Lineage conversion methodologies meet the reprogramming toolbox

Ignacio Sancho-Martinez; Sung Hee Baek; Juan Carlos Izpisua Belmonte

doi:10.1038/ncb2567

Lineage conversion methodologies meet the reprogramming toolbox

Ignacio Sancho-Martinez, Sung Hee Baek^*, Juan Carlos Izpisua Belmonte

^*Corresponding author for this work

Research output: Contribution to journal › Review article › peer-review

95 Scopus citations

Abstract

Lineage conversion has recently attracted increasing attention as a potential alternative to the directed differentiation of pluripotent cells to obtain cells of a given lineage. Different means allowing for cell identity switch have been reported. Lineage conversion relied initially on the discovery of specific transcription factors generally enriched and characteristic of the target cell, and their forced expression in cells of a different fate. This approach has been successful in various cases, from cells of the hematopoietic systems to neurons and cardiomyocytes. Furthermore, recent reports have suggested the possibility of establishing a general lineage conversion approach bypassing pluripotency. This requires a first phase of epigenetic erasure achieved by short overexpression of the factors used to reprogram cells to a pluripotent state (such as a combination of Sox2, Klf4, c-Myc and Oct4), followed by exposure to specific developmental cues. Here we present these different direct conversion methodologies and discuss their potential as alternatives to using induced pluripotent stem cells and differentiation protocols to generate cell populations of a given fate.

Original language	English (US)
Pages (from-to)	892-899
Number of pages	8
Journal	Nature Cell Biology
Volume	14
Issue number	9
DOIs	https://doi.org/10.1038/ncb2567
State	Published - Sep 2012
Externally published	Yes

ASJC Scopus subject areas

Cell Biology

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10.1038/ncb2567

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title = "Lineage conversion methodologies meet the reprogramming toolbox",

abstract = "Lineage conversion has recently attracted increasing attention as a potential alternative to the directed differentiation of pluripotent cells to obtain cells of a given lineage. Different means allowing for cell identity switch have been reported. Lineage conversion relied initially on the discovery of specific transcription factors generally enriched and characteristic of the target cell, and their forced expression in cells of a different fate. This approach has been successful in various cases, from cells of the hematopoietic systems to neurons and cardiomyocytes. Furthermore, recent reports have suggested the possibility of establishing a general lineage conversion approach bypassing pluripotency. This requires a first phase of epigenetic erasure achieved by short overexpression of the factors used to reprogram cells to a pluripotent state (such as a combination of Sox2, Klf4, c-Myc and Oct4), followed by exposure to specific developmental cues. Here we present these different direct conversion methodologies and discuss their potential as alternatives to using induced pluripotent stem cells and differentiation protocols to generate cell populations of a given fate.",

author = "Ignacio Sancho-Martinez and Baek, {Sung Hee} and {Izpisua Belmonte}, {Juan Carlos}",

note = "Funding Information: We would like to thank Emmanuel Nivet for critical discussions on the manuscript. We also thank May Schwarz and Ilir Dubova for administrative support. We apologize to all our colleagues whose work could not be discussed due to space limitations. S.H.B was supported by Creative Research Initiative Program (Research Center for Chromatin Dynamics, 2009-0081563). Work in the laboratory of JCIB was supported by grants from Fundacion Cellex, the G. Harold and Leila Y. Mathers Charitable Foundation, Sanofi, the California Institute of Regenerative Medicine and MINECO.",

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AU - Izpisua Belmonte, Juan Carlos

N1 - Funding Information: We would like to thank Emmanuel Nivet for critical discussions on the manuscript. We also thank May Schwarz and Ilir Dubova for administrative support. We apologize to all our colleagues whose work could not be discussed due to space limitations. S.H.B was supported by Creative Research Initiative Program (Research Center for Chromatin Dynamics, 2009-0081563). Work in the laboratory of JCIB was supported by grants from Fundacion Cellex, the G. Harold and Leila Y. Mathers Charitable Foundation, Sanofi, the California Institute of Regenerative Medicine and MINECO.

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N2 - Lineage conversion has recently attracted increasing attention as a potential alternative to the directed differentiation of pluripotent cells to obtain cells of a given lineage. Different means allowing for cell identity switch have been reported. Lineage conversion relied initially on the discovery of specific transcription factors generally enriched and characteristic of the target cell, and their forced expression in cells of a different fate. This approach has been successful in various cases, from cells of the hematopoietic systems to neurons and cardiomyocytes. Furthermore, recent reports have suggested the possibility of establishing a general lineage conversion approach bypassing pluripotency. This requires a first phase of epigenetic erasure achieved by short overexpression of the factors used to reprogram cells to a pluripotent state (such as a combination of Sox2, Klf4, c-Myc and Oct4), followed by exposure to specific developmental cues. Here we present these different direct conversion methodologies and discuss their potential as alternatives to using induced pluripotent stem cells and differentiation protocols to generate cell populations of a given fate.

AB - Lineage conversion has recently attracted increasing attention as a potential alternative to the directed differentiation of pluripotent cells to obtain cells of a given lineage. Different means allowing for cell identity switch have been reported. Lineage conversion relied initially on the discovery of specific transcription factors generally enriched and characteristic of the target cell, and their forced expression in cells of a different fate. This approach has been successful in various cases, from cells of the hematopoietic systems to neurons and cardiomyocytes. Furthermore, recent reports have suggested the possibility of establishing a general lineage conversion approach bypassing pluripotency. This requires a first phase of epigenetic erasure achieved by short overexpression of the factors used to reprogram cells to a pluripotent state (such as a combination of Sox2, Klf4, c-Myc and Oct4), followed by exposure to specific developmental cues. Here we present these different direct conversion methodologies and discuss their potential as alternatives to using induced pluripotent stem cells and differentiation protocols to generate cell populations of a given fate.

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Lineage conversion methodologies meet the reprogramming toolbox

Abstract

ASJC Scopus subject areas

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