Publication | Open Access
<i>piggyBac</i>-Based Insertional Mutagenesis and Enhancer Detection as a Tool for Functional Insect Genomics
169
Citations
54
References
2003
Year
GeneticsGenomic MechanismMolecular BiologyFunctional Insect GenomicsMolecular GeneticsGenomicsDrosophila MelanogasterPiggybac ExcisionInsertional MutagenesisDevelopmental GeneticsGene ExpressionFunctional GenomicsBiologyDevelopmental BiologyEnhancer DetectionTransposon MutagenesisNatural SciencesGenetic EngineeringMedicineGenome EditingMutagenesis
Transposon mutagenesis provides a fundamental tool for functional genomics. Here we present a non-species-specific, combined enhancer detection and binary expression system based on the transposable element piggyBac: For the different components of this insertional mutagenesis system, we used widely applicable transposons and distinguishable broad-range transformation markers, which should enable this system to be operational in nonmodel arthropods. In a pilot screen in Drosophila melanogaster, piggyBac mutator elements on the X chromosome were mobilized in males by a Hermes-based jumpstarter element providing piggyBac transposase activity under control of the alpha1-tubulin promoter. As primary reporters in the piggyBac mutator elements, we employed the heterologous transactivators GAL4delta or tTA. To identify larval and adult enhancer detectors, strains carrying UASp-EYFP or TRE-EYFP as secondary reporter elements were used. Tissue-specific enhancer activities were readily observed in the GAL4delta/UASp-based systems, but only rarely in the tTA/TRE system. Novel autosomal insertions were recovered with an average jumping rate of 80%. Of these novel insertions, 3.8% showed homozygous lethality, which was reversible by piggyBac excision. Insertions were found in both coding and noncoding regions of characterized genes and also in noncharacterized and non-P-targeted CG-number genes. This indicates that piggyBac will greatly facilitate the intended saturation mutagenesis in Drosophila.
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