A Transgenic Mouse Marking Live Replicating Cells Reveals In Vivo Transcriptional Program of Proliferation

Agnes Klochendler; Noa Weinberg-Corem; Maya Moran; Avital Swisa; Nathalie Pochet; Virginia Savova; Jonas Vikeså; Yves Van de Peer; Michael Brandeis; Aviv Regev; Finn Cilius Nielsen; Yuval Dor; Amir Eden

doi:10.1016/j.devcel.2012.08.009

A Transgenic Mouse Marking Live Replicating Cells Reveals In Vivo Transcriptional Program of Proliferation

Agnes Klochendler, Noa Weinberg-Corem, Maya Moran, Avital Swisa, Nathalie Pochet, Virginia Savova, Jonas Vikeså, Yves Van de Peer, Michael Brandeis, Aviv Regev, Finn Cilius Nielsen, Yuval Dor, Amir Eden

The Hebrew University of Jerusalem

Research output: Contribution to journal › Article › peer-review

Abstract

Most adult mammalian tissues are quiescent, with rare cell divisions serving to maintain homeostasis. At present, the isolation and study of replicating cells from their in vivo niche typically involves immunostaining for intracellular markers of proliferation, causing the loss of sensitive biological material. We describe a transgenic mouse strain, expressing a CyclinB1-GFP fusion reporter, that marks replicating cells in the S/G2/M phases of the cell cycle. Using flow cytometry, we isolate live replicating cells from the liver and compare their transcriptome to that of quiescent cells to reveal gene expression programs associated with cell proliferation in vivo. We find that replicating hepatocytes have reduced expression of genes characteristic of liver differentiation. This reporter system provides a powerful platform for gene expression and metabolic and functional studies of replicating cells in their in vivo niche.

Original language	English
Pages (from-to)	681-690
Number of pages	10
Journal	Developmental Cell
Volume	23
Issue number	4
DOIs	https://doi.org/10.1016/j.devcel.2012.08.009
State	Published - 16 Oct 2012

All Science Journal Classification (ASJC) codes

Molecular Biology
General Biochemistry,Genetics and Molecular Biology
Developmental Biology
Cell Biology

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10.1016/j.devcel.2012.08.009

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Klochendler, A., Weinberg-Corem, N., Moran, M., Swisa, A., Pochet, N., Savova, V., Vikeså, J., Van de Peer, Y., Brandeis, M., Regev, A., Nielsen, F. C., Dor, Y., & Eden, A. (2012). A Transgenic Mouse Marking Live Replicating Cells Reveals In Vivo Transcriptional Program of Proliferation. Developmental Cell, 23(4), 681-690. https://doi.org/10.1016/j.devcel.2012.08.009

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title = "A Transgenic Mouse Marking Live Replicating Cells Reveals In Vivo Transcriptional Program of Proliferation",

abstract = "Most adult mammalian tissues are quiescent, with rare cell divisions serving to maintain homeostasis. At present, the isolation and study of replicating cells from their in vivo niche typically involves immunostaining for intracellular markers of proliferation, causing the loss of sensitive biological material. We describe a transgenic mouse strain, expressing a CyclinB1-GFP fusion reporter, that marks replicating cells in the S/G2/M phases of the cell cycle. Using flow cytometry, we isolate live replicating cells from the liver and compare their transcriptome to that of quiescent cells to reveal gene expression programs associated with cell proliferation in vivo. We find that replicating hepatocytes have reduced expression of genes characteristic of liver differentiation. This reporter system provides a powerful platform for gene expression and metabolic and functional studies of replicating cells in their in vivo niche.",

author = "Agnes Klochendler and Noa Weinberg-Corem and Maya Moran and Avital Swisa and Nathalie Pochet and Virginia Savova and Jonas Vikes{\aa} and {Van de Peer}, Yves and Michael Brandeis and Aviv Regev and Nielsen, {Finn Cilius} and Yuval Dor and Amir Eden",

note = "Funding Information: We thank Ittai Ben-Porath, Shmuel Ben-Sasson, Eithan Galun, Eli Pikarsky, and Gustavo Mostoslavsky for a critical reading of this manuscript, Abed Khalaileh for help in performing partial hepatectomy, and Benzi Zuberi for zygote infection. This work was funded by the Sixth Framework Programme of the European Union and the JDRF Center for Beta Cell Therapy in Diabetes and by an ERC starting grant (to Y.D.). This work was supported in part by a grant from USAID{\textquoteright}s American Schools and Hospitals Abroad (ASHA) Program for the upgrading of the Flow Cytometry Laboratory at the Hebrew University Medical School, I-CORE Program of the Planning and Budgeting Committee, and The Israel Science Foundation #41.11.",

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AU - Klochendler, Agnes

AU - Weinberg-Corem, Noa

AU - Moran, Maya

AU - Swisa, Avital

AU - Pochet, Nathalie

AU - Savova, Virginia

AU - Vikeså, Jonas

AU - Van de Peer, Yves

AU - Brandeis, Michael

AU - Regev, Aviv

AU - Nielsen, Finn Cilius

AU - Dor, Yuval

AU - Eden, Amir

N1 - Funding Information: We thank Ittai Ben-Porath, Shmuel Ben-Sasson, Eithan Galun, Eli Pikarsky, and Gustavo Mostoslavsky for a critical reading of this manuscript, Abed Khalaileh for help in performing partial hepatectomy, and Benzi Zuberi for zygote infection. This work was funded by the Sixth Framework Programme of the European Union and the JDRF Center for Beta Cell Therapy in Diabetes and by an ERC starting grant (to Y.D.). This work was supported in part by a grant from USAID’s American Schools and Hospitals Abroad (ASHA) Program for the upgrading of the Flow Cytometry Laboratory at the Hebrew University Medical School, I-CORE Program of the Planning and Budgeting Committee, and The Israel Science Foundation #41.11.

PY - 2012/10/16

Y1 - 2012/10/16

N2 - Most adult mammalian tissues are quiescent, with rare cell divisions serving to maintain homeostasis. At present, the isolation and study of replicating cells from their in vivo niche typically involves immunostaining for intracellular markers of proliferation, causing the loss of sensitive biological material. We describe a transgenic mouse strain, expressing a CyclinB1-GFP fusion reporter, that marks replicating cells in the S/G2/M phases of the cell cycle. Using flow cytometry, we isolate live replicating cells from the liver and compare their transcriptome to that of quiescent cells to reveal gene expression programs associated with cell proliferation in vivo. We find that replicating hepatocytes have reduced expression of genes characteristic of liver differentiation. This reporter system provides a powerful platform for gene expression and metabolic and functional studies of replicating cells in their in vivo niche.

AB - Most adult mammalian tissues are quiescent, with rare cell divisions serving to maintain homeostasis. At present, the isolation and study of replicating cells from their in vivo niche typically involves immunostaining for intracellular markers of proliferation, causing the loss of sensitive biological material. We describe a transgenic mouse strain, expressing a CyclinB1-GFP fusion reporter, that marks replicating cells in the S/G2/M phases of the cell cycle. Using flow cytometry, we isolate live replicating cells from the liver and compare their transcriptome to that of quiescent cells to reveal gene expression programs associated with cell proliferation in vivo. We find that replicating hepatocytes have reduced expression of genes characteristic of liver differentiation. This reporter system provides a powerful platform for gene expression and metabolic and functional studies of replicating cells in their in vivo niche.

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DO - 10.1016/j.devcel.2012.08.009

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A Transgenic Mouse Marking Live Replicating Cells Reveals In Vivo Transcriptional Program of Proliferation

Abstract

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