Genetic Control of Otic Induction Sensorineural hearing loss due to auditory hair cell damage affects millions of Americans. Embryonic stem cells are a potential source for generation of otic progenitors and hair cells that could be highly useful for cell replacement therapies, developmental studies, and other applications. In order for the stem cell system to reach its full potential to recapitulate otic development and generate pure sensory epithelia in vitro, two critical barriers must be addressed. The first barrier is a lak of biomarkers unique to the otic sensory lineage that would enable unambiguous identification of otic cells. The second barrier is poor understanding of the genetic regulation of otic gene expression and lack of tools for live reporting in cells and embryos for purification of otic cell types. The overall goal of this project is to address these barriers through combined study of mouse inner ear development and stem cell culture to further our understanding of the molecular genetics of otic specification. This will be achieved in aim 1 by characterizing the expression and cell-fate lineage of the gene Fbxo2, which we identified as a highly specific otic sensory marker gene that spans developmental stages.
In aim 2, we will characterize mouse and human promoter/enhancer elements that regulate expression of this gene.
Aim 3 will evaluate Fbxo2 expression in stem cell derived otic progenitors, test the hypothesis that this gene is activated synergistically by specific otic transcription factors, and utilize Fbxo2 promote-driven reporters to purify stem cell-derived otic progenitors and solve the issue of stem cell heterogeneity. Achieving the proposed aims will: 1) improve knowledge of the genetic control of otic induction, 2) produce tools that target inner ear progenitors and sensory cells, 3) enable the in vitro culture and propagation of highly pure otic progenitors and 4) generate knowledge and tools for gene targeting and transplantation therapies for the inner ear.

Public Health Relevance

Embryonic stem cells are a promising source for inner ear progenitors but their efficient use is impeded by lack of biomarkers for purification and, poor understanding of genetic mechanisms of otic specification, which present substantial barriers to progress in the field. The overall goal of this project is to address these barriers through combined study of mouse inner ear development and stem cell culture to further our understanding of the molecular genetics of otic specification. Achieving the proposed aims will produce knowledge and tools for specific targeting and study of inner ear sensory progenitors and solve the issue of stem cell heterogeneity.

Agency
National Institute of Health (NIH)
Institute
National Institute on Deafness and Other Communication Disorders (NIDCD)
Type
Postdoctoral Individual National Research Service Award (F32)
Project #
1F32DC013210-01
Application #
8524802
Study Section
Special Emphasis Panel (ZDC1-SRB-R (38))
Program Officer
Sklare, Dan
Project Start
2013-04-01
Project End
2016-03-31
Budget Start
2013-04-01
Budget End
2014-03-31
Support Year
1
Fiscal Year
2013
Total Cost
$52,190
Indirect Cost
Name
Stanford University
Department
Otolaryngology
Type
Schools of Medicine
DUNS #
009214214
City
Stanford
State
CA
Country
United States
Zip Code
94305
Lee, Jiyoon; B?scke, Robert; Tang, Pei-Ciao et al. (2018) Hair Follicle Development in Mouse Pluripotent Stem Cell-Derived Skin Organoids. Cell Rep 22:242-254
Hartman, Byron H; B?scke, Robert; Ellwanger, Daniel C et al. (2018) Fbxo2VHC mouse and embryonic stem cell reporter lines delineate in vitro-generated inner ear sensory epithelia cells and enable otic lineage selection and Cre-recombination. Dev Biol 443:64-77
Hartman, Byron H; Durruthy-Durruthy, Robert; Laske, Roman D et al. (2015) Identification and characterization of mouse otic sensory lineage genes. Front Cell Neurosci 9:79
Durruthy-Durruthy, Robert; Gottlieb, Assaf; Hartman, Byron H et al. (2014) Reconstruction of the mouse otocyst and early neuroblast lineage at single-cell resolution. Cell 157:964-78