Sequence-specific double-strand alkylation and cleavage of DNA mediated by triple-helix formation
Abstract
Attachment of the nondiffusible electrophile N-bromoacetyl to the 5-position of a thymine at the 5'-end of a pyrimidine oligodeoxyribonucleotide affords sequence specific alkylation of a guanine two base pairs to the 5'-side of a local triple-helix complex in >96% yield. N-Bromoacetyloligodeoxyribonucleotides bind adjacent inverted purine tracts on double-helical DNA by triple-helix formation and alkylate single guanine positions on opposite strands at 37-degrees-C (pH 7.4). After depurination, double-strand cleavage at a single site within plasmid DNA (4 kp in size) occurs in greater than 85% yield. The resulting DNA fragments from site-specific alkylation and cleavage can be ligated with DNA fragments generated by restriction endonuclease digestion. This nonenzymatic approach which couples sequence-specific recognition with sequence-dependent cleavage affords double-strand site-specific cleavage in megabase size DNA. A yeast chromosome, 340 000 base pairs in size, was cleaved at a single site in 85-90% yield.
Additional Information
© 1992 American Chemical Society. Received February 12, 1992. We are grateful for generous support from the National Institutes of Health (GM-35724 and HG-00329), a Parsons predoctoral fellowship to T.J.P., and a Howard Hughes Medical Institute predoctoral fellowship to S.A.S.Additional details
- Eprint ID
- 66938
- Resolver ID
- CaltechAUTHORS:20160510-141758758
- NIH
- GM-35724
- NIH
- HG00329
- Ralph M. Parsons Foundation
- Howard Hughes Medical Institute (HHMI)
- Created
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2016-05-19Created from EPrint's datestamp field
- Updated
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2021-11-11Created from EPrint's last_modified field