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Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells

Biologists rely on morphology, function and specific markers to define the differentiation status of cells. Transcript profiling has expanded the repertoire of these markers by providing the snapshot of cellular status that reflects the activity of all genes. However, such data have been used only t...

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Detalles Bibliográficos
Autores principales: Aiba, Kazuhiro, Nedorezov, Timur, Piao, Yulan, Nishiyama, Akira, Matoba, Ryo, Sharova, Lioudmila V., Sharov, Alexei A., Yamanaka, Shinya, Niwa, Hitoshi, Ko, Minoru S. H.
Formato: Texto
Lenguaje:English
Publicado: Oxford University Press 2009
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2644347/
https://www.ncbi.nlm.nih.gov/pubmed/19112179
http://dx.doi.org/10.1093/dnares/dsn035
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author Aiba, Kazuhiro
Nedorezov, Timur
Piao, Yulan
Nishiyama, Akira
Matoba, Ryo
Sharova, Lioudmila V.
Sharov, Alexei A.
Yamanaka, Shinya
Niwa, Hitoshi
Ko, Minoru S. H.
author_facet Aiba, Kazuhiro
Nedorezov, Timur
Piao, Yulan
Nishiyama, Akira
Matoba, Ryo
Sharova, Lioudmila V.
Sharov, Alexei A.
Yamanaka, Shinya
Niwa, Hitoshi
Ko, Minoru S. H.
author_sort Aiba, Kazuhiro
collection PubMed
description Biologists rely on morphology, function and specific markers to define the differentiation status of cells. Transcript profiling has expanded the repertoire of these markers by providing the snapshot of cellular status that reflects the activity of all genes. However, such data have been used only to assess relative similarities and differences of these cells. Here we show that principal component analysis of global gene expression profiles map cells in multidimensional transcript profile space and the positions of differentiating cells progress in a stepwise manner along trajectories starting from undifferentiated embryonic stem (ES) cells located in the apex. We present three ‘cell lineage trajectories’, which represent the differentiation of ES cells into the first three lineages in mammalian development: primitive endoderm, trophoblast and primitive ectoderm/neural ectoderm. The positions of the cells along these trajectories seem to reflect the developmental potency of cells and can be used as a scale for the potential of cells. Indeed, we show that embryonic germ cells and induced pluripotent cells are mapped near the origin of the trajectories, whereas mouse embryo fibroblast and fibroblast cell lines are mapped near the far end of the trajectories. We suggest that this method can be used as the non-operational semi-quantitative definition of cell differentiation status and developmental potency. Furthermore, the global expression profiles of cell lineages provide a framework for the future study of in vitro and in vivo cell differentiation.
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spelling pubmed-26443472009-04-13 Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells Aiba, Kazuhiro Nedorezov, Timur Piao, Yulan Nishiyama, Akira Matoba, Ryo Sharova, Lioudmila V. Sharov, Alexei A. Yamanaka, Shinya Niwa, Hitoshi Ko, Minoru S. H. DNA Res Full Papers Biologists rely on morphology, function and specific markers to define the differentiation status of cells. Transcript profiling has expanded the repertoire of these markers by providing the snapshot of cellular status that reflects the activity of all genes. However, such data have been used only to assess relative similarities and differences of these cells. Here we show that principal component analysis of global gene expression profiles map cells in multidimensional transcript profile space and the positions of differentiating cells progress in a stepwise manner along trajectories starting from undifferentiated embryonic stem (ES) cells located in the apex. We present three ‘cell lineage trajectories’, which represent the differentiation of ES cells into the first three lineages in mammalian development: primitive endoderm, trophoblast and primitive ectoderm/neural ectoderm. The positions of the cells along these trajectories seem to reflect the developmental potency of cells and can be used as a scale for the potential of cells. Indeed, we show that embryonic germ cells and induced pluripotent cells are mapped near the origin of the trajectories, whereas mouse embryo fibroblast and fibroblast cell lines are mapped near the far end of the trajectories. We suggest that this method can be used as the non-operational semi-quantitative definition of cell differentiation status and developmental potency. Furthermore, the global expression profiles of cell lineages provide a framework for the future study of in vitro and in vivo cell differentiation. Oxford University Press 2009-02 2008-12-26 /pmc/articles/PMC2644347/ /pubmed/19112179 http://dx.doi.org/10.1093/dnares/dsn035 Text en Published by Oxford University Press 2008
spellingShingle Full Papers
Aiba, Kazuhiro
Nedorezov, Timur
Piao, Yulan
Nishiyama, Akira
Matoba, Ryo
Sharova, Lioudmila V.
Sharov, Alexei A.
Yamanaka, Shinya
Niwa, Hitoshi
Ko, Minoru S. H.
Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells
title Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells
title_full Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells
title_fullStr Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells
title_full_unstemmed Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells
title_short Defining Developmental Potency and Cell Lineage Trajectories by Expression Profiling of Differentiating Mouse Embryonic Stem Cells
title_sort defining developmental potency and cell lineage trajectories by expression profiling of differentiating mouse embryonic stem cells
topic Full Papers
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2644347/
https://www.ncbi.nlm.nih.gov/pubmed/19112179
http://dx.doi.org/10.1093/dnares/dsn035
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