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A model for the mechanism of precise integration of a microinjected transgene
Authors:Morag McFarlane  Joanna B. Wilson
Affiliation:(1) Robertson Laboratory of Biotechnology, Division of Molecular Genetics, Institute of Biomedical and Lye Sciences, University of Glasgow, 54 Dumbarton Road, G11 6NN Glasgow, UK
Abstract:A unique transgenic mouse line has undergone transgene integration in a very precise fashion. The phenotype displayed by mice of the line followed the predicted inheritance patterns for X-linked transgene insertion which has been confirmed. In order to investigate the mechanism of integration the DNA sequence of the transgene and cellular junctions have been determined. A comparison between wild type and transgenic mutant sequences at the site of insertion revealed that there was no loss or rearrangement of cellular DNA upon integration of the transgene. The cellular sequences at the transgene 5prime and 3prime joins are contiguous in the wild type. The integrant exists as a head to tail tandem dimer with minimal loss of sequence compared with the injected monomer. Analysis of the site of insertion has revealed a 5 bp homology between the 5prime end of the transgene and the cellular sequences. In addition, adjacent to the site of insertion within the cellular sequences, there are several sequence motifs implicated in recombination events including a clustering of strong consensus sites for DNA topoisomerase type I and a region of homology to the human minisatellite consensus core sequence, theEscherichia coli Chi site and the meiotic recombination hotspot within the Ebeta gene of the murine major histocompatibility complex. This clustering of features is likely to have been factorial in the integrity of the insertion event. A model depicting the mechanism of this precise integration is proposed.
Keywords:recombination hotspot  Chi site  minisatellite  topoisomerase I  transgenic mice  integration site
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