Primordial germ cell specification from embryonic stem cells.

BACKGROUND: Primordial germ cell (PGC) specification is the first crucial step in germ line development. However, owing to significant challenges regarding the in vivo system, such as the complex cellular environment and potential problems with embryo manipulation, it is desirable to generate embryo...

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Main Authors: Wei Wei, Tingting Qing, Xin Ye, Haisong Liu, Donghui Zhang, Weifeng Yang, Hongkui Deng
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2008-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC2602984?pdf=render
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author Wei Wei
Tingting Qing
Xin Ye
Haisong Liu
Donghui Zhang
Weifeng Yang
Hongkui Deng
author_facet Wei Wei
Tingting Qing
Xin Ye
Haisong Liu
Donghui Zhang
Weifeng Yang
Hongkui Deng
author_sort Wei Wei
collection DOAJ
description BACKGROUND: Primordial germ cell (PGC) specification is the first crucial step in germ line development. However, owing to significant challenges regarding the in vivo system, such as the complex cellular environment and potential problems with embryo manipulation, it is desirable to generate embryonic stem (ES) cells that are capable of overcoming these aforementioned limitations in order to provide a potential in vitro model to recapitulate the developmental processes in vivo. METHODOLOGY AND PRINCIPAL FINDINGS: Here, we studied the detailed process of PGC specification from stella-GFP ES cells. We first observed the heterogeneous expression of stella in ES cells. However, neither Stella-positive ES cells nor Stella-negative ES cells shared a similar gene expression pattern with either PGCs or PGC precursors. Second, we derived PGCs from ES cells using two differentiation methods, namely the attachment culture technique and the embryoid body (EB) method. Compared with PGCs derived via the attachment culture technique, PGCs derived via the EB method that had undergone the sequential erasure of Peg3 followed by Igf2r resulted in a cell line in which the expression dynamics of T, Fgf8 and Sox17, in addition to the expression of the epiblast markers, were more similar to the in vivo expression, thus demonstrating that the process of PGC derivation was more faithfully recapitulated using the EB method. Furthermore, we developed an in vitro model of PGC specification in a completely chemically defined medium (CDM) that indicated that BMP4 and Wnt3a promoted PGC derivation, whereas BMP8b and activinA had no observable effect on PGC derivation. CONCLUSIONS AND SIGNIFICANCE: The in vitro model we have established can recapitulate the developmental processes in vivo and provides new insights into the mechanism of PGC specification.
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spelling doaj.art-9b96bce1fb224c06b384cf4d2ea447ee2022-12-22T02:51:38ZengPublic Library of Science (PLoS)PLoS ONE1932-62032008-01-01312e401310.1371/journal.pone.0004013Primordial germ cell specification from embryonic stem cells.Wei WeiTingting QingXin YeHaisong LiuDonghui ZhangWeifeng YangHongkui DengBACKGROUND: Primordial germ cell (PGC) specification is the first crucial step in germ line development. However, owing to significant challenges regarding the in vivo system, such as the complex cellular environment and potential problems with embryo manipulation, it is desirable to generate embryonic stem (ES) cells that are capable of overcoming these aforementioned limitations in order to provide a potential in vitro model to recapitulate the developmental processes in vivo. METHODOLOGY AND PRINCIPAL FINDINGS: Here, we studied the detailed process of PGC specification from stella-GFP ES cells. We first observed the heterogeneous expression of stella in ES cells. However, neither Stella-positive ES cells nor Stella-negative ES cells shared a similar gene expression pattern with either PGCs or PGC precursors. Second, we derived PGCs from ES cells using two differentiation methods, namely the attachment culture technique and the embryoid body (EB) method. Compared with PGCs derived via the attachment culture technique, PGCs derived via the EB method that had undergone the sequential erasure of Peg3 followed by Igf2r resulted in a cell line in which the expression dynamics of T, Fgf8 and Sox17, in addition to the expression of the epiblast markers, were more similar to the in vivo expression, thus demonstrating that the process of PGC derivation was more faithfully recapitulated using the EB method. Furthermore, we developed an in vitro model of PGC specification in a completely chemically defined medium (CDM) that indicated that BMP4 and Wnt3a promoted PGC derivation, whereas BMP8b and activinA had no observable effect on PGC derivation. CONCLUSIONS AND SIGNIFICANCE: The in vitro model we have established can recapitulate the developmental processes in vivo and provides new insights into the mechanism of PGC specification.http://europepmc.org/articles/PMC2602984?pdf=render
spellingShingle Wei Wei
Tingting Qing
Xin Ye
Haisong Liu
Donghui Zhang
Weifeng Yang
Hongkui Deng
Primordial germ cell specification from embryonic stem cells.
PLoS ONE
title Primordial germ cell specification from embryonic stem cells.
title_full Primordial germ cell specification from embryonic stem cells.
title_fullStr Primordial germ cell specification from embryonic stem cells.
title_full_unstemmed Primordial germ cell specification from embryonic stem cells.
title_short Primordial germ cell specification from embryonic stem cells.
title_sort primordial germ cell specification from embryonic stem cells
url http://europepmc.org/articles/PMC2602984?pdf=render
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AT donghuizhang primordialgermcellspecificationfromembryonicstemcells
AT weifengyang primordialgermcellspecificationfromembryonicstemcells
AT hongkuideng primordialgermcellspecificationfromembryonicstemcells