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Publication : Generation and characterization of a mouse line carrying Reck-CreERT2 knock-in allele.

First Author  Matsuzaki T Year  2018
Journal  Genesis Volume  56
Issue  4 Pages  e23099
PubMed ID  29508517 Mgi Jnum  J:261688
Mgi Id  MGI:6155322 Doi  10.1002/dvg.23099
Citation  Matsuzaki T, et al. (2018) Generation and characterization of a mouse line carrying Reck-CreERT2 knock-in allele. Genesis 56(4):e23099
abstractText  Reck encodes a membrane-anchored glycoprotein implicated in the regulation of extracellular metalloproteinases, Notch-signaling, and Wnt7-signaling and shown to play critical roles in embryogenesis and tumor suppression. Precise mechanisms of its actions in vivo, however, remain largely unknown. By homologous recombination, we generated a new Reck allele, Reck(CreERT2) (MGI symbol: Reck<tm3.1(cre/ERT2)Noda>). This allele is defective in terms of Reck function but expected to induce loxP-mediated recombination in the cells committed to express Reck. Similarity in the expression patterns of the Reck(CreERT2) transgene and the endogenous Reck gene was confirmed in five tissues. In the adult hippocampus, induction of Reck expression after transient cerebral ischemia could be demonstrated using this allele. These results indicate the utility of this Cre-driver allele in further studies.
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