[Background] Development of the post-genomic age in Dictyostelium will require the existence of rapid and reliable methods to disrupt genes that would allow the analysis of entire gene families and perhaps the possibility to undertake the complete knock-out analysis of all the protein-coding genes present in Dictyostelium genome.
[Results] Here we present an optimized protocol based on the previously described construction of gene disruption vectors by in vitro transposition. Our method allows a rapid selection of the construct by a simple PCR approach and subsequent sequencing. Disruption constructs were amplified by PCR and the products were directly transformed in Dictyostelium cells. The selection of homologous recombination events was also performed by PCR. We have constructed 41 disruption vectors to target genes of unknown function, highly conserved between Dictyostelium and human, but absent from the genomes of S. cerevisiae and S. pombe. 28 genes were successfully disrupted.
[Conclusion] This is the first step towards the understanding of the function of these conserved genes and exemplifies the easiness to undertake large-scale disruption analysis in Dictyostelium.
This work was supported by grant BMC2003-02814 from the Spanish Ministerio de Educación y Ciencia. Sequence data for Dictyostelium were obtained from the Genome Sequencing Centers of the University of Cologne, Germany, the Institute of Molecular Biotechnology, Department of Genome Analysis, Jena, Germany, the Baylor Collage of Medicine in Houston, Texas, and the Sanger Center in Hinxton, Cambridge, UK.
Peer reviewed