Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.

During embryonic organogenesis, the odontogenic potential resides in dental mesenchyme from the bud stage until birth. Mouse dental mesenchymal cells (mDMCs) isolated from the inductive dental mesenchyme of developing molars are frequently used in the context of tooth development and regeneration. W...

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Main Authors: Yunfei Zheng, Jinglei Cai, Andrew Paul Hutchins, Lingfei Jia, Pengfei Liu, Dandan Yang, Shubin Chen, Lihong Ge, Duanqing Pei, Shicheng Wei
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2016-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC4822848?pdf=render
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spelling doaj-bdca67ae89a6457cbfdcee592531f1fa2020-11-25T02:33:38ZengPublic Library of Science (PLoS)PLoS ONE1932-62032016-01-01114e015289310.1371/journal.pone.0152893Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.Yunfei ZhengJinglei CaiAndrew Paul HutchinsLingfei JiaPengfei LiuDandan YangShubin ChenLihong GeDuanqing PeiShicheng WeiDuring embryonic organogenesis, the odontogenic potential resides in dental mesenchyme from the bud stage until birth. Mouse dental mesenchymal cells (mDMCs) isolated from the inductive dental mesenchyme of developing molars are frequently used in the context of tooth development and regeneration. We wondered if and how the odontogenic potential could be retained when mDMCs were cultured in vitro. In the present study, we undertook to test the odontogenic potential of cultured mDMCs and attempted to maintain the potential during culturing. We found that cultured mDMCs could retain the odontogenic potential for 24 h with a ratio of 60% for tooth formation, but mDMCs were incapable of supporting tooth formation after more than 24 h in culture. This loss of odontogenic potential was accompanied by widespread transcriptomic alteration and, specifically, the downregulation of some dental mesenchyme-specific genes, such as Pax9, Msx1, and Pdgfrα. To prolong the odontogenic potential of mDMCs in vitro, we then cultured mDMCs in a serum-free medium with Knockout Serum Replacement (KSR) and growth factors (fibroblastic growth factor 2 and epidermal growth factor). In this new micromilieu, mDMCs could maintain the odontogenic potential for 48 h with tooth formation ratio of 50%. Moreover, mDMCs cultured in KSR-supplemented medium gave rise to tooth-like structures when recombined with non-dental second-arch epithelium. Among the supplements, KSR is essential for the survival and adhesion of mDMCs, and both Egf and Fgf2 induced the expression of certain dental mesenchyme-related genes. Taken together, our results demonstrated that the transcriptomic changes responded to the alteration of odontogenic potential in cultured mDMCs and a new micromilieu partly retained this potential in vitro, providing insight into the long-term maintenance of odontogenic potential in mDMCs.http://europepmc.org/articles/PMC4822848?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Yunfei Zheng
Jinglei Cai
Andrew Paul Hutchins
Lingfei Jia
Pengfei Liu
Dandan Yang
Shubin Chen
Lihong Ge
Duanqing Pei
Shicheng Wei
spellingShingle Yunfei Zheng
Jinglei Cai
Andrew Paul Hutchins
Lingfei Jia
Pengfei Liu
Dandan Yang
Shubin Chen
Lihong Ge
Duanqing Pei
Shicheng Wei
Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.
PLoS ONE
author_facet Yunfei Zheng
Jinglei Cai
Andrew Paul Hutchins
Lingfei Jia
Pengfei Liu
Dandan Yang
Shubin Chen
Lihong Ge
Duanqing Pei
Shicheng Wei
author_sort Yunfei Zheng
title Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.
title_short Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.
title_full Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.
title_fullStr Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.
title_full_unstemmed Remission for Loss of Odontogenic Potential in a New Micromilieu In Vitro.
title_sort remission for loss of odontogenic potential in a new micromilieu in vitro.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2016-01-01
description During embryonic organogenesis, the odontogenic potential resides in dental mesenchyme from the bud stage until birth. Mouse dental mesenchymal cells (mDMCs) isolated from the inductive dental mesenchyme of developing molars are frequently used in the context of tooth development and regeneration. We wondered if and how the odontogenic potential could be retained when mDMCs were cultured in vitro. In the present study, we undertook to test the odontogenic potential of cultured mDMCs and attempted to maintain the potential during culturing. We found that cultured mDMCs could retain the odontogenic potential for 24 h with a ratio of 60% for tooth formation, but mDMCs were incapable of supporting tooth formation after more than 24 h in culture. This loss of odontogenic potential was accompanied by widespread transcriptomic alteration and, specifically, the downregulation of some dental mesenchyme-specific genes, such as Pax9, Msx1, and Pdgfrα. To prolong the odontogenic potential of mDMCs in vitro, we then cultured mDMCs in a serum-free medium with Knockout Serum Replacement (KSR) and growth factors (fibroblastic growth factor 2 and epidermal growth factor). In this new micromilieu, mDMCs could maintain the odontogenic potential for 48 h with tooth formation ratio of 50%. Moreover, mDMCs cultured in KSR-supplemented medium gave rise to tooth-like structures when recombined with non-dental second-arch epithelium. Among the supplements, KSR is essential for the survival and adhesion of mDMCs, and both Egf and Fgf2 induced the expression of certain dental mesenchyme-related genes. Taken together, our results demonstrated that the transcriptomic changes responded to the alteration of odontogenic potential in cultured mDMCs and a new micromilieu partly retained this potential in vitro, providing insight into the long-term maintenance of odontogenic potential in mDMCs.
url http://europepmc.org/articles/PMC4822848?pdf=render
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