Abstract
The optional group I intron of the mitochondrial 21S rRNA gene of Saccharomyces cerevisiae contains a 235-codon-long open reading frame the translation product of which (the omega transposase) catalyzes the formation of a double-strand break within the intron-minus (omega-) copies of the same gene. Purified omega transposase generates in vitro a 4-base-pair staggered cut with 3' hydroxyl overhangs at the exact position where the intron eventually inserts in the gene. Using randomly mutagenized synthetic oligonucleotides, single-base mutants were produced at 21 positions around the cleavage site. Experiments with these oligonucleotides show that the recognition site extends over an 18-base pair-long sequence within which minimal sequence degeneracy is tolerated. The intron-encoded omega transposase is, therefore, one of the most specific restriction endonucleases known to date.
Dates
| Type | When |
|---|---|
| Created | 19 years, 2 months ago (May 31, 2006, 6:40 a.m.) |
| Deposited | 3 years, 4 months ago (April 13, 2022, 1:01 p.m.) |
| Indexed | 3 weeks, 2 days ago (Aug. 5, 2025, 8:40 a.m.) |
| Issued | 37 years ago (Aug. 1, 1988) |
| Published | 37 years ago (Aug. 1, 1988) |
| Published Online | 37 years ago (Aug. 1, 1988) |
| Published Print | 37 years ago (Aug. 1, 1988) |
@article{Colleaux_1988, title={Recognition and cleavage site of the intron-encoded omega transposase.}, volume={85}, ISSN={1091-6490}, url={http://dx.doi.org/10.1073/pnas.85.16.6022}, DOI={10.1073/pnas.85.16.6022}, number={16}, journal={Proceedings of the National Academy of Sciences}, publisher={Proceedings of the National Academy of Sciences}, author={Colleaux, L and D’Auriol, L and Galibert, F and Dujon, B}, year={1988}, month=aug, pages={6022–6026} }