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Título

Conformational Rearrangements Regulating the DNA Repair Protein APE1

AutorKomaniecka, Nina; Porras, Marta; Cairn, Louis; Santas, Jon Ander; Ferreiro, Nerea; Penelo, Juan Carlos; Bañuelos, Sonia CSIC ORCID
Palabras claveAPE1
BER
DNA repair
Fluorescence
FRET
NPM1
Nucleophosmin
Protein–DNA interaction
Protein structure
Fecha de publicaciónjul-2022
EditorMultidisciplinary Digital Publishing Institute
CitaciónInternational Journal of Molecular Sciences 23(14): 8015 (2022)
ResumenApurinic apyrimidinic endonuclease 1 (APE1) is a key enzyme of the Base Excision Repair (BER) pathway, which primarily manages oxidative lesions of DNA. Once the damaged base is removed, APE1 recognises the resulting abasic site and cleaves the phosphodiester backbone to allow for the correction by subsequent enzymes of the BER machinery. In spite of a wealth of information on APE1 structure and activity, its regulation mechanism still remains to be understood. Human APE1 consists of a globular catalytic domain preceded by a flexible N-terminal extension, which might be involved in the interaction with DNA. Moreover, the binding of the nuclear chaperone nucleophosmin (NPM1) to this region has been reported to impact APE1 catalysis. To evaluate intra- and inter-molecular conformational rearrangements upon DNA binding, incision, and interaction with NPM1, we used Förster resonance energy transfer (FRET), a fluorescence spectroscopy technique sensitive to molecular distances. Our results suggest that the N-terminus approaches the DNA at the downstream side of the abasic site and enables the building of a predictive model of the full-length APE1/DNA complex. Furthermore, the spatial configuration of the N-terminal tail is sensitive to NPM1, which could be related to the regulation of APE1.
Versión del editorhttps://doi.org/10.3390/ijms23148015
URIhttp://hdl.handle.net/10261/296269
DOI10.3390/ijms23148015
ISSN1661-6596
E-ISSN1422-0067
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