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Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts

Although cloned embryos generated by somatic/embryonic stem cell nuclear transfer (SECNT) certainly give rise to viable individuals, they can often undergo embryonic arrest at any stage of embryogenesis, leading to diverse morphological abnormalities. In an effort to gain further insights into repro...

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Autores principales: Fukuda, Atsushi, Cao, Feng, Morita, Shinnosuke, Yamada, Kaori, Jincho, Yuko, Tane, Shouji, Sotomaru, Yusuke, Kono, Tomohiro
Formato: Texto
Lenguaje:English
Publicado: Public Library of Science 2010
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2894852/
https://www.ncbi.nlm.nih.gov/pubmed/20614022
http://dx.doi.org/10.1371/journal.pone.0011274
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author Fukuda, Atsushi
Cao, Feng
Morita, Shinnosuke
Yamada, Kaori
Jincho, Yuko
Tane, Shouji
Sotomaru, Yusuke
Kono, Tomohiro
author_facet Fukuda, Atsushi
Cao, Feng
Morita, Shinnosuke
Yamada, Kaori
Jincho, Yuko
Tane, Shouji
Sotomaru, Yusuke
Kono, Tomohiro
author_sort Fukuda, Atsushi
collection PubMed
description Although cloned embryos generated by somatic/embryonic stem cell nuclear transfer (SECNT) certainly give rise to viable individuals, they can often undergo embryonic arrest at any stage of embryogenesis, leading to diverse morphological abnormalities. In an effort to gain further insights into reprogramming and the properties of SECNT embryos, we performed a large-scale gene expression profiling of 87 single blastocysts using GeneChip microarrays. Sertoli cells, cumulus cells, and embryonic stem cells were used as donor cells. The gene expression profiles of 87 blastocysts were subjected to microarray analysis. Using principal component analysis and hierarchical clustering, the gene expression profiles were clearly classified into 3 clusters corresponding to the type of donor cell. The results revealed that each type of SECNT embryo had a unique gene expression profile that was strictly dependent upon the type of donor cells, although there was considerable variation among the individual profiles within each group. This suggests that the reprogramming process is distinct for embryos cloned from different types of donor cells. Furthermore, on the basis of the results of comparison analysis, we identified 35 genes that were inappropriately reprogrammed in most of the SECNT embryos; our findings demonstrated that some of these genes, such as Asz1, Xlr3a and App, were appropriately reprogrammed only in the embryos with a transcriptional profile that was the closest to that of the controls. Our findings provide a framework to further understand the reprogramming in SECNT embryos.
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spelling pubmed-28948522010-07-07 Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts Fukuda, Atsushi Cao, Feng Morita, Shinnosuke Yamada, Kaori Jincho, Yuko Tane, Shouji Sotomaru, Yusuke Kono, Tomohiro PLoS One Research Article Although cloned embryos generated by somatic/embryonic stem cell nuclear transfer (SECNT) certainly give rise to viable individuals, they can often undergo embryonic arrest at any stage of embryogenesis, leading to diverse morphological abnormalities. In an effort to gain further insights into reprogramming and the properties of SECNT embryos, we performed a large-scale gene expression profiling of 87 single blastocysts using GeneChip microarrays. Sertoli cells, cumulus cells, and embryonic stem cells were used as donor cells. The gene expression profiles of 87 blastocysts were subjected to microarray analysis. Using principal component analysis and hierarchical clustering, the gene expression profiles were clearly classified into 3 clusters corresponding to the type of donor cell. The results revealed that each type of SECNT embryo had a unique gene expression profile that was strictly dependent upon the type of donor cells, although there was considerable variation among the individual profiles within each group. This suggests that the reprogramming process is distinct for embryos cloned from different types of donor cells. Furthermore, on the basis of the results of comparison analysis, we identified 35 genes that were inappropriately reprogrammed in most of the SECNT embryos; our findings demonstrated that some of these genes, such as Asz1, Xlr3a and App, were appropriately reprogrammed only in the embryos with a transcriptional profile that was the closest to that of the controls. Our findings provide a framework to further understand the reprogramming in SECNT embryos. Public Library of Science 2010-06-30 /pmc/articles/PMC2894852/ /pubmed/20614022 http://dx.doi.org/10.1371/journal.pone.0011274 Text en Fukuda et al. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Fukuda, Atsushi
Cao, Feng
Morita, Shinnosuke
Yamada, Kaori
Jincho, Yuko
Tane, Shouji
Sotomaru, Yusuke
Kono, Tomohiro
Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts
title Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts
title_full Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts
title_fullStr Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts
title_full_unstemmed Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts
title_short Identification of Inappropriately Reprogrammed Genes by Large-Scale Transcriptome Analysis of Individual Cloned Mouse Blastocysts
title_sort identification of inappropriately reprogrammed genes by large-scale transcriptome analysis of individual cloned mouse blastocysts
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2894852/
https://www.ncbi.nlm.nih.gov/pubmed/20614022
http://dx.doi.org/10.1371/journal.pone.0011274
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