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Tooth Engineering: Searching for Dental Mesenchymal Cells Sources

The implantation of cultured re-associations between embryonic dental mesenchymal cells and epithelial cells from mouse molars at embryonic day 14 (ED14) allowed making full teeth with crown, root, periodontal ligament fibers, and bone. Although representing valuable tools to set up methodologies em...

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Autores principales: Keller, Laetitia, Kuchler-Bopp, Sabine, Mendoza, Soledad Acuña, Poliard, Anne, Lesot, Hervé
Formato: Texto
Lenguaje:English
Publicado: Frontiers Research Foundation 2011
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3070478/
https://www.ncbi.nlm.nih.gov/pubmed/21483728
http://dx.doi.org/10.3389/fphys.2011.00007
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author Keller, Laetitia
Kuchler-Bopp, Sabine
Mendoza, Soledad Acuña
Poliard, Anne
Lesot, Hervé
author_facet Keller, Laetitia
Kuchler-Bopp, Sabine
Mendoza, Soledad Acuña
Poliard, Anne
Lesot, Hervé
author_sort Keller, Laetitia
collection PubMed
description The implantation of cultured re-associations between embryonic dental mesenchymal cells and epithelial cells from mouse molars at embryonic day 14 (ED14) allowed making full teeth with crown, root, periodontal ligament fibers, and bone. Although representing valuable tools to set up methodologies embryonic cells are not easily available. This work thus aimed to replace the embryonic cells by dental mesenchymal cell lines or cultured expanded embryonic cells, and to test their ability to mediate tooth development in vitro when re-associated with a competent dental epithelium. Histology, immunostaining and RT-PCR allowed getting complementary sets of results. Two different immortalized cell lines from ED18 dental mesenchyme failed in mediating tooth formation. The potentialities of embryonic dental mesenchymal cells decreased from ED14 to ED16 and were lost at ED18. This is likely related to a change in the mesenchymal cell phenotype and/or populations during development. Attempts to cultivate ED14 or ED16 embryonic dental mesenchymal cells prior to re-association led to the loss of their ability to support tooth development. This was accompanied by a down-regulation of Fgf3 transcription. Supplementation of the culture medium with FGF2 allowed restoring Fgf3 expression, but not the ability of mesenchymal cells to engage in tooth formation. Altogether, these observations suggest that a competent cell population exists in the dental mesenchyme at ED14, progressively decreases during development, and cannot as such be maintained in vitro. This study evidenced the need for specific conditions to maintain the ability of dental mesenchymal cells to initiate whole tooth formation, when re-associated with an odontogenic epithelium. Efforts to improve the culture conditions will have to be combined with attempts to characterize the competent cells within the dental mesenchyme.
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spelling pubmed-30704782011-04-11 Tooth Engineering: Searching for Dental Mesenchymal Cells Sources Keller, Laetitia Kuchler-Bopp, Sabine Mendoza, Soledad Acuña Poliard, Anne Lesot, Hervé Front Physiol Physiology The implantation of cultured re-associations between embryonic dental mesenchymal cells and epithelial cells from mouse molars at embryonic day 14 (ED14) allowed making full teeth with crown, root, periodontal ligament fibers, and bone. Although representing valuable tools to set up methodologies embryonic cells are not easily available. This work thus aimed to replace the embryonic cells by dental mesenchymal cell lines or cultured expanded embryonic cells, and to test their ability to mediate tooth development in vitro when re-associated with a competent dental epithelium. Histology, immunostaining and RT-PCR allowed getting complementary sets of results. Two different immortalized cell lines from ED18 dental mesenchyme failed in mediating tooth formation. The potentialities of embryonic dental mesenchymal cells decreased from ED14 to ED16 and were lost at ED18. This is likely related to a change in the mesenchymal cell phenotype and/or populations during development. Attempts to cultivate ED14 or ED16 embryonic dental mesenchymal cells prior to re-association led to the loss of their ability to support tooth development. This was accompanied by a down-regulation of Fgf3 transcription. Supplementation of the culture medium with FGF2 allowed restoring Fgf3 expression, but not the ability of mesenchymal cells to engage in tooth formation. Altogether, these observations suggest that a competent cell population exists in the dental mesenchyme at ED14, progressively decreases during development, and cannot as such be maintained in vitro. This study evidenced the need for specific conditions to maintain the ability of dental mesenchymal cells to initiate whole tooth formation, when re-associated with an odontogenic epithelium. Efforts to improve the culture conditions will have to be combined with attempts to characterize the competent cells within the dental mesenchyme. Frontiers Research Foundation 2011-03-04 /pmc/articles/PMC3070478/ /pubmed/21483728 http://dx.doi.org/10.3389/fphys.2011.00007 Text en Copyright © 2011 Keller, Kuchler-Bopp, Mendoza, Poliard and Lesot. http://www.frontiersin.org/licenseagreement This is an open-access article subject to an exclusive license agreement between the authors and Frontiers Media SA, which permits unrestricted use, distribution, and reproduction in any medium, provided the original authors and source are credited.
spellingShingle Physiology
Keller, Laetitia
Kuchler-Bopp, Sabine
Mendoza, Soledad Acuña
Poliard, Anne
Lesot, Hervé
Tooth Engineering: Searching for Dental Mesenchymal Cells Sources
title Tooth Engineering: Searching for Dental Mesenchymal Cells Sources
title_full Tooth Engineering: Searching for Dental Mesenchymal Cells Sources
title_fullStr Tooth Engineering: Searching for Dental Mesenchymal Cells Sources
title_full_unstemmed Tooth Engineering: Searching for Dental Mesenchymal Cells Sources
title_short Tooth Engineering: Searching for Dental Mesenchymal Cells Sources
title_sort tooth engineering: searching for dental mesenchymal cells sources
topic Physiology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3070478/
https://www.ncbi.nlm.nih.gov/pubmed/21483728
http://dx.doi.org/10.3389/fphys.2011.00007
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