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Mutation analysis of the interactions between Mycobacterium tuberculosis caseinolytic protease C1 (ClpC1) and ecumicin

Authors
Jung, In-PilHa, Na-ReumKim, A-RuKim, Sang-HeonYoon, Moon-Young
Issue Date
Aug-2017
Publisher
ELSEVIER
Keywords
Mycobacterium tuberculosis; Site-directed mutagenesis; Molecular docking; Caseinolytic protease C1; Ecumicin
Citation
INTERNATIONAL JOURNAL OF BIOLOGICAL MACROMOLECULES, v.101, pp.348 - 357
Indexed
SCIE
SCOPUS
Journal Title
INTERNATIONAL JOURNAL OF BIOLOGICAL MACROMOLECULES
Volume
101
Start Page
348
End Page
357
URI
https://scholarworks.bwise.kr/hanyang/handle/2021.sw.hanyang/4113
DOI
10.1016/j.ijbiomac.2017.03.126
ISSN
0141-8130
Abstract
Ecumicin is a well-known and potent inhibitor of Mycobacterium tuberculosis. Although the target of ecumicin is caseinolytic protease Cl (ClpC1), the exact mechanism by which ecumicin inhibits ClpC1 has not been identified. To analyze ecumicin's action on ClpC1, site-directed mutagenesis was performed on its binding site. The estimated binding residues within ClpC1 to ecumicin were selected via in silica analysis using molecular docking. The selected residues were mutated by site-directed mutagenesis and the effects on ecumicin binding were analyzed. Mutation at the R83 residue, especially the R83A mutation, in ClpC1 resulted in strong resistance to ATPase activation and inhibition of proteolytic activity. In addition, binding of ecumicin to the R83A ClpC1 N-terminal domain (residues 1-145) was not observed in native gel analysis. These results reveal that the R83 residue plays an important role in the binding of ecumicin. This result provides a basis for the development of an anti-tuberculosis agent based on ecumicin derivatives.
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