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dc.contributor.authorRamesh, Subramani-
dc.contributor.authorSissel, Juul-
dc.contributor.authorAlexandru, Rotaru-
dc.contributor.authorFelicie F, Andersen-
dc.contributor.authorKurt V., Gothelf-
dc.contributor.authorWael, Mamdouh-
dc.contributor.authorFlemming, Besenbacher-
dc.contributor.authorMingdong, Dong-
dc.contributor.authorBirgitta R, Knudsen-
dc.date.accessioned2023-09-16T06:22:08Z-
dc.date.available2023-09-16T06:22:08Z-
dc.date.issued2010-09-09-
dc.identifier.urihttps://doi.org/10.1021/nn101662a-
dc.description.abstractThe biologically and clinically important nuclear enzyme human topoisomerase I relaxes both positively and negatively supercoiled DNA and binds consequently DNA with supercoils of positive or negative sign with a strong preference over relaxed DNA. One scheme to explain this preference relies on the existence of a secondary DNA binding site in the enzyme facilitating binding to DNA nodes characteristic for plectonemic DNA. Here we demonstrate the ability of human topoisomerase I to induce formation of DNA synapses at protein containing nodes or filaments using atomic force microscopy imaging. By means of a two-dimensional (2D) DNA origami platform, we monitor the interactions between a single human topoisomerase I covalently bound to one DNA fragment and a second DNA fragment protruding from the DNA origami. This novel single molecule origami-based detection scheme provides direct evidence for the existence of a secondary DNA interaction site in human topoisomerase I and lends further credence to the theory of two distinct DNA interaction sites in human topoisomerase I, possibly facilitating binding to DNA nodes characteristic for plectonemic supercoils.en_US
dc.language.isoen_USen_US
dc.publisherACS Publicationsen_US
dc.subjectatomic force microscopy (AFM)en_US
dc.subjectfunctionalized 2D origamien_US
dc.subjecthuman topoisomerase Ien_US
dc.subjectsecondary binding siteen_US
dc.subjectsupercoil recognitionen_US
dc.titleA NOVEL SECONDARY DNA BINDING SITE IN HUMAN TOPOISOMERASE I UNRAVELLED BY USING A 2D DNA ORIGAMI PLATFORMen_US
dc.typeArticleen_US
Appears in Collections:International Journals



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