Protein–Ligand Dissociation Simulated by Parallel Cascade Selection Molecular Dynamics

Tran, Duy Phuoc; Takemura, Kazuhiro; Kuwata, Kazuo; Kitao, Akio

doi:10.1021/acs.jctc.7b00504

Cited by 40 publications

(112 citation statements)

References 77 publications

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“…This computational cost corresponds to a total simulation time of 40 ns (0.1 ns MD per replica × 400 cycles) and total computational cost of 400 ns (40 ns × 10 replicas). Relatively large variations in the number of PaCS-MD cycles required to cause the dissociation were consistent with the results of the earlier paper 31 , which showed that this number varied in different trials when SASA, Vex, cavity volume (Vcav), and also showed no significant change between the two pressure conditions (Table S1). It is worth mentioning that the TIP3P model 41 however, the amount of shrinkage was equivalent only to the size of one water molecule, which is smaller than the observed cavity and volume fluctuations.…”

Section: Resultssupporting

confidence: 89%

“…This showed that the free energy difference between the bound and unbound states significantly decreases as the pressure increases, which clearly indicates weaker binding affinity at higher pressure. Although only five PaCS-MD trials were conducted, the free energy profiles showed small standard deviations, indicating that free energy converges to a certain value independent of dissociation direction if two molecules are sufficiently separated and interactions between the molecules become negligibly small, as shown in earlier work 29,31 . It should be noted that the free energy converged upon complete detachment of the complex, shown by red triangles in Fig.…”

Section: Pressure Impairs Cheyp-flimn Bindingmentioning

confidence: 71%

“…To observe the dissociation process of the aCheYp and FliMN complex, we used a PaCS-MD simulation 27,28 in which mutually-overlapping conformational trajectories are generated by cycles of parallel short MD simulations and selection of MD snapshots closer to dissociation without applying additional bias to the system. In earlier works, PaCS-MD was successful in generating natural dissociation pathways of tri-N-acetyl-d-glucosamine from hen egg white lysozyme 31 and those of the transactivation domain of the p53 protein from the MDM2 protein 29 . In the present work, the dissociation process of the complex was investigated by a procedure similar to that used in the earlier reports.…”

Section: Dissociation Simulation Of the Cheyp-flimn Complex By Pacs-mdmentioning

confidence: 99%

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High pressure inhibits signaling protein binding to the flagellar motor and bacterial chemotaxis through enhanced hydration

Hata

Nishihara

Nishiyama

et al. 2019

Preprint

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In the chemotaxis of Escherichia coli, the cell's behavioral switch involves binding of the phosphorylated form of the chemotaxis signaling protein CheY (CheYp) to the flagellar motor protein FliM, which induces the motor to rotate clockwise; otherwise, the motor rotates counterclockwise. To investigate high-pressure effects on CheYp-FliM binding at atomic resolution, we conduct molecular dynamics simulations of monomeric CheYp, the N-terminal fragment of the FliM (FliMN) that binds to CheYp, and the complex that forms between those proteins at pressures ranging from 0.1 to 100 MPa. The results show that the active form of monomeric CheYp is maintained even at 100 MPa but high pressure increases the water density in the first hydration shell and can cause conformational change of the C-terminal helix. The dissociation process of the complex is investigated by parallel cascade selection molecular dynamics (PaCS-MD), revealing that high pressure considerably induces water penetration into the complex interface. Pressure dependence of standard binding free energy calculated by the Markov state model indicates that the increase of pressure from 0.1 to 100 MPa weakens the binding by ~ 10 kcal/mol. Using highpressure microscopy, we observed that high hydrostatic pressure reversibly fixes the motor rotation in the counter-clockwise orientation, which supports the notion that high pressure inhibits the binding of CheYp to FliM. We conclude that high pressure induces water penetration into the complex interface, which interferes with CheYp-FliM binding and prevents motor reversal.Recently, a new distributed computing method, parallel cascade selection molecular dynamics (PaCS-MD), has been developed to observe events whose timescales are longer than the standard MD length 27,28 . PaCS-MD can simulate dissociation process of protein complexes, whose time scales range from μs to s, without using artificial forces within a short MD simulation time 29 .Additionally, by integrating the distributed MD trajectories using a Markov state model (MSM) 30 , various quantities characterizing molecular interactions can be calculated, such as binding free energy, association/dissociation rate constants, and residence times 29,31 .

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Section: Resultssupporting

confidence: 89%

Section: Pressure Impairs Cheyp-flimn Bindingmentioning

confidence: 71%

Section: Dissociation Simulation Of the Cheyp-flimn Complex By Pacs-mdmentioning

confidence: 99%

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High pressure inhibits signaling protein binding to the flagellar motor and bacterial chemotaxis through enhanced hydration

Hata

Nishihara

Nishiyama

et al. 2019

Preprint

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“…PaCS-MD can simulate dissociation process of protein complexes, whose time scales range from μs to s, without using artificial forces within a short MD simulation time 29 . Additionally, by integrating the distributed MD trajectories using a Markov state model (MSM) 30 , various quantities characterizing molecular interactions can be calculated, such as binding free energy, association/dissociation rate constants, and residence times 29,31 .In the present study, we investigate the effect of high pressure on the interactions between the chemotaxis signaling protein CheY and the flagellar rotor protein FliM by a combination of MD, PaCS-MD/MSM, and high-pressure microscopy. Switching of the bacterial flagellar motor from counter-clockwise (CCW) to clockwise (CW) is triggered by the binding of the phosphorylated CheY (CheYp) to the N-terminal segment of FliM (FliM N ) 32,33 , which is essential for bacterial chemotaxis 34 .…”

mentioning

confidence: 99%

High pressure inhibits signaling protein binding to the flagellar motor and bacterial chemotaxis through enhanced hydration

Hata

Nishihara

Nishiyama

et al. 2020

Sci Rep

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In Escherichia coli, the binding of the chemotaxis signaling protein CheY to the flagellar motor protein FliM induces reversal of the motor rotation. Using molecular dynamics (MD) simulations and parallel cascade selection MD (PaCS-MD), we show that high pressure increases the water density in the first hydration shell of CheY and considerably induces water penetration into the CheY-FliM interface. PaCS-MD enabled us to observe pressure-induced dissociation of the CheY-FliM complex at atomic resolution. Pressure dependence of binding free energy indicates that the increase of pressure from 0.1 to 100 MPa significantly weakens the binding. Using high-pressure microscopy, we observed that high hydrostatic pressure fixes the motor rotation to the counter-clockwise direction. In conclusion, the application of pressure enhances hydration of the proteins and weakens the binding of CheY to FliM, preventing reversal of the flagellar motor.Pressure significantly affects protein structure, dynamics, and functions 1-4 . Very high pressure (above 500 MPa) induces denaturation of many soluble proteins 5-8 , and therefore the mechanism of pressure denaturation has been relatively well investigated, both theoretically and experimentally 4,9,10 . On the other hand, pressures below 100 MPa, a range that covers the typical biosphere on earth, including the deep sea, does not induce large changes in overall secondary and tertiary structure of most protein molecules 1,3,11,12 , but was found to affect behaviors of biological systems at macroscopic levels [13][14][15] . Pressures of ~ 100 MPa are known to interfere with interactions between biomolecules such as proteins and ligands 1,4,14,16,17 , indicating that the mechanism whereby high pressure perturbs such interactions should be elucidated at the molecular level.Molecular dynamics (MD) simulation has been applied to obtain atomic details of structures and functions of biomolecules, including surrounding water and other molecules 18-20 . MD simulations under high pressures have observed enhanced hydration of proteins 21-23 and penetration of water molecules inside proteins with accompanying conformational changes 24,25 . However, it remains difficult to simulate pressure effects on protein-protein interactions, given that the timescale for observing the pressure effects is often longer than the length of typical MD simulations 4,26 . Recently, a new distributed computing method, parallel cascade selection molecular dynamics (PaCS-MD), has been developed to observe events whose timescales are longer than the standard MD length 27,28 . PaCS-MD can simulate dissociation process of protein complexes, whose time scales range from μs to s, without using artificial forces within a short MD simulation time 29 . Additionally, by integrating the distributed MD trajectories using a Markov state model (MSM) 30 , various quantities characterizing molecular interactions can be calculated, such as binding free energy, association/dissociation rate constants, and residence times 29,31 .In the pr...

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“…However, ligand binding/unbinding processes can be excessively longer than microsecond simulation lengths by using computer hardware available to most scientists [13][14][15] . Various methods such as aMD, metadynamics, weighted ensemble, scale-MD, and PaCS-MD have been used to accelerate sampling the ligand binding/unbinding processes [16][17][18][19][20][21][22][23][24][25][26][27] . In terms of the binding paths found, various algorithms such as umbrella sampling 28,29 and milestoning [30][31][32][33] have been used to estimate kinetic rates and free energy profile.…”

Section: Introductionmentioning

confidence: 99%

Transient states and barriers from molecular simulations and milestoning theory: kinetics in ligand-protein recognition and compound design

Tang

Chen

Chang

2017

Preprint

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Abstract:It is important but unclear how protein-ligand system motions affect free energy profiles, create energy barriers, and lead to slow residence time. We computed residence time (RT) and potential of mean force (PMF) of the dissociations of five structure-kinetic relationship (SKRs) series inhibitors of CDK8/CycC using metadynamics and milestoning theory. By using a novel way to represent the reaction coordinate based on principal component analysis (PCA), we found one-to-one mapping of hydrogen bond (H-bond) breakage and protein domain motions with the energy barriers in the PMFs. This work provides a novel and well-defined approach to study the dissociation kinetics of large and flexible systems.peer-reviewed) is the author/funder. All rights reserved. No reuse allowed without permission.The copyright holder for this preprint (which was not . http://dx.doi.org/10.1101/169607 doi: bioRxiv preprint first posted online Jul. 28, 2017; 2 Binding kinetics has become an important topic in molecular recognition because of the growing awareness of the correlation between kinetics and the drug efficacy.1-4 koff and residence time (RT) are particularly important as determinants of the efficacy of a drug candidate. 5 It is desirable to optimize these properties for drug discovery but, binding kinetics and its determinants in the ligand-receptor structures are not yet fully understood.It is also important to predict these quantities computationally when experimental measurements are not available. Therefore, computational methods, which are able to provide an atomistic description of temporal and spatial dissociation pathway details of ligand-receptor, can be employed to unravel the secret behind the RT and kinetics. The copyright holder for this preprint (which was not . http://dx.doi.org/10.1101/169607 doi: bioRxiv preprint first posted online Jul. 28, 2017; 3 this concern in mind, it is nature to solve this issue by using principal component analysis (PCA), a mathematical method that extracts the major motions from a collection of data. Therefore, it is desirable to take the advantage of PCA to suggest a more straightforward but robust way to define reaction coordinate for calculation using milestoning theory.In this work, we used metadynamics to provide dissociation pathways and computed PMF and RT for five ligands from the SKR compounds series 12 using milestoning theory with a novel way for defining the milestones. The details of methods are included in SI. Using Table 1. The relative ranking distinguishes ligand1 and 2 that have much slower RTs than the rest ligands.Among the ligands, ligand 1 has a RT on the millisecond level which reproduces the experimental value the best. The RTs of other ligands are on the micro-or submicro-level.Interestingly, the computed RT of ligand 2, whose experimental RT is slightly slower, is hundred times faster than ligand 1. We noticed that ligand 2 forms half less H-bonds with CDK8 and requires minor protein motions for it to dissociate compared to ligand 1.Therefore...

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Protein–Ligand Dissociation Simulated by Parallel Cascade Selection Molecular Dynamics

Cited by 40 publications

References 77 publications

High pressure inhibits signaling protein binding to the flagellar motor and bacterial chemotaxis through enhanced hydration

High pressure inhibits signaling protein binding to the flagellar motor and bacterial chemotaxis through enhanced hydration

High pressure inhibits signaling protein binding to the flagellar motor and bacterial chemotaxis through enhanced hydration

Transient states and barriers from molecular simulations and milestoning theory: kinetics in ligand-protein recognition and compound design

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