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The transgeneticist's toolbox:: Novel methods for the targeted modification of eukaryotic genomes

Journal

BIOLOGICAL CHEMISTRY
Volume 381, Issue 9-10, Pages 801-813

Publisher

WALTER DE GRUYTER GMBH
DOI: 10.1515/BC.2000.103

Keywords

cosuppresion; gene transfer; genomic site; recombinase-mediated cassette exchange (RMCE); site-specific recombination; scaffold/matrix attached region (S/MAR)

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Classical techniques for gene transfer into mammalian cells involve tedious screening procedures to identify transgenic clones or animals with the appropriate level and stability of expression or with the correct developmental patterns. These first generation technologies are clearly inadequate for complex genetic strategies by which gene regulation can be studied in its entire complexity While site-specific insertions can principally be achieved by homologous recombination or by adapting the recombination apparatus from phages or yeast, these methods usually lack the required efficiency or they perturb expression patterns by the co-insertion of prokaryotic vector parts. Virtually all of these problems can be overcome by recombinase-mediated cassette exchange (RMCE) techniques which cleanly replace a resident cassette that is flanked by two hetero-specific recombination target sites for a second cassette with the analogous design, presented on a targeting vector. After illustrating the fundamentals of site-specific recombination by selected experiments, the authors (arranged in the chronological order of their contribution) will describe their efforts to develop RMCE into a method of wide applicability. Further developments that have been initiated utilizing the particular potential of the RMCE principle will be outlined.

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