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  Governing cell lineage formation in cloned mouse embryos

Balbach, S. T., Esteves, T. C., Brink, T., Gentile, L., McLaughlin, K. J., Adjaye, J. A., et al. (2010). Governing cell lineage formation in cloned mouse embryos. Developmental Biology, 343(1-2), 71-83. doi:10.1016/j.ydbio.2010.04.012.

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Genre: Journal Article
Alternative Title : Dev Biol

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Balbach, S. T., Author
Esteves, T. C., Author
Brink, T.1, Author           
Gentile, L., Author
McLaughlin, K. J., Author
Adjaye, J. A.2, Author
Boiani, M., Author
Affiliations:
1Dept. of Vertebrate Genomics (Head: Hans Lehrach), Max Planck Institute for Molecular Genetics, Max Planck Society, ou_1433550              
2Max Planck Society, ou_persistent13              

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Free keywords: Animals; Cell Lineage; Cloning, Organism; Embryo, Mammalian/cytology/metabolism; Female; Homeodomain Proteins/genetics/metabolism; Male; Mice; Octamer Transcription Factor-3/genetics/metabolism; Trans-Activators/genetics/metabolism
 Abstract: Blastomeres of the pre-implantation mouse embryo form trophectoderm and inner cell mass via a process that requires the transcription factors Tead4, Cdx2, Oct4 and Nanog. In mouse morulae cloned by somatic cell nuclear transfer, we observed that the trophectoderm transcription factor Cdx2 is expressed very differently at the protein level compared to time- and stage-matched fertilized counterparts. Protein levels of Cdx2 in cloned embryos appear 'erratic,' i.e. are widely distributed, when plotted as histograms. In contrast to Cdx2, protein levels of the upstream factor Tead4 and of inner cell mass transcription factors Oct4 and Nanog are similar in cloned and fertilized embryos. These observations suggest that trophectoderm formation is initiated but not maintained correctly in cloned mouse morulae, which is consistent with cloned blastocysts' limited implantation and post-implantation success. Because a cell's ability to differentiate is greatly enhanced if it is surrounded by more cells differentiating the same way, a concept designated community effect by Gurdon, we reasoned that the insufficient cell numbers often observed in cloned embryos might lead to premature Cdx2 expression and differentiation of blastomeres into trophectoderm. Therefore, we created larger cloned embryos by aggregating them at the 4-cell stage. Homologous aggregation stimulates expression of multiple signaling pathways' components and results in cloned embryos with levels of Cdx2 similar to fertilized embryos. Most of the resultant morulae and blastocysts consist of cells of all three founders, indicating that aggregation increases stability of all of the individual components. We conclude that the induction of pluripotency in cloned embryos is more efficient than previously assumed, and we propose that a minimum cell number is necessary to stabilize pluripotency and inhibit premature expression of Cdx2 in cloned mouse embryos.

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Language(s): eng - English
 Dates: 2010-07-01
 Publication Status: Issued
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 Table of Contents: -
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 Identifiers: eDoc: 541918
DOI: 10.1016/j.ydbio.2010.04.012
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Title: Developmental Biology
  Alternative Title : Dev Biol
Source Genre: Journal
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Pages: - Volume / Issue: 343 (1-2) Sequence Number: - Start / End Page: 71 - 83 Identifier: ISSN: 1095-564X (Electronic)