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Generation of iPSC-Derived Human Peripheral Sensory Neurons Releasing Substance P Elicited by TRPV1 Agonists

Authors :
Marília Z. P. Guimarães
Rodrigo De Vecchi
Gabriela Vitória
Jaroslaw K. Sochacki
Bruna S. Paulsen
Igor Lima
Felipe Rodrigues da Silva
Rodrigo F. M. da Costa
Newton G. Castro
Lionel Breton
Stevens K. Rehen
MARÍLIA Z. P. GUIMARÃES, D’Or Institute for Research and Education, UFRJ
GABRIELA VITÓRIA, L’Oréal Research & Innovation
JAROSLAW K. SOCHACKI, L’Oréal Research & Innovation
BRUNA S. PAULSEN, L’Oréal Research & Innovation
IGOR LIMA, L’Oréal Research & Innovation
RODRIGO DE VECCHI, L’Oréal Research & Innovation, Unicamp
RODRIGO F. M. DA COSTA, L’Oréal Research & Innovation
NEWTON G. CASTRO, UFRJ
LIONEL BRETON, L’Oréal Research & Innovation
STEVENS K. REHEN, D’Or Institute for Research and Education, UFRJ.
FELIPE RODRIGUES DA SILVA, CNPTIA, Unicamp
Source :
Frontiers in Molecular Neuroscience, Repositório Institucional da EMBRAPA (Repository Open Access to Scientific Information from EMBRAPA-Alice), Empresa Brasileira de Pesquisa Agropecuária (Embrapa), instacron:EMBRAPA, Frontiers in Molecular Neuroscience, Vol 11 (2018)
Publication Year :
2018
Publisher :
Frontiers Media, 2018.

Abstract

Neural crest stem cells (NCPCs) have been shown to differentiate into various cell types and tissues during embryonic development, including sensory neurons. The few studies addressing the generation of NCPCs and peripheral sensory neurons (PSNs) from human induced pluripotent stem cells (hiPSCs), generated sensory cells without displaying robust activity. Here, we describe an efficient strategy for hiPSCs differentiation into NCPCs and functional PSNs using chemically defined media and factors to achieve efficient differentiation, confirmed by the expression of specific markers. After 10 days hiPSCs differentiated into NCPCs, cells were then maintained in neural induction medium containing defined growth factors for PSNs differentiation, followed by 10 days in neonatal human epidermal keratinocytes- (HEKn-) conditioned medium (CM). We observed a further increase in PSN markers expression and neurites length after CM treatment. The resulting neurons elicited action potentials after current injection and released substance P (SP) in response to nociceptive agents such as anandamide and resiniferatoxin. Anandamide induced substance P release via activation of TRPV1 and not CB1. Transcriptomic analysis of the PSNs revealed the main dorsal root ganglia neuronal markers and a transcriptional profile compatible with C fiber-low threshold mechanoreceptors. TRPV1 was detected by immunofluorescence and RNA-Seq in multiple experiments. In conclusion, the developed strategy generated PSNs useful for drug screening that could be applied to patient-derived hiPSCs, consisting in a powerful tool to model human diseases in vitro. Made available in DSpace on 2019-02-07T23:37:27Z (GMT). No. of bitstreams: 1 APGenerationiPSCFelipe.pdf: 7505321 bytes, checksum: 135c87796cec61c67776b2a6e5db7f0f (MD5) Previous issue date: 2019-02-07 Article 277.

Details

Language :
English
Database :
OpenAIRE
Journal :
Frontiers in Molecular Neuroscience, Repositório Institucional da EMBRAPA (Repository Open Access to Scientific Information from EMBRAPA-Alice), Empresa Brasileira de Pesquisa Agropecuária (Embrapa), instacron:EMBRAPA, Frontiers in Molecular Neuroscience, Vol 11 (2018)
Accession number :
edsair.doi.dedup.....5f1c1460be31266949f712b331df4dff