Your search keyword '"Beglov D"' showing total 71 results

1. Use of pessary for cervical insufficiency: a discussion

Author

Marochko, K. V., primary, Parfenova, Ya. A., additional, Artymuk, N. V., additional, Novikova, O. N., additional, and Beglov, D. E., additional

Published

2023

2. Risk factors for extremely preterm and very preterm birth

Author

Beglov, D. E., primary, Artymuk, N. V., additional, Novikova, O. N., additional, Marochko, K. V., additional, and Parfenova, Ya. A., additional

Published

2022

3. Hormonal and immunological features of women with cervical insuffciency

Author

Beglov, D. E., primary, Artymuk, N. V., additional, and Novikova, O. N., additional

Published

2022

4. 89 Computational mapping reveals effect of Hoogsteen breathing on duplex DNA reactivity with formaldehyde

Author

Bohnuud, T., primary, Beglov, D., additional, Ngan, C.H., additional, Zerbe, B., additional, Hall, D.R., additional, Brenke, R., additional, Vajda, S., additional, Frank-Kamenetskii, M.D., additional, and Kozakov, D., additional

Published

2013

5. FTMAP: extended protein mapping with user-selected probe molecules

Author

Ngan, C. H., primary, Bohnuud, T., additional, Mottarella, S. E., additional, Beglov, D., additional, Villar, E. A., additional, Hall, D. R., additional, Kozakov, D., additional, and Vajda, S., additional

Published

2012

6. Solvation Free Energy of Polar and Nonpolar Molecules in Water:  An Extended Interaction Site Integral Equation Theory in Three Dimensions

Author

Du, Q., Beglov, D., and Roux, B.

Abstract

The solvation free energy of polar and nonpolar molecules in water is examined using the statistical mechanical integral equation theory which was recently introduced by Beglov and Roux (J. Phys. Chem. 1997, 101, 7821). The integral equation is an extension of previous theories based on the reference interaction site model (RISM) and the hypernetted chain equation (HNC) to determine the one-dimensional site−site radial pair correlation functions. Since the integral equation provides the average density of the solvent interaction sites in three-dimensional (3d) space around a complex molecular solute of arbitrary shape, it is thereby referred to as the 3d-RISM-HNC integral equation. In the present paper, the accuracy of the 3d-RISM-HNC integral equation is examined by comparing the calculated excess solvation free energy at infinite dilution with experimental data for a set of nonpolar (n-alkanes) and polar (n-alcohols, n-carboxylic acids, and simple amides) molecules. Thermodynamic integration is used to calculate the excess solvation free energy on the basis of the average site densities obtained by the 3d-RISM-HNC equation. Two extensions were made to improve the accuracy of the integral equation. First, the susceptibility of pure liquid water (an input for calculating the excess solvation free energy of molecules in the infinite dilution limit) was obtained by combining information from a molecular dynamics simulation with the RISM-HNC integral equation. Second, empirical water hydrogen and water oxygen bridge functions were introduced and optimized for improving the accuracy of the theory. The calculated solvation free energies are in good accord with experimental data, although further work will be required for quantitatively accurate results. These preliminary results indicate that the 3d-RISM-HNC equation with well-calibrated optimized bridge functions is a promising approach for calculating the hydration free energy of complex molecules.

Published

2000

7. AN ENERGY-WISE COMPUTER SIMULATION OF DNA-ION-WATER INTERACTIONS EXPLAINS THE ABNORMAL STRUCTURE OF POLY[d(A)]:POLY[d(T)].

Author

RIKHIREV, M. E., BEGLOV, D. B., and SKURATOVSKII, I. YA.

Subjects

COMPUTER simulation, DNA, MOLECULAR interactions, WATER analysis, MOLECULAR graphics, MOLECULAR structure

Published

1993

8. An Integral Equation To Describe the Solvation of Polar Molecules in Liquid Water

Author

Beglov, D. and Roux, B.

Abstract

We developed and implemented a statistical mechanical integral equation theory to describe the hydration structure of complex molecules. The theory, which is an extension of the reference interaction site model (RISM) in three dimensions, yields the average density from the solvent interactions sites at all points r around a molecular solute of arbitrary shape. Both solute−solvent electrostatic and van der Waals interactions are fully included, and solvent packing is taken into account. The approach is illustrated by calculating the average oxygen and hydrogen density of liquid water around two molecular solutes:  water and N-methylacetamide. Molecular dynamics simulations are performed to test the results obtained from the integral equation. It is observed that important microscopic structural features of the average water density due to hydrogen bonding are reproduced by the integral equation. The integral equation has a simple formal structure and is easy to implement numerically. It offers a powerful alternative to computer simulations with explicit solvent molecules and to continuum solvent representations for incorporating solvation effects in a wide range of applications.

Published

1997

9. Atomic Radii for Continuum Electrostatics Calculations Based on Molecular Dynamics Free Energy Simulations

Author

Nina, M., Beglov, D., and Roux, B.

Abstract

The electrostatic contribution to the solvation free energy of the 20 naturally occurring amino acids is examined using atomic models. The amino acids are modeled by N-acetyl-X-N‘-methylamide. Free energy perturbation techniques with explicit water molecules are used to evaluate the contribution of solute−solvent electrostatic interactions to the solvation free energies. An analysis based on the radial solvent charge distribution yields a basic rule to determine a set of atomic Born radii defining the dielectric boundary between the solute and the solvent in continuum electrostatic models. Minor adjustments are made to refine the atomic Born radii in order to reproduce quantitatively the electrostatic contribution to the solvation free energy calculated by free energy perturbation techniques. The good agreement of continuum electrostatic and molecular dynamics free energy perturbations suggests that the new set of atomic Born radii may be used as a computationally inexpensive alternative to the microscopic treatment of solvent with explicit water molecules.

Published

1997

10. Continuum Solvation Model: computation of electrostatic forces from numerical solutions to the Poisson-Boltzmann equation

Author

Im, W., Beglov, D., and Roux, B.

Published

1998

11. Buckle of the A-T pair in the Bh-form of poly(dA):poly(dT)

Author

Lipanov, A. A., primary, Beglov, D. B., additional, Alexeev, D. G., additional, and Skuratovsky, I. Ya., additional

Published

1989

12. DNA steric accessibility for water molecules and ions in the case of B-D transition

Author

Beglov, D. B., primary, Lipanov, A. A., additional, and Chuprina, V. P., additional

Published

1989

13. Expanding FTMap for Fragment-Based Identification of Pharmacophore Regions in Ligand Binding Sites.

Author

Khan O, Jones G, Lazou M, Joseph-McCarthy D, Kozakov D, Beglov D, and Vajda S

Subjects

Ligands, Binding Sites, Protein Binding, Pharmacophore, Drug Discovery methods

Abstract

The knowledge of ligand binding hot spots and of the important interactions within such hot spots is crucial for the design of lead compounds in the early stages of structure-based drug discovery. The computational solvent mapping server FTMap can reliably identify binding hot spots as consensus clusters, free energy minima that bind a variety of organic probe molecules. However, in its current implementation, FTMap provides limited information on regions within the hot spots that tend to interact with specific pharmacophoric features of potential ligands. E-FTMap is a new server that expands on the original FTMap protocol. E-FTMap uses 119 organic probes, rather than the 16 in the original FTMap, to exhaustively map binding sites, and identifies pharmacophore features as atomic consensus sites where similar chemical groups bind. We validate E-FTMap against a set of 109 experimentally derived structures of fragment-lead pairs, finding that highly ranked pharmacophore features overlap with the corresponding atoms in both fragments and lead compounds. Additionally, comparisons of mapping results to ensembles of bound ligands reveal that pharmacophores generated with E-FTMap tend to sample highly conserved protein-ligand interactions. E-FTMap is available as a web server at https://eftmap.bu.edu.

Published

2024

14. Uncertainty quantification of receptor ligand binding sites prediction.

Author

Chen N, Yu D, Beglov D, Kon M, and Castrillon-Candas JE

Abstract

Recent advancements in protein docking site prediction have highlighted the limitations of traditional rigid docking algorithms, like PIPER, which often neglect critical stochastic elements such as solvent-induced fluctuations. These oversights can lead to inaccuracies in identifying viable docking sites due to the complexity of high-dimensional, stochastic energy manifolds with low regularity. To address this issue, our research introduces a novel model where the molecular shapes of ligands and receptors are represented using multi-variate Karhunen-Lo `eve (KL) expansions. This method effectively captures the stochastic nature of energy manifolds, allowing for a more accurate representation of molecular interactions.Developed as a plugin for PIPER, our scientific computing software enhances the platform, delivering robust uncertainty measures for the energy manifolds of ranked binding sites. Our results demonstrate that top-ranked binding sites, characterized by lower uncertainty in the stochastic energy manifold, align closely with actual docking sites. Conversely, sites with higher uncertainty correlate with less optimal docking positions. This distinction not only validates our approach but also sets a new standard in protein docking predictions, offering substantial implications for future molecular interaction research and drug development.

Published

2024

15. Impact of AlphaFold on structure prediction of protein complexes: The CASP15-CAPRI experiment.

Author

Lensink MF, Brysbaert G, Raouraoua N, Bates PA, Giulini M, Honorato RV, van Noort C, Teixeira JMC, Bonvin AMJJ, Kong R, Shi H, Lu X, Chang S, Liu J, Guo Z, Chen X, Morehead A, Roy RS, Wu T, Giri N, Quadir F, Chen C, Cheng J, Del Carpio CA, Ichiishi E, Rodriguez-Lumbreras LA, Fernandez-Recio J, Harmalkar A, Chu LS, Canner S, Smanta R, Gray JJ, Li H, Lin P, He J, Tao H, Huang SY, Roel-Touris J, Jimenez-Garcia B, Christoffer CW, Jain AJ, Kagaya Y, Kannan H, Nakamura T, Terashi G, Verburgt JC, Zhang Y, Zhang Z, Fujuta H, Sekijima M, Kihara D, Khan O, Kotelnikov S, Ghani U, Padhorny D, Beglov D, Vajda S, Kozakov D, Negi SS, Ricciardelli T, Barradas-Bautista D, Cao Z, Chawla M, Cavallo L, Oliva R, Yin R, Cheung M, Guest JD, Lee J, Pierce BG, Shor B, Cohen T, Halfon M, Schneidman-Duhovny D, Zhu S, Yin R, Sun Y, Shen Y, Maszota-Zieleniak M, Bojarski KK, Lubecka EA, Marcisz M, Danielsson A, Dziadek L, Gaardlos M, Gieldon A, Liwo A, Samsonov SA, Slusarz R, Zieba K, Sieradzan AK, Czaplewski C, Kobayashi S, Miyakawa Y, Kiyota Y, Takeda-Shitaka M, Olechnovic K, Valancauskas L, Dapkunas J, Venclovas C, Wallner B, Yang L, Hou C, He X, Guo S, Jiang S, Ma X, Duan R, Qui L, Xu X, Zou X, Velankar S, and Wodak SJ

Subjects

Protein Conformation, Protein Binding, Molecular Docking Simulation, Computational Biology methods, Software, Protein Interaction Mapping methods, Algorithms

Abstract

We present the results for CAPRI Round 54, the 5th joint CASP-CAPRI protein assembly prediction challenge. The Round offered 37 targets, including 14 homodimers, 3 homo-trimers, 13 heterodimers including 3 antibody-antigen complexes, and 7 large assemblies. On average ~70 CASP and CAPRI predictor groups, including more than 20 automatics servers, submitted models for each target. A total of 21 941 models submitted by these groups and by 15 CAPRI scorer groups were evaluated using the CAPRI model quality measures and the DockQ score consolidating these measures. The prediction performance was quantified by a weighted score based on the number of models of acceptable quality or higher submitted by each group among their five best models. Results show substantial progress achieved across a significant fraction of the 60+ participating groups. High-quality models were produced for about 40% of the targets compared to 8% two years earlier. This remarkable improvement is due to the wide use of the AlphaFold2 and AlphaFold2-Multimer software and the confidence metrics they provide. Notably, expanded sampling of candidate solutions by manipulating these deep learning inference engines, enriching multiple sequence alignments, or integration of advanced modeling tools, enabled top performing groups to exceed the performance of a standard AlphaFold2-Multimer version used as a yard stick. This notwithstanding, performance remained poor for complexes with antibodies and nanobodies, where evolutionary relationships between the binding partners are lacking, and for complexes featuring conformational flexibility, clearly indicating that the prediction of protein complexes remains a challenging problem., (© 2023 The Authors. Proteins: Structure, Function, and Bioinformatics published by Wiley Periodicals LLC.)

Published

2023

16. The ClusPro AbEMap web server for the prediction of antibody epitopes.

Author

Desta IT, Kotelnikov S, Jones G, Ghani U, Abyzov M, Kholodov Y, Standley DM, Beglov D, Vajda S, and Kozakov D

Subjects

Epitopes, Antigens, Antibodies, Epitope Mapping, Furylfuramide, Proteins chemistry

Abstract

Antibodies play an important role in the immune system by binding to molecules called antigens at their respective epitopes. These interfaces or epitopes are structural entities determined by the interactions between an antibody and an antigen, making them ideal systems to analyze by using docking programs. Since the advent of high-throughput antibody sequencing, the ability to perform epitope mapping using only the sequence of the antibody has become a high priority. ClusPro, a leading protein-protein docking server, together with its template-based modeling version, ClusPro-TBM, have been re-purposed to map epitopes for specific antibody-antigen interactions by using the Antibody Epitope Mapping server (AbEMap). ClusPro-AbEMap offers three different modes for users depending on the information available on the antibody as follows: (i) X-ray structure, (ii) computational/predicted model of the structure or (iii) only the amino acid sequence. The AbEMap server presents a likelihood score for each antigen residue of being part of the epitope. We provide detailed information on the server's capabilities for the three options and discuss how to obtain the best results. In light of the recent introduction of AlphaFold2 (AF2), we also show how one of the modes allows users to use their AF2-generated antibody models as input. The protocol describes the relative advantages of the server compared to other epitope-mapping tools, its limitations and potential areas of improvement. The server may take 45-90 min depending on the size of the proteins., (© 2023. Springer Nature Limited.)

Published

2023

17. High Accuracy Prediction of PROTAC Complex Structures.

Author

Ignatov M, Jindal A, Kotelnikov S, Beglov D, Posternak G, Tang X, Maisonneuve P, Poda G, Batey RA, Sicheri F, Whitty A, Tonge PJ, Vajda S, and Kozakov D

Subjects

Proteolysis, Ubiquitination, Ubiquitin-Protein Ligases metabolism, Proteins metabolism

Abstract

The design of PROteolysis-TArgeting Chimeras (PROTACs) requires bringing an E3 ligase into proximity with a target protein to modulate the concentration of the latter through its ubiquitination and degradation. Here, we present a method for generating high-accuracy structural models of E3 ligase-PROTAC-target protein ternary complexes. The method is dependent on two computational innovations: adding a "silent" convolution term to an efficient protein-protein docking program to eliminate protein poses that do not have acceptable linker conformations and clustering models of multiple PROTACs that use the same E3 ligase and target the same protein. Results show that the largest consensus clusters always have high predictive accuracy and that the ensemble of models can be used to predict the dissociation rate and cooperativity of the ternary complex that relate to the degrading activity of the PROTAC. The method is demonstrated by applications to known PROTAC structures and a blind test involving PROTACs against BRAF mutant V600E. The results confirm that PROTACs function by stabilizing a favorable interaction between the E3 ligase and the target protein but do not necessarily exploit the most energetically favorable geometry for interaction between the proteins.

Published

2023

18. Mapping of antibody epitopes based on docking and homology modeling.

Author

Desta IT, Kotelnikov S, Jones G, Ghani U, Abyzov M, Kholodov Y, Standley DM, Sabitova M, Beglov D, Vajda S, and Kozakov D

Subjects

Epitopes metabolism, Molecular Dynamics Simulation, Proteins chemistry, Protein Binding, Antibodies chemistry, Antigens chemistry

Abstract

Antibodies are key proteins produced by the immune system to target pathogen proteins termed antigens via specific binding to surface regions called epitopes. Given an antigen and the sequence of an antibody the knowledge of the epitope is critical for the discovery and development of antibody based therapeutics. In this work, we present a computational protocol that uses template-based modeling and docking to predict epitope residues. This protocol is implemented in three major steps. First, a template-based modeling approach is used to build the antibody structures. We tested several options, including generation of models using AlphaFold2. Second, each antibody model is docked to the antigen using the fast Fourier transform (FFT) based docking program PIPER. Attention is given to optimally selecting the docking energy parameters depending on the input data. In particular, the van der Waals energy terms are reduced for modeled antibodies relative to x-ray structures. Finally, ranking of antigen surface residues is produced. The ranking relies on the docking results, that is, how often the residue appears in the docking poses' interface, and also on the energy favorability of the docking pose in question. The method, called PIPER-Map, has been tested on a widely used antibody-antigen docking benchmark. The results show that PIPER-Map improves upon the existing epitope prediction methods. An interesting observation is that epitope prediction accuracy starting from antibody sequence alone does not significantly differ from that of starting from unbound (i.e., separately crystallized) antibody structure., (© 2022 Wiley Periodicals LLC.)

Published

2023

19. Benchmark Sets for Binding Hot Spot Identification in Fragment-Based Ligand Discovery.

Author

Wakefield AE, Yueh C, Beglov D, Castilho MS, Kozakov D, Keserű GM, Whitty A, and Vajda S

Subjects

Binding Sites, Ligands, Protein Binding, Benchmarking, Proteins metabolism

Abstract

Binding hot spots are regions of proteins that, due to their potentially high contribution to the binding free energy, have high propensity to bind small molecules. We present benchmark sets for testing computational methods for the identification of binding hot spots with emphasis on fragment-based ligand discovery. Each protein structure in the set binds a fragment, which is extended into larger ligands in other structures without substantial change in its binding mode. Structures of the same proteins without any bound ligand are also collected to form an unbound benchmark. We also discuss a set developed by Astex Pharmaceuticals for the validation of hot and warm spots for fragment binding. The set is based on the assumption that a fragment that occurs in diverse ligands in the same subpocket identifies a binding hot spot. Since this set includes only ligand-bound proteins, we added a set with unbound structures. All four sets were tested using FTMap, a computational analogue of fragment screening experiments to form a baseline for testing other prediction methods, and differences among the sets are discussed.

Published

2020

20. ClusPro in rounds 38 to 45 of CAPRI: Toward combining template-based methods with free docking.

Author

Padhorny D, Porter KA, Ignatov M, Alekseenko A, Beglov D, Kotelnikov S, Ashizawa R, Desta I, Alam N, Sun Z, Brini E, Dill K, Schueler-Furman O, Vajda S, and Kozakov D

Subjects

Amino Acid Sequence, Benchmarking, Binding Sites, Humans, Ligands, Peptides metabolism, Protein Binding, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Interaction Domains and Motifs, Protein Interaction Mapping, Protein Multimerization, Proteins metabolism, Research Design, Structural Homology, Protein, Thermodynamics, Molecular Docking Simulation, Peptides chemistry, Proteins chemistry, Software

Abstract

Targets in the protein docking experiment CAPRI (Critical Assessment of Predicted Interactions) generally present new challenges and contribute to new developments in methodology. In rounds 38 to 45 of CAPRI, most targets could be effectively predicted using template-based methods. However, the server ClusPro required structures rather than sequences as input, and hence we had to generate and dock homology models. The available templates also provided distance restraints that were directly used as input to the server. We show here that such an approach has some advantages. Free docking with template-based restraints using ClusPro reproduced some interfaces suggested by weak or ambiguous templates while not reproducing others, resulting in correct server predicted models. More recently we developed the fully automated ClusPro TBM server that performs template-based modeling and thus can use sequences rather than structures of component proteins as input. The performance of the server, freely available for noncommercial use at https://tbm.cluspro.org, is demonstrated by predicting the protein-protein targets of rounds 38 to 45 of CAPRI., (© 2020 Wiley Periodicals, Inc.)

Published

2020

21. Structure-Based Analysis of Cryptic-Site Opening.

Author

Sun Z, Wakefield AE, Kolossvary I, Beglov D, and Vajda S

Subjects

Binding Sites, Crystallography, X-Ray, Ligands, Models, Molecular, Molecular Dynamics Simulation, Protein Binding, Protein Conformation, Proteins chemistry, Proteins metabolism

Abstract

Many proteins in their unbound structures have cryptic sites that are not appropriately sized for drug binding. We consider here 32 proteins from the recently published CryptoSite set with validated cryptic sites, and study whether the sites remain cryptic in all available X-ray structures of the proteins solved without any ligand bound near the sites. It was shown that only few of these proteins have binding pockets that never form without ligand binding. Sites that are cryptic in some structures but spontaneously form in others are also rare. In most proteins the forming of pockets is affected by mutations or ligand binding at locations far from the cryptic site. To further explore these mechanisms, we applied adiabatic biased molecular dynamics simulations to guide the proteins from their ligand-free structures to ligand-bound conformations, and studied the distribution of druggability scores of the pockets located at the cryptic sites., Competing Interests: Declaration of Interests The current affiliation of I.K. is Silicon Therapeutics, Boston, MA, 02215, USA. D.B. is an employee and shareholder of Acpharis Inc., Holliston, MA 01746, USA, in addition to his affiliation with Boston University. S.V. is a shareholder of Acpharis Inc. The other authors declare no competing interests., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2020

22. Template-based modeling by ClusPro in CASP13 and the potential for using co-evolutionary information in docking.

Author

Porter KA, Padhorny D, Desta I, Ignatov M, Beglov D, Kotelnikov S, Sun Z, Alekseenko A, Anishchenko I, Cong Q, Ovchinnikov S, Baker D, Vajda S, and Kozakov D

Subjects

Algorithms, Binding Sites genetics, Databases, Protein, Humans, Molecular Docking Simulation, Molecular Dynamics Simulation, Protein Interaction Mapping, Proteins chemistry, Proteins genetics, Structural Homology, Protein, Computational Biology, Protein Conformation, Proteins ultrastructure, Software

Abstract

As a participant in the joint CASP13-CAPRI46 assessment, the ClusPro server debuted its new template-based modeling functionality. The addition of this feature, called ClusPro TBM, was motivated by the previous CASP-CAPRI assessments and by the proven ability of template-based methods to produce higher-quality models, provided templates are available. In prior assessments, ClusPro submissions consisted of models that were produced via free docking of pre-generated homology models. This method was successful in terms of the number of acceptable predictions across targets; however, analysis of results showed that purely template-based methods produced a substantially higher number of medium-quality models for targets for which there were good templates available. The addition of template-based modeling has expanded ClusPro's ability to produce higher accuracy predictions, primarily for homomeric but also for some heteromeric targets. Here we review the newest additions to the ClusPro web server and discuss examples of CASP-CAPRI targets that continue to drive further development. We also describe ongoing work not yet implemented in the server. This includes the development of methods to improve template-based models and the use of co-evolutionary information for data-assisted free docking., (© 2019 Wiley Periodicals, Inc. The World Health Organization retains copyright and all other rights in the manuscript of this article as submitted for publication.)

Published

2019

23. Blind prediction of homo- and hetero-protein complexes: The CASP13-CAPRI experiment.

Author

Lensink MF, Brysbaert G, Nadzirin N, Velankar S, Chaleil RAG, Gerguri T, Bates PA, Laine E, Carbone A, Grudinin S, Kong R, Liu RR, Xu XM, Shi H, Chang S, Eisenstein M, Karczynska A, Czaplewski C, Lubecka E, Lipska A, Krupa P, Mozolewska M, Golon Ł, Samsonov S, Liwo A, Crivelli S, Pagès G, Karasikov M, Kadukova M, Yan Y, Huang SY, Rosell M, Rodríguez-Lumbreras LA, Romero-Durana M, Díaz-Bueno L, Fernandez-Recio J, Christoffer C, Terashi G, Shin WH, Aderinwale T, Maddhuri Venkata Subraman SR, Kihara D, Kozakov D, Vajda S, Porter K, Padhorny D, Desta I, Beglov D, Ignatov M, Kotelnikov S, Moal IH, Ritchie DW, Chauvot de Beauchêne I, Maigret B, Devignes MD, Ruiz Echartea ME, Barradas-Bautista D, Cao Z, Cavallo L, Oliva R, Cao Y, Shen Y, Baek M, Park T, Woo H, Seok C, Braitbard M, Bitton L, Scheidman-Duhovny D, Dapkūnas J, Olechnovič K, Venclovas Č, Kundrotas PJ, Belkin S, Chakravarty D, Badal VD, Vakser IA, Vreven T, Vangaveti S, Borrman T, Weng Z, Guest JD, Gowthaman R, Pierce BG, Xu X, Duan R, Qiu L, Hou J, Ryan Merideth B, Ma Z, Cheng J, Zou X, Koukos PI, Roel-Touris J, Ambrosetti F, Geng C, Schaarschmidt J, Trellet ME, Melquiond ASJ, Xue L, Jiménez-García B, van Noort CW, Honorato RV, Bonvin AMJJ, and Wodak SJ

Subjects

Algorithms, Binding Sites genetics, Databases, Protein, Models, Molecular, Protein Binding genetics, Protein Interaction Mapping, Proteins chemistry, Proteins genetics, Structural Homology, Protein, Computational Biology, Protein Conformation, Proteins ultrastructure, Software

Abstract

We present the results for CAPRI Round 46, the third joint CASP-CAPRI protein assembly prediction challenge. The Round comprised a total of 20 targets including 14 homo-oligomers and 6 heterocomplexes. Eight of the homo-oligomer targets and one heterodimer comprised proteins that could be readily modeled using templates from the Protein Data Bank, often available for the full assembly. The remaining 11 targets comprised 5 homodimers, 3 heterodimers, and two higher-order assemblies. These were more difficult to model, as their prediction mainly involved "ab-initio" docking of subunit models derived from distantly related templates. A total of ~30 CAPRI groups, including 9 automatic servers, submitted on average ~2000 models per target. About 17 groups participated in the CAPRI scoring rounds, offered for most targets, submitting ~170 models per target. The prediction performance, measured by the fraction of models of acceptable quality or higher submitted across all predictors groups, was very good to excellent for the nine easy targets. Poorer performance was achieved by predictors for the 11 difficult targets, with medium and high quality models submitted for only 3 of these targets. A similar performance "gap" was displayed by scorer groups, highlighting yet again the unmet challenge of modeling the conformational changes of the protein components that occur upon binding or that must be accounted for in template-based modeling. Our analysis also indicates that residues in binding interfaces were less well predicted in this set of targets than in previous Rounds, providing useful insights for directions of future improvements., (© 2019 Wiley Periodicals, Inc.)

Published

2019

24. Amidino-Rocaglates: A Potent Class of eIF4A Inhibitors.

Author

Chu J, Zhang W, Cencic R, Devine WG, Beglov D, Henkel T, Brown LE, Vajda S, Porco JA Jr, and Pelletier J

Subjects

Animals, Antineoplastic Agents metabolism, Antineoplastic Agents pharmacology, Antineoplastic Agents therapeutic use, Benzofurans metabolism, Cell Survival drug effects, DEAD-box RNA Helicases chemistry, DEAD-box RNA Helicases genetics, DEAD-box RNA Helicases metabolism, Drug Design, Eukaryotic Initiation Factor-4A genetics, Eukaryotic Initiation Factor-4A metabolism, Female, Humans, Lymphoma drug therapy, Lymphoma metabolism, Lymphoma pathology, Mice, Mice, Inbred C57BL, Protein Biosynthesis drug effects, RNA chemistry, RNA metabolism, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Ribosomes metabolism, Structure-Activity Relationship, Amidines chemistry, Antineoplastic Agents chemistry, Benzofurans chemistry, Eukaryotic Initiation Factor-4A antagonists & inhibitors

Abstract

Rocaglates share a common cyclopenta[b]benzofuran core that inhibits eukaryotic translation initiation by modifying the behavior of the RNA helicase, eIF4A. Working as interfacial inhibitors, rocaglates stabilize the association between eIF4A and RNA, which can lead to the formation of steric barriers that block initiating ribosomes. There is significant interest in the development and expansion of rocaglate derivatives, as several members of this family have been shown to possess potent anti-neoplastic activity in vitro and in vivo. To further our understanding of rocaglate diversity and drug design, herein we explore the RNA clamping activity of >200 unique rocaglate derivatives. Through this, we report on the identification and characterization of a potent class of synthetic rocaglates called amidino-rocaglates. These compounds are among the most potent rocaglates documented to date and, taken together, this work offers important information that will guide the future design of rocaglates with improved biological properties., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019

25. Discovery of Macrocyclic Inhibitors of Apurinic/Apyrimidinic Endonuclease 1.

Author

Trilles R, Beglov D, Chen Q, He H, Wireman R, Reed A, Chennamadhavuni S, Panek JS, Brown LE, Vajda S, Porco JA Jr, Kelley MR, and Georgiadis MM

Subjects

Catalytic Domain, Cell Line, Tumor, DNA Damage drug effects, DNA-(Apurinic or Apyrimidinic Site) Lyase chemistry, DNA-(Apurinic or Apyrimidinic Site) Lyase metabolism, Drug Discovery, Enzyme Inhibitors chemical synthesis, Enzyme Inhibitors metabolism, Humans, Lactams, Macrocyclic chemical synthesis, Lactams, Macrocyclic metabolism, Lactones chemical synthesis, Lactones metabolism, Molecular Docking Simulation, Molecular Structure, Protein Binding, Small Molecule Libraries chemical synthesis, Small Molecule Libraries metabolism, Small Molecule Libraries pharmacology, Structure-Activity Relationship, DNA-(Apurinic or Apyrimidinic Site) Lyase antagonists & inhibitors, Enzyme Inhibitors pharmacology, Lactams, Macrocyclic pharmacology, Lactones pharmacology

Abstract

Apurinic/apyrimidinic endonuclease 1 (APE1) is an essential base excision repair enzyme that is upregulated in a number of cancers, contributes to resistance of tumors treated with DNA-alkylating or -oxidizing agents, and has recently been identified as an important therapeutic target. In this work, we identified hot spots for binding of small organic molecules experimentally in high resolution crystal structures of APE1 and computationally through the use of FTMAP analysis ( http://ftmap.bu.edu/ ). Guided by these hot spots, a library of drug-like macrocycles was docked and then screened for inhibition of APE1 endonuclease activity. In an iterative process, hot-spot-guided docking, characterization of inhibition of APE1 endonuclease, and cytotoxicity of cancer cells were used to design next generation macrocycles. To assess target selectivity in cells, selected macrocycles were analyzed for modulation of DNA damage. Taken together, our studies suggest that macrocycles represent a promising class of compounds for inhibition of APE1 in cancer cells.

Published

2019

26. Cryptic binding sites on proteins: definition, detection, and druggability.

Author

Vajda S, Beglov D, Wakefield AE, Egbert M, and Whitty A

Subjects

Animals, Computer-Aided Design, Humans, Ligands, Machine Learning, Molecular Docking Simulation, Molecular Dynamics Simulation, Proteins metabolism, Binding Sites drug effects, Drug Discovery methods, Proteins chemistry

Abstract

Many proteins in their unbound structures lack surface pockets appropriately sized for drug binding. Hence, a variety of experimental and computational tools have been developed for the identification of cryptic sites that are not evident in the unbound protein but form upon ligand binding, and can provide tractable drug target sites. The goal of this review is to discuss the definition, detection, and druggability of such sites, and their potential value for drug discovery. Novel methods based on molecular dynamics simulations are particularly promising and yield a large number of transient pockets, but it has been shown that only a minority of such sites are generally capable of binding ligands with substantial affinity. Based on recent studies, current methodology can be improved by combining molecular dynamics with fragment docking and machine learning approaches., (Copyright © 2018 Elsevier Ltd. All rights reserved.)

Published

2018

27. Exploring the structural origins of cryptic sites on proteins.

Author

Beglov D, Hall DR, Wakefield AE, Luo L, Allen KN, Kozakov D, Whitty A, and Vajda S

Subjects

Binding Sites, Ligands, Molecular Dynamics Simulation, Protein Binding, Protein Conformation, Proteins chemistry

Abstract

Molecular dynamics (MD) simulations of proteins reveal the existence of many transient surface pockets; however, the factors determining what small subset of these represent druggable or functionally relevant ligand binding sites, called "cryptic sites," are not understood. Here, we examine multiple X-ray structures for a set of proteins with validated cryptic sites, using the computational hot spot identification tool FTMap. The results show that cryptic sites in ligand-free structures generally have a strong binding energy hot spot very close by. As expected, regions around cryptic sites exhibit above-average flexibility, and close to 50% of the proteins studied here have unbound structures that could accommodate the ligand without clashes. Nevertheless, the strong hot spot neighboring each cryptic site is almost always exploited by the bound ligand, suggesting that binding may frequently involve an induced fit component. We additionally evaluated the structural basis for cryptic site formation, by comparing unbound to bound structures. Cryptic sites are most frequently occluded in the unbound structure by intrusion of loops (22.5%), side chains (19.4%), or in some cases entire helices (5.4%), but motions that create sites that are too open can also eliminate pockets (19.4%). The flexibility of cryptic sites frequently leads to missing side chains or loops (12%) that are particularly evident in low resolution crystal structures. An interesting observation is that cryptic sites formed solely by the movement of side chains, or of backbone segments with fewer than five residues, result only in low affinity binding sites with limited use for drug discovery., Competing Interests: The authors declare no conflict of interest.

Published

2018

28. Protein-ligand docking using FFT based sampling: D3R case study.

Author

Padhorny D, Hall DR, Mirzaei H, Mamonov AB, Moghadasi M, Alekseenko A, Beglov D, and Kozakov D

Subjects

17-alpha-Hydroxyprogesterone chemistry, Binding Sites, Calcifediol chemistry, Computer-Aided Design, Drug Design, Humans, Ligands, Monte Carlo Method, Protein Binding, Proteins chemistry, 17-alpha-Hydroxyprogesterone pharmacology, Calcifediol pharmacology, Fourier Analysis, Molecular Docking Simulation, Proteins metabolism

Abstract

Fast Fourier transform (FFT) based approaches have been successful in application to modeling of relatively rigid protein-protein complexes. Recently, we have been able to adapt the FFT methodology to treatment of flexible protein-peptide interactions. Here, we report our latest attempt to expand the capabilities of the FFT approach to treatment of flexible protein-ligand interactions in application to the D3R PL-2016-1 challenge. Based on the D3R assessment, our FFT approach in conjunction with Monte Carlo minimization off-grid refinement was among the top performing methods in the challenge. The potential advantage of our method is its ability to globally sample the protein-ligand interaction landscape, which will be explored in further applications.

Published

2018

29. ClusPro PeptiDock: efficient global docking of peptide recognition motifs using FFT.

Author

Porter KA, Xia B, Beglov D, Bohnuud T, Alam N, Schueler-Furman O, and Kozakov D

Subjects

Algorithms, Cyclins chemistry, Cyclins metabolism, Databases, Protein, Fourier Analysis, Peptides chemistry, Peptides metabolism, Computational Biology methods, Molecular Docking Simulation methods, Protein Conformation, Protein Interaction Domains and Motifs, Software

Abstract

Summary: We present an approach for the efficient docking of peptide motifs to their free receptor structures. Using a motif based search, we can retrieve structural fragments from the Protein Data Bank (PDB) that are very similar to the peptide's final, bound conformation. We use a Fast Fourier Transform (FFT) based docking method to quickly perform global rigid body docking of these fragments to the receptor. According to CAPRI peptide docking criteria, an acceptable conformation can often be found among the top-ranking predictions., Availability and Implementation: The method is available as part of the protein-protein docking server ClusPro at https://peptidock.cluspro.org/nousername.php., Contact: midas@laufercenter.org or oraf@ekmd.huji.ac.il., Supplementary Information: Supplementary data are available at Bioinformatics online., (© The Author (2017). Published by Oxford University Press. All rights reserved. For Permissions, please email: journals.permissions@oup.com)

Published

2017

30. New additions to the ClusPro server motivated by CAPRI.

Author

Vajda S, Yueh C, Beglov D, Bohnuud T, Mottarella SE, Xia B, Hall DR, and Kozakov D

Subjects

Benchmarking, Binding Sites, Cluster Analysis, Crystallography, X-Ray, Databases, Protein, Internet, Protein Binding, Protein Conformation, Protein Interaction Mapping, Protein Multimerization, Research Design, Structural Homology, Protein, Thermodynamics, Algorithms, Computational Biology methods, Molecular Docking Simulation methods, Proteins chemistry, Software, Water chemistry

Abstract

The heavily used protein-protein docking server ClusPro performs three computational steps as follows: (1) rigid body docking, (2) RMSD based clustering of the 1000 lowest energy structures, and (3) the removal of steric clashes by energy minimization. In response to challenges encountered in recent CAPRI targets, we added three new options to ClusPro. These are (1) accounting for small angle X-ray scattering data in docking; (2) considering pairwise interaction data as restraints; and (3) enabling discrimination between biological and crystallographic dimers. In addition, we have developed an extremely fast docking algorithm based on 5D rotational manifold FFT, and an algorithm for docking flexible peptides that include known sequence motifs. We feel that these developments will further improve the utility of ClusPro. However, CAPRI emphasized several shortcomings of the current server, including the problem of selecting the right energy parameters among the five options provided, and the problem of selecting the best models among the 10 generated for each parameter set. In addition, results convinced us that further development is needed for docking homology models. Finally, we discuss the difficulties we have encountered when attempting to develop a refinement algorithm that would be computationally efficient enough for inclusion in a heavily used server. Proteins 2017; 85:435-444. © 2016 Wiley Periodicals, Inc., (© 2016 Wiley Periodicals, Inc.)

Published

2017

31. The ClusPro web server for protein-protein docking.

Author

Kozakov D, Hall DR, Xia B, Porter KA, Padhorny D, Yueh C, Beglov D, and Vajda S

Subjects

Algorithms, Databases, Protein, Heparin metabolism, Protein Multimerization, Protein Structure, Quaternary, Thermodynamics, Computational Biology methods, Internet, Protein Interaction Mapping methods

Abstract

The ClusPro server (https://cluspro.org) is a widely used tool for protein-protein docking. The server provides a simple home page for basic use, requiring only two files in Protein Data Bank (PDB) format. However, ClusPro also offers a number of advanced options to modify the search; these include the removal of unstructured protein regions, application of attraction or repulsion, accounting for pairwise distance restraints, construction of homo-multimers, consideration of small-angle X-ray scattering (SAXS) data, and location of heparin-binding sites. Six different energy functions can be used, depending on the type of protein. Docking with each energy parameter set results in ten models defined by centers of highly populated clusters of low-energy docked structures. This protocol describes the use of the various options, the construction of auxiliary restraints files, the selection of the energy parameters, and the analysis of the results. Although the server is heavily used, runs are generally completed in <4 h.

Published

2017

32. Prediction of homoprotein and heteroprotein complexes by protein docking and template-based modeling: A CASP-CAPRI experiment.

Author

Lensink MF, Velankar S, Kryshtafovych A, Huang SY, Schneidman-Duhovny D, Sali A, Segura J, Fernandez-Fuentes N, Viswanath S, Elber R, Grudinin S, Popov P, Neveu E, Lee H, Baek M, Park S, Heo L, Rie Lee G, Seok C, Qin S, Zhou HX, Ritchie DW, Maigret B, Devignes MD, Ghoorah A, Torchala M, Chaleil RA, Bates PA, Ben-Zeev E, Eisenstein M, Negi SS, Weng Z, Vreven T, Pierce BG, Borrman TM, Yu J, Ochsenbein F, Guerois R, Vangone A, Rodrigues JP, van Zundert G, Nellen M, Xue L, Karaca E, Melquiond AS, Visscher K, Kastritis PL, Bonvin AM, Xu X, Qiu L, Yan C, Li J, Ma Z, Cheng J, Zou X, Shen Y, Peterson LX, Kim HR, Roy A, Han X, Esquivel-Rodriguez J, Kihara D, Yu X, Bruce NJ, Fuller JC, Wade RC, Anishchenko I, Kundrotas PJ, Vakser IA, Imai K, Yamada K, Oda T, Nakamura T, Tomii K, Pallara C, Romero-Durana M, Jiménez-García B, Moal IH, Férnandez-Recio J, Joung JY, Kim JY, Joo K, Lee J, Kozakov D, Vajda S, Mottarella S, Hall DR, Beglov D, Mamonov A, Xia B, Bohnuud T, Del Carpio CA, Ichiishi E, Marze N, Kuroda D, Roy Burman SS, Gray JJ, Chermak E, Cavallo L, Oliva R, Tovchigrechko A, and Wodak SJ

Subjects

Algorithms, Amino Acid Motifs, Bacteria chemistry, Binding Sites, Computational Biology methods, Humans, International Cooperation, Internet, Protein Binding, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Folding, Protein Interaction Domains and Motifs, Protein Multimerization, Protein Structure, Tertiary, Sequence Homology, Amino Acid, Thermodynamics, Computational Biology statistics & numerical data, Models, Statistical, Molecular Docking Simulation, Molecular Dynamics Simulation, Proteins chemistry, Software

Abstract

We present the results for CAPRI Round 30, the first joint CASP-CAPRI experiment, which brought together experts from the protein structure prediction and protein-protein docking communities. The Round comprised 25 targets from amongst those submitted for the CASP11 prediction experiment of 2014. The targets included mostly homodimers, a few homotetramers, and two heterodimers, and comprised protein chains that could readily be modeled using templates from the Protein Data Bank. On average 24 CAPRI groups and 7 CASP groups submitted docking predictions for each target, and 12 CAPRI groups per target participated in the CAPRI scoring experiment. In total more than 9500 models were assessed against the 3D structures of the corresponding target complexes. Results show that the prediction of homodimer assemblies by homology modeling techniques and docking calculations is quite successful for targets featuring large enough subunit interfaces to represent stable associations. Targets with ambiguous or inaccurate oligomeric state assignments, often featuring crystal contact-sized interfaces, represented a confounding factor. For those, a much poorer prediction performance was achieved, while nonetheless often providing helpful clues on the correct oligomeric state of the protein. The prediction performance was very poor for genuine tetrameric targets, where the inaccuracy of the homology-built subunit models and the smaller pair-wise interfaces severely limited the ability to derive the correct assembly mode. Our analysis also shows that docking procedures tend to perform better than standard homology modeling techniques and that highly accurate models of the protein components are not always required to identify their association modes with acceptable accuracy. Proteins 2016; 84(Suppl 1):323-348. © 2016 Wiley Periodicals, Inc., (© 2016 Wiley Periodicals, Inc.)

Published

2016

33. Quantifying the chameleonic properties of macrocycles and other high-molecular-weight drugs.

Author

Whitty A, Zhong M, Viarengo L, Beglov D, Hall DR, and Vajda S

Subjects

Drug Design, Humans, Macrocyclic Compounds pharmacology, Models, Molecular, Molecular Weight, Macrocyclic Compounds chemistry

Abstract

Key to the pharmaceutical utility of certain macrocyclic drugs is a 'chameleonic' ability to change their conformation to expose polar groups in aqueous solution, but bury them when traversing lipid membranes. Based on analysis of the structures of 20 macrocyclic compounds that are approved oral drugs, we propose that good solubility requires a topological polar surface area (TPSA, in Å(2)) of ≥0.2×molecular weight (MW). Meanwhile, good passive membrane permeability requires a molecular (i.e., 3D) PSA in nonpolar environments of ≤140Å(2). We show that one or other of these limits is almost invariably violated for compounds with MW>600Da, suggesting that some degree of chameleonic behavior is required for most high MW oral drugs., (Copyright © 2016. Published by Elsevier Ltd.)

Published

2016

34. The FTMap family of web servers for determining and characterizing ligand-binding hot spots of proteins.

Author

Kozakov D, Grove LE, Hall DR, Bohnuud T, Mottarella SE, Luo L, Xia B, Beglov D, and Vajda S

Subjects

Binding Sites, Databases, Protein, Internet, Ligands, Molecular Probes, Protein Conformation, Computational Biology methods, Proteins chemistry, Proteins metabolism

Abstract

FTMap is a computational mapping server that identifies binding hot spots of macromolecules-i.e., regions of the surface with major contributions to the ligand-binding free energy. To use FTMap, users submit a protein, DNA or RNA structure in PDB (Protein Data Bank) format. FTMap samples billions of positions of small organic molecules used as probes, and it scores the probe poses using a detailed energy expression. Regions that bind clusters of multiple probe types identify the binding hot spots in good agreement with experimental data. FTMap serves as the basis for other servers, namely FTSite, which is used to predict ligand-binding sites, FTFlex, which is used to account for side chain flexibility, FTMap/param, used to parameterize additional probes and FTDyn, for mapping ensembles of protein structures. Applications include determining the druggability of proteins, identifying ligand moieties that are most important for binding, finding the most bound-like conformation in ensembles of unliganded protein structures and providing input for fragment-based drug design. FTMap is more accurate than classical mapping methods such as GRID and MCSS, and it is much faster than the more-recent approaches to protein mapping based on mixed molecular dynamics. By using 16 probe molecules, the FTMap server finds the hot spots of an average-size protein in <1 h. As FTFlex performs mapping for all low-energy conformers of side chains in the binding site, its completion time is proportionately longer.

Published

2015

35. Energy Minimization on Manifolds for Docking Flexible Molecules.

Author

Mirzaei H, Zarbafian S, Villar E, Mottarella S, Beglov D, Vajda S, Paschalidis ICh, Vakili P, and Kozakov D

Subjects

Algorithms, Ligands, Molecular Docking Simulation, Pliability, Rotation, Proteins chemistry, Small Molecule Libraries chemistry

Abstract

In this paper, we extend a recently introduced rigid body minimization algorithm, defined on manifolds, to the problem of minimizing the energy of interacting flexible molecules. The goal is to integrate moving the ligand in six dimensional rotational/translational space with internal rotations around rotatable bonds within the two molecules. We show that adding rotational degrees of freedom to the rigid moves of the ligand results in an overall optimization search space that is a manifold to which our manifold optimization approach can be extended. The effectiveness of the method is shown for three different docking problems of increasing complexity. First, we minimize the energy of fragment-size ligands with a single rotatable bond as part of a protein mapping method developed for the identification of binding hot spots. Second, we consider energy minimization for docking a flexible ligand to a rigid protein receptor, an approach frequently used in existing methods. In the third problem, we account for flexibility in both the ligand and the receptor. Results show that minimization using the manifold optimization algorithm is substantially more efficient than minimization using a traditional all-atom optimization algorithm while producing solutions of comparable quality. In addition to the specific problems considered, the method is general enough to be used in a large class of applications such as docking multidomain proteins with flexible hinges. The code is available under open source license (at http://cluspro.bu.edu/Code/Code&#95;Rigtree.tar) and with minimal effort can be incorporated into any molecular modeling package.

Published

2015

36. In silico identification of an aryl hydrocarbon receptor antagonist with biological activity in vitro and in vivo.

Author

Parks AJ, Pollastri MP, Hahn ME, Stanford EA, Novikov O, Franks DG, Haigh SE, Narasimhan S, Ashton TD, Hopper TG, Kozakov D, Beglov D, Vajda S, Schlezinger JJ, and Sherr DH

Subjects

Animals, Bone Marrow Cells drug effects, COS Cells, Cell Line, Cell Line, Tumor, Cell Movement drug effects, Cell Proliferation drug effects, Chlorocebus aethiops, Humans, Ligands, Male, Mice, Mice, Inbred C57BL, Stromal Cells drug effects, Triple Negative Breast Neoplasms drug therapy, Biological Factors pharmacology, Receptors, Aryl Hydrocarbon antagonists & inhibitors

Abstract

The aryl hydrocarbon receptor (AHR) is critically involved in several physiologic processes, including cancer progression and multiple immune system activities. We, and others, have hypothesized that AHR modulators represent an important new class of targeted therapeutics. Here, ligand shape-based virtual modeling techniques were used to identify novel AHR ligands on the basis of previously identified chemotypes. Four structurally unique compounds were identified. One lead compound, 2-((2-(5-bromofuran-2-yl)-4-oxo-4H-chromen-3-yl)oxy)acetamide (CB7993113), was further tested for its ability to block three AHR-dependent biologic activities: triple-negative breast cancer cell invasion or migration in vitro and AHR ligand-induced bone marrow toxicity in vivo. CB7993113 directly bound both murine and human AHR and inhibited polycyclic aromatic hydrocarbon (PAH)- and TCDD-induced reporter activity by 75% and 90% respectively. A novel homology model, comprehensive agonist and inhibitor titration experiments, and AHR localization studies were consistent with competitive antagonism and blockade of nuclear translocation as the primary mechanism of action. CB7993113 (IC50 3.3 × 10(-7) M) effectively reduced invasion of human breast cancer cells in three-dimensional cultures and blocked tumor cell migration in two-dimensional cultures without significantly affecting cell viability or proliferation. Finally, CB7993113 effectively inhibited the bone marrow ablative effects of 7,12-dimethylbenz[a]anthracene in vivo, demonstrating drug absorption and tissue distribution leading to pharmacological efficacy. These experiments suggest that AHR antagonists such as CB7993113 may represent a new class of targeted therapeutics for immunomodulation and/or cancer therapy., (Copyright © 2014 by The American Society for Pharmacology and Experimental Therapeutics.)

Published

2014

37. Ligand binding and activation of PPARγ by Firemaster® 550: effects on adipogenesis and osteogenesis in vitro.

Author

Pillai HK, Fang M, Beglov D, Kozakov D, Vajda S, Stapleton HM, Webster TF, and Schlezinger JJ

Subjects

Adipocytes, Animals, Bone Marrow Cells cytology, Bone Marrow Cells metabolism, Cell Line, Child, Dust analysis, Environmental Exposure analysis, Humans, Mice, PPAR gamma antagonists & inhibitors, Adipogenesis drug effects, Bone Marrow Cells drug effects, Flame Retardants toxicity, Osteogenesis drug effects, PPAR gamma metabolism, Stromal Cells drug effects

Abstract

Background: The use of alternative flame retardants has increased since the phase out of pentabromodiphenyl ethers (pentaBDEs). One alternative, Firemaster® 550 (FM550), induces obesity in rats. Triphenyl phosphate (TPP), a component of FM550, has a structure similar to that of organotins, which are obesogenic in rodents., Objectives: We tested the hypothesis that components of FM550 are biologically active peroxisome proliferator-activated receptor γ (PPARγ) ligands and estimated indoor exposure to TPP., Methods: FM550 and its components were assessed for ligand binding to and activation of human PPARγ. Solvent mapping was used to model TPP in the PPARγ binding site. Adipocyte and osteoblast differentiation were assessed in bone marrow multipotent mesenchymal stromal cell models. We estimated exposure of children to TPP using a screening-level indoor exposure model and house dust concentrations determined previously., Results: FM550 bound human PPARγ, and binding appeared to be driven primarily by TPP. Solvent mapping revealed that TPP interacted with binding hot spots within the PPARγ ligand binding domain. FM550 and its organophosphate components increased human PPARγ1 transcriptional activity in a Cos7 reporter assay and induced lipid accumulation and perilipin protein expression in BMS2 cells. FM550 and TPP diverted osteogenic differentiation toward adipogenesis in primary mouse bone marrow cultures. Our estimates suggest that dust ingestion is the major route of exposure of children to TPP., Conclusions: Our findings suggest that FM550 components bind and activate PPARγ. In addition, in vitro exposure initiated adipocyte differentiation and antagonized osteogenesis. TPP likely is a major contributor to these biological actions. Given that TPP is ubiquitous in house dust, further studies are warranted to investigate the health effects of FM550.

Published

2014

38. Efficient Maintenance and Update of Nonbonded Lists in Macromolecular Simulations.

Author

Chowdhury R, Beglov D, Moghadasi M, Paschalidis IC, Vakili P, Vajda S, Bajaj C, and Kozakov D

Abstract

Molecular mechanics and dynamics simulations use distance based cutoff approximations for faster computation of pairwise van der Waals and electrostatic energy terms. These approximations traditionally use a precalculated and periodically updated list of interacting atom pairs, known as the "nonbonded neighborhood lists" or nblists, in order to reduce the overhead of finding atom pairs that are within distance cutoff. The size of nblists grows linearly with the number of atoms in the system and superlinearly with the distance cutoff, and as a result, they require significant amount of memory for large molecular systems. The high space usage leads to poor cache performance, which slows computation for large distance cutoffs. Also, the high cost of updates means that one cannot afford to keep the data structure always synchronized with the configuration of the molecules when efficiency is at stake. We propose a dynamic octree data structure for implicit maintenance of nblists using space linear in the number of atoms but independent of the distance cutoff. The list can be updated very efficiently as the coordinates of atoms change during the simulation. Unlike explicit nblists, a single octree works for all distance cutoffs. In addition, octree is a cache-friendly data structure, and hence, it is less prone to cache miss slowdowns on modern memory hierarchies than nblists. Octrees use almost 2 orders of magnitude less memory, which is crucial for simulation of large systems, and while they are comparable in performance to nblists when the distance cutoff is small, they outperform nblists for larger systems and large cutoffs. Our tests show that octree implementation is approximately 1.5 times faster in practical use case scenarios as compared to nblists.

Published

2014

39. How proteins bind macrocycles.

Author

Villar EA, Beglov D, Chennamadhavuni S, Porco JA Jr, Kozakov D, Vajda S, and Whitty A

Subjects

Binding Sites drug effects, Biological Availability, Crystallography, X-Ray, Drug Design, Mass Spectrometry, Models, Molecular, Molecular Weight, Pharmaceutical Preparations metabolism, Proteins metabolism, Small Molecule Libraries, Macrocyclic Compounds metabolism, Protein Binding drug effects

Abstract

The potential utility of synthetic macrocycles (MCs) as drugs, particularly against low-druggability targets such as protein-protein interactions, has been widely discussed. There is little information, however, to guide the design of MCs for good target protein-binding activity or bioavailability. To address this knowledge gap, we analyze the binding modes of a representative set of MC-protein complexes. The results, combined with consideration of the physicochemical properties of approved macrocyclic drugs, allow us to propose specific guidelines for the design of synthetic MC libraries with structural and physicochemical features likely to favor strong binding to protein targets as well as good bioavailability. We additionally provide evidence that large, natural product-derived MCs can bind targets that are not druggable by conventional, drug-like compounds, supporting the notion that natural product-inspired synthetic MCs can expand the number of proteins that are druggable by synthetic small molecules.

Published

2014

40. Docking server for the identification of heparin binding sites on proteins.

Author

Mottarella SE, Beglov D, Beglova N, Nugent MA, Kozakov D, and Vajda S

Subjects

Binding Sites, Heparitin Sulfate metabolism, Humans, Monte Carlo Method, Protein Conformation, Solvents chemistry, Heparin metabolism, Molecular Docking Simulation, Proteins chemistry, Proteins metabolism

Abstract

Many proteins of widely differing functionality and structure are capable of binding heparin and heparan sulfate. Since crystallizing protein-heparin complexes for structure determination is generally difficult, computational docking can be a useful approach for understanding specific interactions. Previous studies used programs originally developed for docking small molecules to well-defined pockets, rather than for docking polysaccharides to highly charged shallow crevices that usually bind heparin. We have extended the program PIPER and the automated protein-protein docking server ClusPro to heparin docking. Using a molecular mechanics energy function for scoring and the fast Fourier transform correlation approach, the method generates and evaluates close to a billion poses of a heparin tetrasaccharide probe. The docked structures are clustered using pairwise root-mean-square deviations as the distance measure. It was shown that clustering of heparin molecules close to each other but having different orientations and selecting the clusters with the highest protein-ligand contacts reliably predicts the heparin binding site. In addition, the centers of the five most populated clusters include structures close to the native orientation of the heparin. These structures can provide starting points for further refinement by methods that account for flexibility such as molecular dynamics. The heparin docking method is available as an advanced option of the ClusPro server at http://cluspro.bu.edu/ .

Published

2014

41. Encounter complexes and dimensionality reduction in protein-protein association.

Author

Kozakov D, Li K, Hall DR, Beglov D, Zheng J, Vakili P, Schueler-Furman O, Paschalidis ICh, Clore GM, and Vajda S

Subjects

Molecular Docking Simulation, Protein Binding, Protein Conformation, Thermodynamics, Proteins chemistry, Proteins metabolism

Abstract

An outstanding challenge has been to understand the mechanism whereby proteins associate. We report here the results of exhaustively sampling the conformational space in protein-protein association using a physics-based energy function. The agreement between experimental intermolecular paramagnetic relaxation enhancement (PRE) data and the PRE profiles calculated from the docked structures shows that the method captures both specific and non-specific encounter complexes. To explore the energy landscape in the vicinity of the native structure, the nonlinear manifold describing the relative orientation of two solid bodies is projected onto a Euclidean space in which the shape of low energy regions is studied by principal component analysis. Results show that the energy surface is canyon-like, with a smooth funnel within a two dimensional subspace capturing over 75% of the total motion. Thus, proteins tend to associate along preferred pathways, similar to sliding of a protein along DNA in the process of protein-DNA recognition. DOI: http://dx.doi.org/10.7554/eLife.01370.001.

Published

2014

42. Organization of the human mitochondrial transcription initiation complex.

Author

Yakubovskaya E, Guja KE, Eng ET, Choi WS, Mejia E, Beglov D, Lukin M, Kozakov D, and Garcia-Diaz M

Subjects

DNA-Binding Proteins metabolism, DNA-Directed RNA Polymerases metabolism, Humans, Mitochondrial Proteins metabolism, Models, Molecular, Promoter Regions, Genetic, Transcription Factors metabolism, DNA-Binding Proteins chemistry, DNA-Directed RNA Polymerases chemistry, Methyltransferases chemistry, Mitochondria genetics, Mitochondrial Proteins chemistry, Transcription Factors chemistry, Transcription Initiation, Genetic

Abstract

Initiation of transcription in human mitochondria involves two factors, TFAM and TFB2M, in addition to the mitochondrial RNA polymerase, POLRMT. We have investigated the organization of the human mitochondrial transcription initiation complex on the light-strand promoter (LSP) through solution X-ray scattering, electron microscopy (EM) and biochemical studies. Our EM results demonstrate a compact organization of the initiation complex, suggesting that protein-protein interactions might help mediate initiation. We demonstrate that, in the absence of DNA, only POLRMT and TFAM form a stable interaction, albeit one with low affinity. This is consistent with the expected transient nature of the interactions necessary for initiation and implies that the promoter DNA acts as a scaffold that enables formation of the full initiation complex. Docking of known crystal structures into our EM maps results in a model for transcriptional initiation that strongly correlates with new and existing biochemical observations. Our results reveal the organization of TFAM, POLRMT and TFB2M around the LSP and represent the first structural characterization of the entire mitochondrial transcriptional initiation complex.

Published

2014

43. Stimulators of translation identified during a small molecule screening campaign.

Author

Shin U, Williams DE, Kozakov D, Hall DR, Beglov D, Vajda S, Andersen RJ, and Pelletier J

Subjects

Adenosine Triphosphate metabolism, Azepines pharmacology, Drug Evaluation, Preclinical, High-Throughput Screening Assays, Models, Molecular, Protein Conformation, Pyrroles pharmacology, eIF-2 Kinase chemistry, eIF-2 Kinase metabolism, Protein Biosynthesis drug effects, Small Molecule Libraries pharmacology

Abstract

In screening a library of natural and synthetic products for eukaryotic translation modulators, we identified two natural products, isohymenialdisine and hymenialdisine, that exhibit stimulatory effects on translation. The characterization of these compounds led to the insight that mRNA used to program the translation extracts during high-throughput assay setup was leading to phosphorylation of eIF2α, a potent negative regulatory event that is mediated by one of four kinases. We identified double-stranded RNA-dependent protein kinase (PKR) as the eIF2α kinase that was being activated by exogenously added mRNA template. Characterization of the mode of action of isohymenialdisine revealed that it directly acts on PKR by inhibiting autophosphorylation, perturbs the PKR-eIF2α phosphorylation axis, and can be modeled into the PKR ATP binding site. Our results identify a source of "false positives" for high-throughput screen campaigns using translation extracts, raising a cautionary note for this type of screen.

Published

2014

44. Detection of peptide-binding sites on protein surfaces: the first step toward the modeling and targeting of peptide-mediated interactions.

Author

Lavi A, Ngan CH, Movshovitz-Attias D, Bohnuud T, Yueh C, Beglov D, Schueler-Furman O, and Kozakov D

Subjects

Binding Sites, Databases, Protein, Ligands, Models, Molecular, Protein Binding, Protein Conformation, Software, Computational Biology, Membrane Proteins chemistry, Peptides chemistry, Protein Interaction Maps

Abstract

Peptide-mediated interactions, in which a short linear motif binds to a globular domain, play major roles in cellular regulation. An accurate structural model of this type of interaction is an excellent starting point for the characterization of the binding specificity of a given peptide-binding domain. A number of different protocols have recently been proposed for the accurate modeling of peptide-protein complex structures, given the structure of the protein receptor and the binding site on its surface. When no information about the peptide binding site(s) is a priori available, there is a need for new approaches to locate peptide-binding sites on the protein surface. While several approaches have been proposed for the general identification of ligand binding sites, peptides show very specific binding characteristics, and therefore, there is a need for robust and accurate approaches that are optimized for the prediction of peptide-binding sites. Here, we present PeptiMap, a protocol for the accurate mapping of peptide binding sites on protein structures. Our method is based on experimental evidence that peptide-binding sites also bind small organic molecules of various shapes and polarity. Using an adaptation of ab initio ligand binding site prediction based on fragment mapping (FTmap), we optimize a protocol that specifically takes into account peptide binding site characteristics. In a high-quality curated set of peptide-protein complex structures PeptiMap identifies for most the accurate site of peptide binding among the top ranked predictions. We anticipate that this protocol will significantly increase the number of accurate structural models of peptide-mediated interactions., (Copyright © 2013 Wiley Periodicals, Inc.)

Published

2013

45. How good is automated protein docking?

Author

Kozakov D, Beglov D, Bohnuud T, Mottarella SE, Xia B, Hall DR, and Vajda S

Subjects

Computational Biology, Computer Simulation, Databases, Protein, Humans, Internet, Models, Molecular, Monte Carlo Method, Protein Conformation, Proteomics, Molecular Docking Simulation, Protein Interaction Mapping, Proteins chemistry, Software

Abstract

The protein docking server ClusPro has been participating in critical assessment of prediction of interactions (CAPRI) since its introduction in 2004. This article evaluates the performance of ClusPro 2.0 for targets 46-58 in Rounds 22-27 of CAPRI. The analysis leads to a number of important observations. First, ClusPro reliably yields acceptable or medium accuracy models for targets of moderate difficulty that have also been successfully predicted by other groups, and fails only for targets that have few acceptable models submitted. Second, the quality of automated docking by ClusPro is very close to that of the best human predictor groups, including our own submissions. This is very important, because servers have to submit results within 48 h and the predictions should be reproducible, whereas human predictors have several weeks and can use any type of information. Third, while we refined the ClusPro results for manual submission by running computationally costly Monte Carlo minimization simulations, we observed significant improvement in accuracy only for two of the six complexes correctly predicted by ClusPro. Fourth, new developments, not seen in previous rounds of CAPRI, are that the top ranked model provided by ClusPro was acceptable or better quality for all these six targets, and that the top ranked model was also the highest quality for five of the six, confirming that ranking models based on cluster size can reliably identify the best near-native conformations., (Copyright © 2013 Wiley Periodicals, Inc.)

Published

2013

46. Community-wide evaluation of methods for predicting the effect of mutations on protein-protein interactions.

Author

Moretti R, Fleishman SJ, Agius R, Torchala M, Bates PA, Kastritis PL, Rodrigues JP, Trellet M, Bonvin AM, Cui M, Rooman M, Gillis D, Dehouck Y, Moal I, Romero-Durana M, Perez-Cano L, Pallara C, Jimenez B, Fernandez-Recio J, Flores S, Pacella M, Praneeth Kilambi K, Gray JJ, Popov P, Grudinin S, Esquivel-Rodríguez J, Kihara D, Zhao N, Korkin D, Zhu X, Demerdash ON, Mitchell JC, Kanamori E, Tsuchiya Y, Nakamura H, Lee H, Park H, Seok C, Sarmiento J, Liang S, Teraguchi S, Standley DM, Shimoyama H, Terashi G, Takeda-Shitaka M, Iwadate M, Umeyama H, Beglov D, Hall DR, Kozakov D, Vajda S, Pierce BG, Hwang H, Vreven T, Weng Z, Huang Y, Li H, Yang X, Ji X, Liu S, Xiao Y, Zacharias M, Qin S, Zhou HX, Huang SY, Zou X, Velankar S, Janin J, Wodak SJ, and Baker D

Subjects

Algorithms, Mutation, Protein Binding, Databases, Protein, Protein Interaction Mapping

Abstract

Community-wide blind prediction experiments such as CAPRI and CASP provide an objective measure of the current state of predictive methodology. Here we describe a community-wide assessment of methods to predict the effects of mutations on protein-protein interactions. Twenty-two groups predicted the effects of comprehensive saturation mutagenesis for two designed influenza hemagglutinin binders and the results were compared with experimental yeast display enrichment data obtained using deep sequencing. The most successful methods explicitly considered the effects of mutation on monomer stability in addition to binding affinity, carried out explicit side-chain sampling and backbone relaxation, evaluated packing, electrostatic, and solvation effects, and correctly identified around a third of the beneficial mutations. Much room for improvement remains for even the best techniques, and large-scale fitness landscapes should continue to provide an excellent test bed for continued evaluation of both existing and new prediction methodologies., (© 2013 Wiley Periodicals, Inc.)

Published

2013

47. FTFlex: accounting for binding site flexibility to improve fragment-based identification of druggable hot spots.

Author

Grove LE, Hall DR, Beglov D, Vajda S, and Kozakov D

Subjects

Binding Sites, Ligands, Models, Molecular, Protein Conformation, Proteins metabolism, Software, Solvents chemistry, Algorithms, Drug Design, Proteins chemistry

Abstract

Unlabelled: Computational solvent mapping finds binding hot spots, determines their druggability and provides information for drug design. While mapping of a ligand-bound structure yields more accurate results, usually the apo structure serves as the starting point in design. The FTFlex algorithm, implemented as a server, can modify an apo structure to yield mapping results that are similar to those of the respective bound structure. Thus, FTFlex is an extension of our FTMap server, which only considers rigid structures. FTFlex identifies flexible residues within the binding site and determines alternative conformations using a rotamer library. In cases where the mapping results of the apo structure were in poor agreement with those of the bound structure, FTFlex was able to yield a modified apo structure, which lead to improved FTMap results. In cases where the mapping results of the apo and bound structures were in good agreement, no new structure was predicted., Availability: FTFlex is freely available as a web-based server at http://ftflex.bu.edu/.

Published

2013

48. Comprehensive experimental and computational analysis of binding energy hot spots at the NF-κB essential modulator/IKKβ protein-protein interface.

Author

Golden MS, Cote SM, Sayeg M, Zerbe BS, Villar EA, Beglov D, Sazinsky SL, Georgiadis RM, Vajda S, Kozakov D, and Whitty A

Subjects

Alanine chemistry, Algorithms, Amino Acids chemistry, Anisotropy, Computational Biology, Genetic Vectors, I-kappa B Kinase genetics, Models, Molecular, Mutagenesis, Mutagenesis, Site-Directed, Protein Binding, Recombinant Fusion Proteins, Signal Transduction, X-Ray Diffraction, I-kappa B Kinase chemistry, NF-kappa B chemistry, NF-kappa B genetics

Abstract

We report a comprehensive analysis of binding energy hot spots at the protein-protein interaction (PPI) interface between nuclear factor kappa B (NF-κB) essential modulator (NEMO) and IκB kinase subunit β (IKKβ), an interaction that is critical for NF-κB pathway signaling, using experimental alanine scanning mutagenesis and also the FTMap method for computational fragment screening. The experimental results confirm that the previously identified NEMO binding domain (NBD) region of IKKβ contains the highest concentration of hot-spot residues, the strongest of which are W739, W741, and L742 (ΔΔG = 4.3, 3.5, and 3.2 kcal/mol, respectively). The region occupied by these residues defines a potentially druggable binding site on NEMO that extends for ~16 Å to additionally include the regions that bind IKKβ L737 and F734. NBD residues D738 and S740 are also important for binding but do not make direct contact with NEMO, instead likely acting to stabilize the active conformation of surrounding residues. We additionally found two previously unknown hot-spot regions centered on IKKβ residues L708/V709 and L719/I723. The computational approach successfully identified all three hot-spot regions on IKKβ. Moreover, the method was able to accurately quantify the energetic importance of all hot-spot residues involving direct contact with NEMO. Our results provide new information to guide the discovery of small-molecule inhibitors that target the NEMO/IKKβ interaction. They additionally clarify the structural and energetic complementarity between "pocket-forming" and "pocket-occupying" hot-spot residues, and further validate computational fragment mapping as a method for identifying hot spots at PPI interfaces.

Published

2013

49. Flexible Refinement of Protein-Ligand Docking on Manifolds.

Author

Mirzaei H, Villar E, Mottarella S, Beglov D, Paschalidis IC, Vajda S, Kozakov D, and Vakili P

Abstract

Our work is motivated by energy minimization of biological macromolecules, an essential step in computational docking. By allowing some ligand flexibility, we generalize a recently introduced novel representation of rigid body minimization as an optimization on the [Formula: see text] manifold, rather than on the commonly used Special Euclidean group SE (3). We show that the resulting flexible docking can also be formulated as an optimization on a Lie group that is the direct product of simpler Lie groups for which geodesics and exponential maps can be easily obtained. Our computational results for a local optimization algorithm developed based on this formulation show that it is about an order of magnitude faster than the state-of-the-art local minimization algorithms for computational protein-small molecule docking.

Published

2013

50. A New Approach to Rigid Body Minimization with Application to Molecular Docking.

Author

Mirzaei H, Kozakov D, Beglov D, Paschalidis IC, Vajda S, and Vakili P

Abstract

Our work is motivated by energy minimization in the space of rigid affine transformations of macromolecules, an essential step in computational protein-protein docking. We introduce a novel representation of rigid body motion that leads to a natural formulation of the energy minimization problem as an optimization on the [Formula: see text] manifold, rather than the commonly used SE (3). The new representation avoids the complications associated with optimization on the SE (3) manifold and provides additional flexibilities for optimization not available in that formulation. The approach is applicable to general rigid body minimization problems. Our computational results for a local optimization algorithm developed based on the new approach show that it is about an order of magnitude faster than a state of art local minimization algorithms for computational protein-protein docking.

Published

2012