Analysis of DNA Looping Interactions by Type II Restriction Enzymes That Require Two Copies of Their Recognition Sites

Overview

Journal J Mol Biol

Publisher Elsevier

Specialties Microbiology
Molecular Biology

Date 2001 Aug 9

PMID 11493005

Citations 16

Authors

S E Milsom

S E Halford

M L Embleton

M D Szczelkun

Affiliations

Soon will be listed here.

Abstract

Before cleaving DNA substrates with two recognition sites, the Cfr10I, NgoMIV, NaeI and SfiI restriction endonucleases bridge the two sites through 3D space, looping out the intervening DNA. To characterise their looping interactions, the enzymes were added to plasmids with two recognition sites interspersed with two res sites for site-specific recombination by Tn21 resolvase, in buffers that contained either EDTA or CaCl2 so as to preclude DNA cleavage by the endonuclease; the extent to which the res sites were sequestered into separate loops was evaluated from the degree of inhibition of resolvase. With Cfr10I, a looped complex was detected in the presence but not in the absence of Ca(2+); it had a lifetime of about 90 seconds. Neither NgoMIV nor NaeI gave looped complexes of sufficient stability to be detected by this method. In contrast, SfiI with Ca(2+) produced a looped complex that survived for more than seven hours, whereas its looping interaction in EDTA lasts for about four minutes. When resolvase was added to a SfiI binding reaction in EDTA followed immediately by CaCl2, the looped DNA was blocked from recombination while the unlooped DNA underwent recombination. By measuring the distribution between looped and unlooped DNA at various SfiI concentrations, and by fitting the data to a model for DNA binding by a tetrameric protein to two sites in cis, an equilibrium constant for the looping interaction was determined. The equilibrium constant was essentially independent of the length of DNA between the SfiI sites.

Citing Articles

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DNA cleavage site selection by Type III restriction enzymes provides evidence for head-on protein collisions following 1D bidirectional motion.

Schwarz F, van Aelst K, Toth J, Seidel R, Szczelkun M Nucleic Acids Res. 2011; 39(18):8042-51.

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Differences between Ca2+ and Mg2+ in DNA binding and release by the SfiI restriction endonuclease: implications for DNA looping.

Bellamy S, Kovacheva Y, Zulkipli I, Halford S Nucleic Acids Res. 2009; 37(16):5443-53.

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Dissecting protein-induced DNA looping dynamics in real time.

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A switch in the mechanism of communication between the two DNA-binding sites in the SfiI restriction endonuclease.

Bellamy S, Milsom S, Kovacheva Y, Sessions R, Halford S J Mol Biol. 2007; 373(5):1169-83.

PMID: 17870087 PMC: 2082129. DOI: 10.1016/j.jmb.2007.08.030.