Abstract
Topological knots can be formed in vitro by incubating covalently closed double stranded DNA and purified topoisomerase II from the yeast Saccharomyces cerevisiae in an ATP-dependent reaction. Knotting production requires a starting enzyme/DNA mass ratio of 1. Analysis of knotted DNA was carried out by using both one- and two-dimensional agarose gel electrophoresis. The knots generated are efficiently untied, and give relaxed DNA rings, by catalytic amounts of topoisomerase II, but not by topoisomerase I. Time course analysis shows the knotting formation over relaxed and supercoiled DNA. When supercoiled DNA was used as a susbtrate, knots appear immediately whereas no transient relaxed rings were observed. The cell-free extract from Xenopus oocytes S-150 cannot assemble nucleosomes on knotted DNA templates as revealed by topological and micrococcal nuclease analysis. Nevertheless, the presence of knotted DNA templates does not inhibit the assembly over the relaxed plasmid. Finally, a pretreatment of knotted DNA with trace amounts of topoisomerase II before the addition of the S-150 yields a canonical minichromosome assembled in vitro. Taking into account these results, I suggest a mechanism of chromatin assembly regulation directed by topoisomerase II.
Highlights
Breaking and rejoining one or two strands
The process finishes after the resealing of the broken duplex, which exits through the first gate depending on ATP hydrolysis
When topoisomerase II is single or double stranded breaks, pro- employed at a catalytic level, both unknotting and relaxing duce different topological forms called topoisomers [1, 2]
Summary
Breaking and rejoining one or two strands. The ATP dependence on the knotting activity is controversial: topoisomerase II knotting of circular duplex DNA, using purified enzyme from Drosophila embryos, is greatly enhanced by ATP [14]. DNA topoisomerases are a kind of enzymes which, by chang- percoiled This ATP-driven reaction depends on the addition of ing the topological structure of the DNA by means of transient stoichiometric amounts of enzyme. When topoisomerase II is single (in class I) or double (in class II) stranded breaks, pro- employed at a catalytic level, both unknotting and relaxing duce different topological forms called topoisomers [1, 2]. These activities over knotted or supercoiled DNA templates are enzymes can knot/unknot, catenate/decatenate, and su- achieved.
Sign-in/Register to view highlights & summary 
Published Version (
Free)
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call