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Direct Investigation of Slow Correlated Dynamics in Proteins via Dipolar Interactions.


ABSTRACT: The synchronization of native state motions as they transition between microstates influences catalysis kinetics, mediates allosteric interactions, and reduces the conformational entropy of proteins. However, it has proven difficult to describe native microstates because they are usually minimally frustrated and may interconvert on the micro- to millisecond time scale. Direct observation of concerted equilibrium fluctuations would therefore be an important tool for describing protein native states. Here we propose a strategy that relates NMR cross-correlated relaxation (CCR) rates between dipolar interactions to residual dipolar couplings (RDCs) of individual consecutive H(N)-N and H(?)-C(?) bonds, which act as a proxy for the peptide planes and the side chains, respectively. Using Xplor-NIH ensemble structure calculations restrained with the RDC and CCR data, we observe collective motions on time scales slower than nanoseconds in the backbone for GB3. To directly access the correlations from CCR, we develop a structure-free data analysis. The resulting dynamic correlation map is consistent with the ensemble-restrained simulations and reveals a complex network. In general, we find that the bond motions are on average slightly correlated and that the local environment dominates many observations. Despite this, some patterns are typical over entire secondary structure elements. In the ?-sheet, nearly all bonds are weakly correlated, and there is an approximately binary alternation in correlation intensity corresponding to the solvent exposure/shielding alternation of the side chains. For ?-helices, there is also a weak correlation in the H(N)-N bonds. The degree of correlation involving H(?)-C(?) bonds is directly affected by side-chain fluctuations, whereas loops show complex and nonuniform behavior.

SUBMITTER: Fenwick RB 

PROVIDER: S-EPMC5055379 | biostudies-literature | 2016 Jul

REPOSITORIES: biostudies-literature

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Direct Investigation of Slow Correlated Dynamics in Proteins via Dipolar Interactions.

Fenwick R Bryn RB   Schwieters Charles D CD   Vögeli Beat B  

Journal of the American Chemical Society 20160701 27


The synchronization of native state motions as they transition between microstates influences catalysis kinetics, mediates allosteric interactions, and reduces the conformational entropy of proteins. However, it has proven difficult to describe native microstates because they are usually minimally frustrated and may interconvert on the micro- to millisecond time scale. Direct observation of concerted equilibrium fluctuations would therefore be an important tool for describing protein native stat  ...[more]

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