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BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin

Because mouse embryonic stem cells (mESCs) do not contribute to the formation of extraembryonic placenta when they are injected into blastocysts, it is believed that mESCs do not differentiate into trophoblast whereas human embryonic stem cells (hESCs) can express trophoblast markers when exposed to...

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Autores principales: Hayashi, Yohei, Furue, Miho Kusuda, Tanaka, Satoshi, Hirose, Michiko, Wakisaka, Noriko, Danno, Hiroki, Ohnuma, Kiyoshi, Oeda, Shiho, Aihara, Yuko, Shiota, Kunio, Ogura, Atsuo, Ishiura, Shoichi, Asashima, Makoto
Formato: Texto
Lenguaje:English
Publicado: Springer-Verlag 2009
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2862943/
https://www.ncbi.nlm.nih.gov/pubmed/20033790
http://dx.doi.org/10.1007/s11626-009-9266-6
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author Hayashi, Yohei
Furue, Miho Kusuda
Tanaka, Satoshi
Hirose, Michiko
Wakisaka, Noriko
Danno, Hiroki
Ohnuma, Kiyoshi
Oeda, Shiho
Aihara, Yuko
Shiota, Kunio
Ogura, Atsuo
Ishiura, Shoichi
Asashima, Makoto
author_facet Hayashi, Yohei
Furue, Miho Kusuda
Tanaka, Satoshi
Hirose, Michiko
Wakisaka, Noriko
Danno, Hiroki
Ohnuma, Kiyoshi
Oeda, Shiho
Aihara, Yuko
Shiota, Kunio
Ogura, Atsuo
Ishiura, Shoichi
Asashima, Makoto
author_sort Hayashi, Yohei
collection PubMed
description Because mouse embryonic stem cells (mESCs) do not contribute to the formation of extraembryonic placenta when they are injected into blastocysts, it is believed that mESCs do not differentiate into trophoblast whereas human embryonic stem cells (hESCs) can express trophoblast markers when exposed to bone morphogenetic protein 4 (BMP4) in vitro. To test whether mESCs have the potential to differentiate into trophoblast, we assessed the effect of BMP4 on mESCs in a defined monolayer culture condition. The expression of trophoblast-specific transcription factors such as Cdx2, Dlx3, Esx1, Gata3, Hand1, Mash2, and Plx1 was specifically upregulated in the BMP4-treated differentiated cells, and these cells expressed trophoblast markers. These results suggest that BMP4 treatment in defined culture conditions enabled mESCs to differentiate into trophoblast. This differentiation was inhibited by serum or leukemia inhibitory factor, which are generally used for mESC culture. In addition, we studied the mechanism underlying BMP4-directed mESC differentiation into trophoblast. Our results showed that BMP4 activates the Smad pathway in mESCs inducing Cdx2 expression, which plays a crucial role in trophoblast differentiation, through the binding of Smad protein to the Cdx2 genomic enhancer sequence. Our findings imply that there is a common molecular mechanism underlying hESC and mESC differentiation into trophoblast.
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spelling pubmed-28629432010-05-04 BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin Hayashi, Yohei Furue, Miho Kusuda Tanaka, Satoshi Hirose, Michiko Wakisaka, Noriko Danno, Hiroki Ohnuma, Kiyoshi Oeda, Shiho Aihara, Yuko Shiota, Kunio Ogura, Atsuo Ishiura, Shoichi Asashima, Makoto In Vitro Cell Dev Biol Anim Article Because mouse embryonic stem cells (mESCs) do not contribute to the formation of extraembryonic placenta when they are injected into blastocysts, it is believed that mESCs do not differentiate into trophoblast whereas human embryonic stem cells (hESCs) can express trophoblast markers when exposed to bone morphogenetic protein 4 (BMP4) in vitro. To test whether mESCs have the potential to differentiate into trophoblast, we assessed the effect of BMP4 on mESCs in a defined monolayer culture condition. The expression of trophoblast-specific transcription factors such as Cdx2, Dlx3, Esx1, Gata3, Hand1, Mash2, and Plx1 was specifically upregulated in the BMP4-treated differentiated cells, and these cells expressed trophoblast markers. These results suggest that BMP4 treatment in defined culture conditions enabled mESCs to differentiate into trophoblast. This differentiation was inhibited by serum or leukemia inhibitory factor, which are generally used for mESC culture. In addition, we studied the mechanism underlying BMP4-directed mESC differentiation into trophoblast. Our results showed that BMP4 activates the Smad pathway in mESCs inducing Cdx2 expression, which plays a crucial role in trophoblast differentiation, through the binding of Smad protein to the Cdx2 genomic enhancer sequence. Our findings imply that there is a common molecular mechanism underlying hESC and mESC differentiation into trophoblast. Springer-Verlag 2009-12-24 2010 /pmc/articles/PMC2862943/ /pubmed/20033790 http://dx.doi.org/10.1007/s11626-009-9266-6 Text en © The Author(s) 2009 https://creativecommons.org/licenses/by-nc/4.0/ This article is distributed under the terms of the Creative Commons Attribution Noncommercial License which permits any noncommercial use, distribution, and reproduction in any medium, provided the original author(s) and source are credited.
spellingShingle Article
Hayashi, Yohei
Furue, Miho Kusuda
Tanaka, Satoshi
Hirose, Michiko
Wakisaka, Noriko
Danno, Hiroki
Ohnuma, Kiyoshi
Oeda, Shiho
Aihara, Yuko
Shiota, Kunio
Ogura, Atsuo
Ishiura, Shoichi
Asashima, Makoto
BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin
title BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin
title_full BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin
title_fullStr BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin
title_full_unstemmed BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin
title_short BMP4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin
title_sort bmp4 induction of trophoblast from mouse embryonic stem cells in defined culture conditions on laminin
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2862943/
https://www.ncbi.nlm.nih.gov/pubmed/20033790
http://dx.doi.org/10.1007/s11626-009-9266-6
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