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Transcriptional supercoiling boosts topoisomerase II-mediated knotting of intracellular DNA

Valdes, A.
•
Coronel, L.
•
Martinez-Garcia, B.
altro
Roca, J.
2019
  • journal article

Periodico
NUCLEIC ACIDS RESEARCH
Abstract
Recent studies have revealed that the DNA cross-inversion mechanism of topoisomerase II (topo II) not only removes DNA supercoils and DNA replication intertwines, but also produces small amounts of DNA knots within the clusters of nucleosomes that conform to eukaryotic chromatin. Here, we examine how transcriptional supercoiling of intracellular DNA affects the occurrence of these knots. We show that although (-) supercoiling does not change the basal DNA knotting probability, (+) supercoiling of DNA generated in front of the transcribing complexes increases DNA knot formation over 25-fold. The increase of topo II-mediated DNA knotting occurs both upon accumulation of (+) supercoiling in topoisomerase-deficient cells and during normal transcriptional supercoiling of DNA in TOP1 TOP2 cells. We also show that the high knotting probability (Pkn ≥ 0.5) of (+) supercoiled DNA reflects a 5-fold volume compaction of the nucleosomal fibers in vivo. Our findings indicate that topo II-mediated DNA knotting could be inherent to transcriptional supercoiling of DNA and other chromatin condensation processes and establish, therefore, a new crucial role of topoisomerase II in resetting the knotting-unknotting homeostasis of DNA during chromatin dynamics.
DOI
10.1093/nar/gkz491
WOS
WOS:000490556600034
Archivio
http://hdl.handle.net/20.500.11767/111096
info:eu-repo/semantics/altIdentifier/scopus/2-s2.0-85070343284
Diritti
open access
Soggetti
  • Chromatin

  • DNA Topoisomerases, T...

  • DNA Topoisomerases, T...

  • DNA, Fungal

  • DNA, Superhelical

  • Human

  • Nucleosome

  • Saccharomyces cerevis...

  • Saccharomyces cerevis...

  • Transcription, Geneti...

  • Nucleic Acid Conforma...

  • Settore FIS/03 - Fisi...

Scopus© citazioni
11
Data di acquisizione
Jun 14, 2022
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Web of Science© citazioni
16
Data di acquisizione
Mar 8, 2024
Visualizzazioni
2
Data di acquisizione
Apr 19, 2024
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