Literature DB >> 28518103

Structure-function Studies in Mouse Embryonic Stem Cells Using Recombinase-mediated Cassette Exchange.

Tim Pieters1, Lieven Haenebalcke2, Kenneth Bruneel3, Niels Vandamme3, Tino Hochepied2, Jolanda van Hengel4, Dagmar Wirth5, Geert Berx3, Jody J Haigh6, Frans van Roy3, Steven Goossens7.   

Abstract

Gene engineering in mouse embryos or embryonic stem cells (mESCs) allows for the study of the function of a given protein. Proteins are the workhorses of the cell and often consist of multiple functional domains, which can be influenced by posttranslational modifications. The depletion of the entire protein in conditional or constitutive knock-out (KO) mice does not take into account this functional diversity and regulation. An mESC line and a derived mouse model, in which a docking site for FLPe recombination-mediated cassette exchange (RMCE) was inserted within the ROSA26 (R26) locus, was previously reported. Here, we report on a structure-function approach that allows for molecular dissection of the different functionalities of a multidomain protein. To this end, RMCE-compatible mice must be crossed with KO mice and then RMCE-compatible KO mESCs must be isolated. Next, a panel of putative rescue constructs can be introduced into the R26 locus via RMCE targeting. The candidate rescue cDNAs can be easily inserted between RMCE sites of the targeting vector using recombination cloning. Next, KO mESCs are transfected with the targeting vector in combination with an FLPe recombinase expression plasmid. RMCE reactivates the promoter-less neomycin-resistance gene in the ROSA26 docking sites and allows for the selection of the correct targeting event. In this way, high targeting efficiencies close to 100% are obtained, allowing for insertion of multiple putative rescue constructs in a semi-high throughput manner. Finally, a multitude of R26-driven rescue constructs can be tested for their ability to rescue the phenotype that was observed in parental KO mESCs. We present a proof-of-principle structure-function study in p120 catenin (p120ctn) KO mESCs using endoderm differentiation in embryoid bodies (EBs) as the phenotypic readout. This approach enables the identification of important domains, putative downstream pathways, and disease-relevant point mutations that underlie KO phenotypes for a given protein.

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Year:  2017        PMID: 28518103      PMCID: PMC5565114          DOI: 10.3791/55575

Source DB:  PubMed          Journal:  J Vis Exp        ISSN: 1940-087X            Impact factor:   1.355


  29 in total

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Authors:  K L Tucker; Y Wang; J Dausman; R Jaenisch
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Journal:  Expert Opin Drug Discov       Date:  2007-04       Impact factor: 6.098

3.  Metazoan evolution of the armadillo repeat superfamily.

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Authors:  M J Evans; M H Kaufman
Journal:  Nature       Date:  1981-07-09       Impact factor: 49.962

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Journal:  Nat Rev Genet       Date:  2005-06       Impact factor: 53.242

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Journal:  Proc Natl Acad Sci U S A       Date:  2006-11-06       Impact factor: 11.205

7.  Molecular cloning of the human p120ctn catenin gene (CTNND1): expression of multiple alternatively spliced isoforms.

Authors:  A Keirsebilck; S Bonné; K Staes; J van Hengel; F Nollet; A Reynolds; F van Roy
Journal:  Genomics       Date:  1998-06-01       Impact factor: 5.736

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Journal:  Blood       Date:  2016-09-28       Impact factor: 22.113

Review 9.  Functions of p120ctn in development and disease.

Authors:  Tim Pieters; Jolanda van Hengel; Frans van Roy
Journal:  Front Biosci (Landmark Ed)       Date:  2012-01-01

10.  Efficient mouse transgenesis using Gateway-compatible ROSA26 locus targeting vectors and F1 hybrid ES cells.

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Journal:  Nucleic Acids Res       Date:  2009-03-11       Impact factor: 16.971

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Journal:  J Exp Med       Date:  2021-08-18       Impact factor: 14.307

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Journal:  Sci Rep       Date:  2019-07-22       Impact factor: 4.379

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