Much of the information about the function of
D. melanogaster genes has come from
P-element mutagenesis. The major drawback of the
P element, however, is its strong bias for insertion into some genes (hotspots) and against insertion into others (coldspots). Within genes, 5′-UTRs are preferential targets. For the successful completion of the Drosophila Genome Disruption Project, the use of transposon vectors other than
P will be necessary. We examined here the suitability of the
Minos element from
Drosophila hydei as a tool for Drosophila genomics. Previous work has shown that
Minos, a member of the
Tc1/mariner family of transposable elements, is active in diverse organisms and cultured cells; it produces stable integrants in the germ line of several insect species, in the mouse, and in human cells. We generated and analyzed 96
Minos integrations into the Drosophila genome and devised an efficient “jump-starting” scheme for production of single insertions. The ratio of insertions into genes
vs. intergenic DNA is consistent with a random distribution. Within genes, there is a statistically significant preference for insertion into introns rather than into exons. About 30% of all insertions were in introns and ~55% of insertions were into or next to genes that have so far not been hit by the
P element. The insertion sites exhibit, in contrast to other transposons, little sequence requirement beyond the TA dinucleotide insertion target. We further demonstrate that induced remobilization of
Minos insertions can delete nearby sequences. Our results suggest that
Minos is a useful tool complementing the
P element for insertional mutagenesis and genomic analysis in Drosophila.
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