed to vectors encoding enhanced green fluorescent protein (eGFP). We focused on the synthetic AAV9-PHP.B capsid, which has been demonstrated to be efficient for driving eGFP expression in the sensory hair cells of mouse and non-human primate inner ears. We report that AAV9-PHP.B also drives eGFP expression in fetal cochlear hair cells and in fetal and adult vestibular hair cells in explants of human inner ear sensory epithelia, which suggests that both the experimental paradigm and the viral capsid may be valuable for translation to clinical application. MDPI 2022-06-10 /pmc/articles/PMC9221426/ /pubmed/35740941 http://dx.doi.org/10.3390/biom12060816 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
van Beelen, Edward S. A.
van der Valk, Wouter H.
Verhagen, Thijs O.
de Groot, John C. M. J.
Madison, Margot A.
Shadmanfar, Wijs
Hensen, Erik F.
Jansen, Jeroen C.
van Benthem, Peter Paul G.
Holt, Jeffrey R.
Locher, Heiko
Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors
title Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors
title_full Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors
title_fullStr Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors
title_full_unstemmed Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors
title_short Efficient Viral Transduction in Fetal and Adult Human Inner Ear Explants with AAV9-PHP.B Vectors
title_sort efficient viral transduction in fetal and adult human inner ear explants with aav9-php.b vectors
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9221426/
https://www.ncbi.nlm.nih.gov/pubmed/35740941
http://dx.doi.org/10.3390/biom12060816
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