Structural highlights
Function
[T2C2_HAEIF] Recognizes the double-stranded sequence GTYRAC and cleaves after Y-3.
Publication Abstract from PubMed
The crystal structure of the HincII restriction endonuclease-DNA complex shows that degenerate specificity for blunt-ended cleavage at GTPyPuAC sequences arises from indirect readout of conformational preferences at the center pyrimidine-purine step. Protein-induced distortion of the DNA is accomplished by intercalation of glutamine side chains into the major groove on either side of the recognition site, generating bending by either tilt or roll at three distinct loci. The intercalated side chains propagate a concerted shift of all six target-site base pairs toward the minor groove, producing an unusual cross-strand purine stacking at the center pyrimidine-purine step. Comparison of the HincII and EcoRV cocrystal structures suggests that sequence-dependent differences in base-stacking free energies are a crucial underlying factor mediating protein recognition by indirect readout.
Sequence selectivity and degeneracy of a restriction endonuclease mediated by DNA intercalation.,Horton NC, Dorner LF, Perona JJ Nat Struct Biol. 2002 Jan;9(1):42-7. PMID:11742344[1]
From MEDLINE®/PubMed®, a database of the U.S. National Library of Medicine.
See Also
References
- ↑ Horton NC, Dorner LF, Perona JJ. Sequence selectivity and degeneracy of a restriction endonuclease mediated by DNA intercalation. Nat Struct Biol. 2002 Jan;9(1):42-7. PMID:11742344 doi:10.1038/nsb741
