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Nucleic Acids Research 2005 33(4):e43; doi:10.1093/nar/gni043
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Published online 1 March 2005

© The Author 2005. Published by Oxford University Press. All rights reserved
The online version of this article has been published under an open access model. Users are entitled to use, reproduce, disseminate, or display the open access version of this article for non-commercial purposes provided that: the original authorship is properly and fully attributed; the Journal and Oxford University Press are attributed as the original place of publication with the correct citation details given; if an article is subsequently reproduced or disseminated not in its entirety but only in part or as a derivative work this must be clearly indicated. For commercial re-use, please contact journals.permissions{at}oupjournals.org


Methods Online

An efficient system to establish multiple embryonic stem cell lines carrying an inducible expression unit

Shinji Masui*, Daisuke Shimosato, Yayoi Toyooka, Rika Yagi, Kazue Takahashi and Hitoshi Niwa

Laboratory for Pluripotent Cell Studies, RIKEN Center for Developmental Biology Minatojima-minamimachi 2-2-3, Kobe, Japan

*To whom correspondence should be addressed. Tel: +81 78 306 1930; Fax: +81 78 306 1929; Email: masui{at}cdb.riken.jp

Received December 17, 2004. Revised February 10, 2005. Accepted February 10, 2005.

The growing use of mouse embryonic stem (ES) cells in research emphasizes their importance in studies of molecular mechanisms that maintain pluripotency and direct cellular differentiation. Although systems for regulatable transgene expression are essential for fine analysis of cellular processes at the molecular level, a strategy for the establishment of multiple ES cell lines carrying any of these systems has not yet been described. Here, we report our development of the ROSA-TET system, an effective system for the establishment of multiple ES cell lines carrying a tetracycline (Tc)-regulatable transgene at the Gt (ROSA)26asSor (ROSA26) locus. This system contains a knock-in step of a construct carrying both loxP and its mutant sequences into the ROSA26 locus, followed by a subsequent exchange step that introduces a cDNA to be Tc-regulated to the locus using the recombinase-mediated cassette exchange reaction. Both steps are demonstrated to give desired clones with high efficiency, suggesting that this system can be introduced readily into any ES cell lines, leading to the simultaneous establishment of multiple cell lines carrying different Tc-regulated cDNAs. We believe that use of this system will strongly accelerate molecular biological research using ES cells.


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