Physical Origin of Anharmonic Dynamics in Proteins: New Insights From Resolution-Dependent Neutron Scattering on Homomeric Polypeptides

Neutron scattering reveals a complex dynamics in polypeptide chains, with two main onsets of anharmonicity whose physical origin and biological role are still debated. In this study the dynamics of strategically selected homomeric polypeptides is investigated with elastic neutron scattering using different energy resolutions and compared with that of a real protein. Our data spotlight the dependence of anharmonic transition temperatures and fluctuation amplitudes on energy resolution, which we quantitatively explain in terms of a two-site model for the protein-hydration water energy landscape. Experimental data strongly suggest that the protein dynamical transition is not a mere resolution effect but is due to a real physical effect. Activation barriers and free energy values obtained for the protein dynamical transition allow us to make a connection with the two-well interaction potential of supercooledconfined water proposed to explain a low-density -- high-density liquid-liquid transition

Hydration dependence of myoglobin dynamics studied with elastic neutron scattering, differential scanning calorimetry and broadband dielectric spectroscopy

In this work we present a thorough investigation of the hydration dependence of myoglobin dynamics. The study is performed on D2O-hydrated protein powders in the hydration range 0<h<0.5 (h≡gr[D2O]/gr[protein]) and in the temperature range 20-300K. The protein equilibrium fluctuations are investigated with Elastic Neutron Scattering using the spectrometer IN13 at ILL (Grenoble), while the relaxations of the protein + hydration water system are investigated with Broadband Dielectric Spectroscopy; finally, Differential Scanning Calorimetry is used to obtain a thermodynamic description of the system. The effect of increasing hydration is to speed up the relaxations of the myoglobin + hydration water system and, thermodynamically, to decrease the glass transition temperature; these effects tend to saturate at h values greater than ~0.3. Moreover, the calorimetric scans put in evidence the occurrence of an endothermic peak whose onset temperature is located at ~230K independent of hydration. From the point of view of the protein equilibrium fluctuations, while the amplitude of anharmonic mean square displacements is found to increase with hydration, their onset temperature (i.e. the onset temperature of the well known “protein dynamical transition”) is hydration independent. On the basis of the above results, the relevance of protein + hydration water relaxations and of the thermodynamic state of hydration water to the onset of the protein dynamical transition is discussed

The “Protein Dynamical Transition” Does Not Require the Protein Polypeptide Chain

We give experimental evidence that the main features of protein dynamics revealed by neutron scattering, i.e., the “protein dynamical transition” and the “boson peak”, do not need the protein polypeptide chain. We show that a rapid increase of hydrogen atoms fluctuations at about 220 K, analogous to the one observed in hydrated myoglobin powders, is also observed in a hydrated amino acids mixture with the chemical composition of myoglobin but lacking the polypeptide chain; in agreement with the protein behavior, the transition is abolished in the dry mixture. Further, an excess of low-frequency vibrational modes around 3 meV, typically observed in protein powders, is also observed in our mixture. Our results confirm that the dynamical transition is a water-driven onset and indicate that it mainly involves the amino acid side chains. Taking together the present data and recent results on the dynamics of a protein in denatured conformation and on the activity of dehydrated proteins, it can be concluded that the “protein dynamical transition” is neither a necessary nor a sufficient condition for active protein conformation and function

Photochemical mechanism of an atypical algal phytochrome

International audiencePhytochromes are bilin-containing photoreceptors that are typically sensitive to the red/far-red region of the visible spectrum. Recently, phytochromes from certain eukaryotic algae have become attractive targets for optogenetic applications because of their unique ability to respond to multiple wavelengths of light. Herein, a combination of time-resolved spectroscopy and structural approaches across picosecond to second timescales have been used to map photochemical mechanisms and structural changes in this atypical group of phytochromes. The photochemistry of an orange/far-red light-sensitive algal phytochrome from Dolihomastix tenuilepis has been investigated by using a combination of visible, IR and X-ray scattering probes. The entire photocycle, correlated with accompanying structural changes in the cofactor/protein, are reported. This study identifies a complex photocycle for this atypical phytochrome. It also highlights a need to combine outcomes from a range of biophysical approaches to unravel complex photochemical and macromolecular processes in multi-domain photoreceptor proteins that are the basis of biological light-mediated signalling

Protein/Hydration Water Dynamics in Hard Confinement: Dielectric Relaxations and Picoseconds Hydrogen Fluctuations

In this review we report on some experimental studies on the dynamics of Myoglobin in a confined geometry, obtained by encapsulation in a porous silica matrix, at low hydration levels. After formation through the solgel method, the samples were left aging/drying in order to reach a condition where only one or two water layers surround the proteins. In order to put in evidence the specific effect of confinement in the silica host, we compared this system with another one (i.e. hydrated powder) where proteins are confined by other proteins. Using elastic neutron scattering we investigate the temperature dependence of the mean square displacements of non-exchangeable hydrogen atoms of sol-gel encapsulated Myoglobin. In order to clarify the effect of hydration the study was extended to samples at 0.2, 0.3 and 0.5 [gr water]/[gr protein] fractions and comparison was made with Myoglobin powders at the same average hydration and with a dry powder sample. Comparison between the data relative to the different samples indicates that geometrical confinement within the matrix plays a crucial role in protein dynamics and conformational stability, the effect of sol-gel encapsulation being essentially a reduction of collective protein motions likely related to the slowing down of solvent confined diffusion. A dielectric spectroscopy investigation on the same systems helped us to clarify the effect of encapsulation on protein/solvent dynamics. In agreement with elastic neutron scattering, although in a much slower time scale, dielectric spectroscopy indicates a suppression of cooperative relaxation inside the gel, together with a clear dependence of relaxation rates on the hydration degree

Quaternary relaxations in sol-gel encapsulated hemoglobin studied via NIR and UV spectroscopy

In this work, we study the kinetics of the R f T transition in hemoglobin using a combination of near-infrared and near-ultraviolet spectroscopy. We use a sol-gel encapsulation protocol to decelerate the conformational transitions and to avoid spectral perturbations arising from ligand migration and recombination. We monitor two spectroscopic markers: band III in the near-IR, which is a fine probe of the heme pocket conformation, and the tryptophan band in the near-UV, which probes the formation of the Trpâ37-AspR94 hydrogen bond, characteristic of the T structure, at the critical R1â2 subunit interface. The time evolution of these two bands is monitored after deoxygenation of encapsulated oxyhemoglobin, obtained by diffusion of a reducing agent into the porous silica matrix. Characteristic spectral shifts are observed: comparison with myoglobin enables us to assign them to quaternary structure relaxations. Band III spectral relaxation is clearly nonexponential, and analysis with the Maximum Entropy Method enables us to identify three processes. On the other hand, near-UV spectral relaxation follows an exponential decay with a time constant closely corresponding to the second process observed in the near IR. Very interestingly, the rates of all processes markedly depend on the viscosity of the co-encapsulated solvent, following a power law. Our results reveal correlations between heme pocket relaxations, induced by the R f T transition, and structural event(s) occurring at the R1â2 interface and highlight their solvent dependence. The power law viscosity dependence of relaxation rates suggests that the observed protein relaxations are “slaved” to the co-encapsulated solvent. The stepwise character of the quaternary transition is also evidence