Functional Loop Dynamics and Characterization of the Inactive State of the NS2B-NS3 Dengue Protease due to Allosteric Inhibitor Binding

Jonniya, Nisha Amarnath;Kar, Parimal;

Please use this identifier to cite or link to this item: https://dspace.iiti.ac.in/handle/123456789/10876

Title:	Functional Loop Dynamics and Characterization of the Inactive State of the NS2B-NS3 Dengue Protease due to Allosteric Inhibitor Binding
Authors:	Jonniya, Nisha Amarnath;Kar, Parimal;
Keywords:	Complex networks; Molecular dynamics; Proteins; Viruses; Active site; Allosteric inhibitor; Atomistic molecular dynamics simulations; Conformational dynamics; Dengue hemorrhagic fever; Dengue virus; Flavivirus; Loop dynamics; Two-component; Wild types; Locks (fasteners); peptide hydrolase; proteinase inhibitor; serine proteinase; viral protein; chemistry; dengue; Dengue virus; enzyme active site; Flavivirus; human; metabolism; Catalytic Domain; Dengue; Dengue Virus; Flavivirus; Humans; Peptide Hydrolases; Protease Inhibitors; Serine Endopeptidases; Viral Nonstructural Proteins
Issue Date:	2022
Publisher:	American Chemical Society
Citation:	Jonniya, N. A., & Kar, P. (2022). Functional loop dynamics and characterization of the inactive state of the NS2B-NS3 dengue protease due to allosteric inhibitor binding. Journal of Chemical Information and Modeling, 62(16), 3800-3813. doi:10.1021/acs.jcim.2c00461
Abstract:	Dengue virus, a flavivirus that causes dengue shock syndrome and dengue hemorrhagic fever, is currently prevalent worldwide. A two-component protease (NS2B-NS3) is essential for maturation, representing an important target for designing anti-flavivirus drugs. Previously, consideration has been centered on developing active-site inhibitors of NS2B-NS3pro. However, the flat and charged nature of its active site renders difficulties in developing inhibitors, suggesting an alternative strategy for identifying allosteric inhibitors. The allosterically sensitive site of the dengue protease is located near Ala125, between the 120s loop and 150s loop. Using atomistic molecular dynamics simulations, we have explored the protease's conformational dynamics upon binding of an allosteric inhibitor. Furthermore, characterization of the inherent flexible loops (71-75s loop, 120s loop, and 150s loop) is carried out for allosteric-inhibitor-bound wild-type and mutant A125C variants and a comparison is performed with its unbound state to extract the structural changes describing the inactive state of the protease. Our study reveals that compared to the unliganded system, the inhibitor-bound system shows large structural changes in the 120s loop and 150s loop in contrast to the rigid 71-75s loop. The unliganded system shows a closed-state pocket in contrast to the open state for the wild-type complex that locks the protease into the open and inactive-state conformations. However, the mutant complex fluctuates between open and closed states. Also, we tried to see how mutation and binding of an allosteric inhibitor perturb the connectivity in a protein structure network (PSN) at contact levels. Altogether, our study reveals the mechanism of conformational rearrangements of loops at the molecular level, locking the protein in an inactive conformation, which may be useful for developing allosteric inhibitors. © 2022 American Chemical Society. All rights reserved.
URI:	https://doi.org/10.1021/acs.jcim.2c00461 https://dspace.iiti.ac.in/handle/123456789/10876
ISSN:	1549-9596
Type of Material:	Journal Article
Appears in Collections:	Department of Biosciences and Biomedical Engineering

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