Nathan W. Jenkins scite author profile

Computational methodologies are increasingly addressing modeling of the whole cell at the molecular level. Proteins and their interactions are the key component of cellular processes. Techniques for modeling protein interactions, thus far, have included protein docking and molecular simulation. The latter approaches account for the dynamics of the interactions but are relatively slow, if carried out at all-atom resolution, or are significantly coarse grained. Protein docking algorithms are far more efficient in sampling spatial coordinates. However, they do not account for the kinetics of the association (i.e., they do not involve the time coordinate). Our proof-of-concept study bridges the two modeling approaches, developing an approach that can reach unprecedented simulation timescales at all-atom resolution. The global intermolecular energy landscape of a large system of proteins was mapped by the pairwise fast Fourier transform docking and sampled in space and time by Monte Carlo simulations. The simulation protocol was parametrized on existing data and validated on a number of observations from experiments and molecular dynamics simulations. The simulation protocol performed consistently across very different systems of proteins at different protein concentrations. It recapitulated data on the previously observed protein diffusion rates and aggregation. The speed of calculation allows reaching second-long trajectories of protein systems that approach the size of the cells, at atomic resolution.

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Direct synthesis of arenecarboxamides through Friedel–Crafts acylation using ureas

Ying

Gamage

Lovro

et al. 2014

Tetrahedron Letters

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Docking-based long timescale simulation of cell-size protein systems at atomic resolution

Vakser

Grudinin

Jenkins

et al. 2022

Preprint

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Computational methodologies are increasingly addressing modeling of the whole cell at the molecular level. Proteins and their interactions are the key component of cellular processes. Techniques for modeling protein interactions, so far, have included protein docking and molecular simulation. The latter approaches account for the dynamics of the interactions, but are relatively slow, if carried out at all-atom resolution, or are significantly coarse-grained. Protein docking algorithms are far more efficient in sampling spatial coordinates. However, they do not account for the kinetics of the association (i.e., they do not involve the time coordinate). Our proof-of-concept study bridges the two modeling approaches, developing an approach that can reach unprecedented simulation timescales at all-atom resolution. The global intermolecular energy landscape of a large system of proteins was mapped by the pairwise Fast Fourier Transform docking and sampled in space and time by Monte Carlo simulations. The simulation protocol was parametrized on existing data and validated on a number of observations from experiments and molecular dynamics simulations. The simulation protocol performed consistently across very different systems of proteins at different protein concentrations. It recapitulated data on the previously observed protein diffusion rates and aggregation. The speed of calculation allows reaching second-long trajectories of protein systems that approach the size of the cells, at atomic resolution.

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Corrigendum to “Direct synthesis of arenecarboxamides through Friedel–Crafts acylation using ureas” [Tetrahedron Lett. 55 (33) (2014) 4541–4544]

Ying¹,

Gamage²,

Lovro³

et al. 2015

Tetrahedron Letters

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Size of the protein-protein energy funnel in crowded environment

Jenkins

Kundrotas²,

Vakser³

2022

Front. Mol. Biosci.

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Association of proteins to a significant extent is determined by their geometric complementarity. Large-scale recognition factors, which directly relate to the funnel-like intermolecular energy landscape, provide important insights into the basic rules of protein recognition. Previously, we showed that simple energy functions and coarse-grained models reveal major characteristics of the energy landscape. As new computational approaches increasingly address structural modeling of a whole cell at the molecular level, it becomes important to account for the crowded environment inside the cell. The crowded environment drastically changes protein recognition properties, and thus significantly alters the underlying energy landscape. In this study, we addressed the effect of crowding on the protein binding funnel, focusing on the size of the funnel. As crowders occupy the funnel volume, they make it less accessible to the ligands. Thus, the funnel size, which can be defined by ligand occupancy, is generally reduced with the increase of the crowders concentration. This study quantifies this reduction for different concentration of crowders and correlates this dependence with the structural details of the interacting proteins. The results provide a better understanding of the rules of protein association in the crowded environment.

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Nathan W. Jenkins

Docking-based long timescale simulation of cell-size protein systems at atomic resolution

Direct synthesis of arenecarboxamides through Friedel–Crafts acylation using ureas

Docking-based long timescale simulation of cell-size protein systems at atomic resolution

Corrigendum to “Direct synthesis of arenecarboxamides through Friedel–Crafts acylation using ureas” [Tetrahedron Lett. 55 (33) (2014) 4541–4544]

Size of the protein-protein energy funnel in crowded environment

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