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Publication : Deletion and replacement of the mouse adult beta-globin genes by a "plug and socket" repeated targeting strategy.

First Author  Detloff PJ Year  1994
Journal  Mol Cell Biol Volume  14
Issue  10 Pages  6936-43
PubMed ID  7935410 Mgi Jnum  J:20916
Mgi Id  MGI:68976 Doi  10.1128/mcb.14.10.6936
Citation  Detloff PJ, et al. (1994) Deletion and replacement of the mouse adult beta-globin genes by a plug and socket repeated targeting strategy. Mol Cell Biol 14(10):6936-43
abstractText  We describe a two-step strategy to alter any mouse locus repeatedly and efficiently by direct positive selection. Using conventional targeting for the first step, a functional neo gene and a nonfunctional HPRT minigene (the socket) are introduced into the genome of HPRT- embryonic stem (ES) cells close to the chosen locus, in this case the beta-globin locus. For the second step, a targeting construct (the plug) that recombines homologously with the integrated socket and supplies the remaining portion of the HPRT minigene is used; this homologous recombination generates a functional HPRT gene and makes the ES cells hypoxanthine-aminopterin-thymidine resistant. At the same time, the plug provides DNA sequences that recombine homologously with sequences in the target locus and modifies them in the desired manner; the plug is designed so that correctly targeted cells also lose the neo gene and become G418 sensitive. We have used two different plugs to make alterations in the mouse beta-globin locus starting with the same socket-containing ES cell line. One plug deleted 20 kb of DNA containing the two adult beta-globin genes. The other replaced the same region with the human beta-globin gene containing the mutation responsible for sickle cell anemia.
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