The isolation of strand-specific nicking endonucleases from a randomized SapI expression library

doi:10.1093/nar/gkh674

Nucleic Acids Research 2004 32(12):3661-3671; doi:10.1093/nar/gkh674

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Published online 9 July 2004

The isolation of strand-specific nicking endonucleases from a randomized SapI expression library

James C. Samuelson, Zhenyu Zhu and Shuang-yong Xu^*

New England Biolabs, Inc., 32 Tozer Road, Beverly, MA 01915, USA

^* To whom correspondence should be addressed. Tel: +1 978 998 7287; Fax: +1 978 921 1350; Email: xus{at}neb.com

Received May 18, 2004; Revised and Accepted June 8, 2004

The Type IIS restriction endonuclease SapI recognizes the DNAsequence 5'-GCTCTTC-3' (top strand by convention) and cleavesdownstream (N1/N4) indicating top- and bottom-strand spacing,respectively. The asymmetric nature of DNA recognition presentedthe possibility that one, if not two, nicking variants mightbe created from SapI. To explore this possibility, two parallelselection procedures were designed to isolate either top-strandnicking or bottom-strand nicking variants from a randomly mutatedSapI expression library. These procedures take advantage ofa SapI substrate site designed into the expression plasmid,which allows for in vitro selection of plasmid clones possessinga site-specific and strand-specific nick. A procedure designedto isolate bottom-strand nicking enzymes yielded Nb.SapI-1 containinga critical R420I substitution near the end of the protein. Thetop-strand procedure yielded several SapI variants with a distinctpreference for top-strand cleavage. Mutations present withinthe selected clones were segregated to confirm a top-strandnicking phenotype for single variants Q240R, E250K, G271R orK273R. The nature of the amino acid substitutions found in theselected variants provides evidence that SapI may possess twoactive sites per monomer. This work presents a framework forestablishing the mechanism of SapI DNA cleavage.

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