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eGFP fluorescence observed in Rosa26Cre-GFP/wt embryos

Bright labelling of individualized cells is observed under whole mount confocal microscopy from Rosa26Cre-GFP/wt embryos

Ubiquitous β-gal staining is observed embryos generated from Rosa26Cre-GFP/wt and Rosa26loxP-STOP-loxP-lacZ/oxP-STOP-loxP-lacZ animals

Evolution of the fluorescence observed in newborn Rosa26Cre-GFP/wt mice - day 0.5

Evolution of the fluorescence observed in newborn Rosa26Cre-GFP/wt mice - day 3.5

Evolution of the fluorescence observed in newborn Rosa26Cre-GFP/wt mice - day 7.5

Schematic representation of the Cre and FlpO deleter alleles

Highly-efficient, fluorescent, locus directed Cre and FlpO deleter mice on a pure C57BL/6N genetic background

In order to facilitate the use of the new mutant resources developed in the mouse, we have generated Cre and FlpO deleter mice on a pure inbred C57BL/6N background. The new transgenic constructs were designed to drive either the Cre or FlpO recombinase, fused to a specific fluorescent marker (respectively the eGFP or the eYFP) and were inserted by homologous recombination in the neutral Rosa26 locus. They allow a rapid, cost-effective and efficient identification of the carrier individuals through the co-expression of the fluorescent marker.

The main advantages of these deleters are:

Preservation of a pure genetic background when used to remove specific selection cassette or to induce complete loss-of-function allele (pure inbred C57BL/6N background)
Insertion in the Rosa26 locus
Simplicity of genotype identification (fluorescence evaluation)
High and stable recombination efficiency (up to 100%)
Expression of cre and FlpO in developing oocytes irrespectively of the transmission of the Cre and FlpO transgenes

PubMed
reference

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the FlpO deleter

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the Cre deleter