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NMR Investigation of the Interaction between the RecQ C-Terminal Domain of Human Bloom Syndrome Protein and G-Quadruplex DNA from the Human c-Myc Promoter

Authors
Lee, SungjinLee, Ae-ReeRyu, Kyoung-SeokLee, Joon-HwaPark, Chin-Ju
Issue Date
15-Feb-2019
Publisher
Academic Press
Keywords
G-quadruplex; Bloom syndrome protein; RQC domain; NMR; hydrogen-deuterium exchange
Citation
Journal of Molecular Biology, v.431, no.4, pp 794 - 806
Pages
13
Indexed
SCI
SCIE
SCOPUS
Journal Title
Journal of Molecular Biology
Volume
431
Number
4
Start Page
794
End Page
806
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/9428
DOI
10.1016/j.jmb.2019.01.010
ISSN
0022-2836
1089-8638
Abstract
Bloom syndrome protein (BLM) is one of five human RecQ helicases that participate in DNA metabolism. RecQ C-terminal (RQC) domain is the main DNA binding module of BLM and specifically recognizes G-quadruplex (G4) DNA structures. Because G4 processing by BLM is essential for regulating replication and transcription, both G4 and BLM are considered as potential targets for anticancer therapy. Although several studies have revealed the detailed mechanism of G4 unwinding by BLM, the initial recognition of the G4 structure by the RQC domain is unclear. Here, we investigated the interaction between BLM RQC and the G4 DNA from the c-Myc promoter by NMR spectroscopy. While the signals broadened upon reciprocal titrations, the beta-wing of RQC had significant chemical shift perturbations and experienced millisecond timescale dynamics upon G4 binding. A point mutation in the beta-wing (N1164A) reduced G4 binding affinity. Our hydrogen deuterium exchange data indicate that imino protons of G4 were exchanged with deuterium much faster in the presence of RQC. We suggest that RQC binds to G4 by using the beta-wing as a separating pin to destabilize the G4. By providing information about the RQC G4 interaction, our study yields insight into potential strategies for preventing G4 processing by BLM. (C) 2019 Elsevier Ltd. All rights reserved.
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