Abstract
The protein dynamical transition at ∼ 200 K, where the biomolecule transforms from a harmonic, non-functional form to an anharmonic, functional state, has been thought to be slaved to the thermal activation of dynamics in its surface hydration water. Here, by selectively probing the dynamics of protein and hydration water using elastic neutron scattering and isotopic labelling, we found that the onset of anharmonicity in the two components around 200 K are decoupled. The one in protein is an intrinsic transition, whose characteristic temperature is independent of the instrumental resolution time, but varies with the biomolecular structure and the amount of hydration, while the one of water is merely a resolution effect.
eLife assessment:
The study answers the important question of whether the conformational dynamics of proteins are slaved by the motion of solvent water or are intrinsic to the polypeptide. The results from neutron scattering experiments, involving isotopic labelling, carried out on a set of four structurally different proteins are convincing, showing that protein motions are not coupled to the solvent. A strength of this work is the study of a set of proteins using spectroscopy covering a range of resolutions, however, it suffers from some scholarly shortcomings and limited discussion of results. The work is of broad interest to researchers in the fields of protein biophysics and biochemistry.
Introduction
It is well established that the internal dynamics of a protein is crucial for its functions, including allosteric conformational changes (1), ligand binding (2) and enzymatic reactions (3). In particular, hydrated proteins exhibit a dynamical transition around 200 K, across which the slope of the temperature dependence of the atomic displacements changes significantly and the biomolecule transforms from a rigid, harmonic state, to a flexible, anharmonic form (4-12). This transition has been linked to the thermal onset of function in a number of proteins, e.g, myoglobin (13), ribonuclease (6), elastase (14) and bacteriorhodopsin (15), all of which become inactive below the dynamical transition temperature. A prevailing scenario is that the internal dynamics of the protein is slaved to the motion of the surrounding hydration water (7,12,16-19), and thus the protein dynamical transition results from the changes in the dynamics of the hydration water with temperature (5,7,12,17,20). This scenario is indirectly supported by the experimental finding that the presence of the protein dynamical transition requires a minimum amount of hydration water, ∼ 0.2 gram water/gram protein (4,8). Further support comes from the results of all-atom molecular dynamics simulations, suggesting that it is the activation of the translational motions of surface water molecules around 200 K that leads to the dynamical transition in the underlying protein (5,7,20).
This ‘slaving’ scenario can be examined directly by an experiment using isotopic labelling in combination with elastic neutron scattering methods (7,21). Neutrons are highly sensitive to hydrogen atoms as their incoherent scattering cross section is an order of magnitude higher than the incoherent and coherent scattering cross sections of other elements (22-24). Thus, neutron signals collected on an ordinary protein powder hydrated in D2O reflect the dynamics of the protein while signals from the perdeuterated sample in H2O inform about the motion of water. The experimental results derived from this combined approach are, however, inconsistent (7,21,25). Measurements performed on perdeuterated maltose binding protein hydrated in H2O revealed a harmonic-to-anharmonic transition for hydration water taking place at the same temperature as that of the underlying protein (7). In contrast, a similar experiment on perdeuterated green fluorescence protein showed that the anharmonic onset in hydration water occurs at a lower temperature than that of the protein (21). More recent measurements on lysozyme hydrated in both D2O and H2O found that the transition temperature of protein and water coincided when examining their atomic displacements at 1 ns, but took place at different temperatures when changing the explored time scale to 3 ns (25). Therefore, there remains an unanswered question concerning whether the transition in dynamics of protein around 200 K is indeed coupled to that of the hydration water, whose resolution is of fundamental importance to understand the mechanism governing the nature of their interaction.
To address this, it requires a systematic measurement of the temperature dependence of atomic displacements of the protein and its surface water separately, as a function of hydration levels, h (gram water/gram protein), and at different time scales (instrument resolutions). Here, we performed elastic neutron scattering experiments on a number of protein powders hydrated in D2O and on the perdeuterated counterparts hydrated in H2O, to track the dynamics of protein and hydration water independently. Moreover, using a range of neutron instruments with distinct resolutions, we tested the effect of the explored time scales on the dynamics of the two components. Four globular proteins with different secondary and tertiary structures (see Fig.S1 and Table SI) were studied here. We found that the onset temperature (Ton) of the protein dynamical transition varies with both biomolecular structure and hydration level, but is independent of the instrumental resolution time. Conversely, Ton of the hydration water is insensitive to both the protein structure and the level of hydration, but solely determined by the instrument resolution. Therefore, the dynamical transition of the protein is decoupled from the onset of anharmonic dynamics of its hydration water around 200 K. The onset in water cannot be assigned to a physical transition, but to a resolution effect. In contrast, the protein dynamical transition is an intrinsic change in the dynamics of the biomolecules. Complementary differential scanning calorimetry (DSC) measurements revealed a step-like change in the heat flow around the transition temperature of the protein, similar to the glass transition observed in polymers. This suggests that the dynamical transition in the protein results from a similar process involving the freezing of the structural relaxation of the protein molecules beyond equilibrium.
Results
Elastic Neutron Scattering Experiments
The quantity measured in the neutron experiment is the elastic intensity, i.e. the intensity of the elastic peak in the dynamic structure factor, S(q, Δt), where q is the scattering wave vector and Δt is the resolution time of the neutron spectrometer. S(q, Δt) is an estimate of the average amplitude of the atomic motions up to Δt (11,22). Three neutron backscattering spectrometers were chosen to cover a wide range of timescales; HFBS at the NIST Center for Neutron Scattering, USA, DNA at the Materials and Life Science Experimental Facility at J-PARC in Japan, and OSIRIS at the ISIS Neutron and Muon Facility, UK. The instrumental energy resolutions are 1 μeV, 13 μeV, 25.4 μeV and 100 μeV, corresponding to timescales of ∼1 ns, ∼80 ps, ∼40 ps, and ∼10 ps, respectively. Four globular proteins were investigated, myoglobin (MYO), cytochrome P450 (CYP), lysozyme (LYS), and green fluorescent protein (GFP), the detailed structural features of which are presented in Fig. S1 and Table SI. For simplicity, the hydrogenated and perdeuterated proteins are noted as H-protein and D-protein, respectively. Details of the sample preparation and neutron experiments are provided in Supplemental Material (SM).
Dynamics of protein
Figs. 1a to g show the temperature dependence of S(q, Δt) collected on H-LYS, H-MYO and H-CYP in dry and hydrated state with D2O measured by neutron spectrometers of different resolutions, Δt. Since the measurements were performed on H-protein in D2O, the signals reflect the dynamics of the proteins. A clear deviation can be seen in the temperature dependence of S(q, Δt) for the hydrated protein from that of the dry powder, which is defined as the onset temperature, Ton (8,12,25-27), of the protein dynamical transition. The advantage of such definition is that it highlights the effect of hydration on the anharmonic dynamics in proteins while removing the contribution from the local side groups, e.g., methyl groups, whose motions are hydration independent (11,28). As shown in Ref. (12,29), the activation temperature of the rotations of methyl group varies with the instrument resolution, which will cloud the present analysis. Two important conclusions can be drawn from Fig.1. (i) Ton is distinct for each protein, LYS (213 K), MYO (198 K) and CYP (228 K), and (ii) it is independent of the timescale explored even though the resolutions of the neutron spectrometers differ by orders of magnitude. Using the same set of data, we also analyzed the temperature dependence of the mean squared atomic displacements, <x2(Δt)> (see details in SM and results in Fig. S2) and obtained similar conclusions.
Resolution dependence of the onset of protein dynamical transition. Neutron spectrometers with different resolutions (1, 13, 25.4 and 100 □eV) were applied. Elatic intensity S(q, Δt) of (a, b) dry H-LYS and H-LYS in D2O at h = 0.3, (c, d) dry H-MYO and H-MYO in D2O at h = 0.3, and (e-g) dry H-CYP and H-CYP in D2O at h = 0.4. All the experimental S(q, Δt) are normalized to data measured at ∼10 K and summed over values of q ranging from 0.45 to 1.75 Å−1. The dashed lines in each figure identify the onset temperatures of the transition, Ton, where the neutron data of the hydrated system deviate from the dry form. The same analyses are used in Figs. 2 to 4 and S2 to S5.
These findings suggest that the dynamical transition in the protein is an intrinsic property of the hydrated biomolecule, and it depends on the structure and chemistry of the protein concerned. Our results are consistent with Ref. (12), which demonstrated that Ton in both protein and polypeptide is independent of the resolution of the neutron spectrometer, if one carefully removes the contributions from methyl rotations and vibrations to <x2(Δt)> measured by elastic neutron scattering. Additionally, Ref. (25) showed that, as compared to the dry form, the D2O-hydrated lysozyme presents an approximately resolution-independent Ton, again in agreement with our findings.
Fig. 2 compares the temperature dependence of S(q, Δt) measured on H-CYP and H-LYS in D2O at different hydration levels, h. Evidently Ton of the protein increases from 228 to 248 K when reducing h from 0.4 to 0.2 (Figs. 2a) by using the neutron instrument with Δt = 1 ns. A similar hydration dependence of Ton is also observed when we replot the neutron data measured on H-LYS hydrated in D2O reported in Ref. (26) (Fig. 2c). It can be found that Ton of lysozyme changes systematically from 195 to 225 K, when decreasing h from 0.45 to 0.18. Similar conclusion can be obtained when we analyzed < x2(Δt)> (see Fig. S3)
Hydration dependence of the onset of protein dynamical transition. S(q, Δt) of (a) dry H-CYP and H-CYP in D2O at h = 0.2 and 0.4 and (c) dry H-LYS and H-LYS in D2O at h = 0.18, 0.30 and 0.45, all measured using HFBS with the instrumental resolution of 1 μeV. All the Data in (c) were replotted from Ref. (26). (b) DSC curves obtained for dry H-CYP and H-CYP in water at h = 0.2 and 0.4. TDSC is defined as the midpoint between two heat flow baselines, where ΔH1 = ΔH2 (35,36,49).
The results from the neutron scattering experiments suggest that the dynamical transition in proteins is an intrinsic property of the biomolecule and strongly depends on the amount of water surrounding it. Such an intrinsic transition can result either from a critical phase transition, e.g., water to ice (30,31), or from freezing of the structural relaxation of the system beyond the equilibrium time (∼100 - 1000 s) of the experiment, in analogy to the glass transition in polymers from rubbery state to the glass form (32-34). Both of them will significantly increase the mechanical modulus of the material and suppress the atomic displacements at the fast time scales (pico-to-nanosecond) probed by the neutron spectrometers (30-34) like those used in this work. To explore the microscopic nature of the protein dynamical transition, we performed differential scanning calorimetry (DSC) measurements on CYP at dry, h = 0.2 and 0.4. As illustrated by Fig. 2b, H-CYP at h = 0.2 and h = 0.4 exhibit a step-like transition in the heat flow at 245 K and 225 K, respectively, while no such transition is observed in dry H-CYP. Such step-like transition in heat flow is normally defined as the glass transition in polymers (35,36).
For simplicity, the step-like transition identified by DSC is noted as TDSC. When comparing Figs 2b with Fig. 2a, one can find that the values of TDSC approximate those of Ton probed by neutrons. TDSC of hydrated myoglobin was reported by literature to be 190 K (37), which is again in good agreement with the value of Ton in Fig. 1. More importantly, TDSC and Ton present the same hydration dependence, i.e., both increase with decrease of h (see Figs. 2a and 2b). Therefore, we can conclude that the onset of anharmonicity around 200 K in proteins measured by neutron scattering as shown in Figs. 1 and 2 results from the freezing of the structural relaxation of the biomolecule beyond the equilibrium when cooling the system below TDSC, similar to the glass transition in polymers. Similar interpretation has also been suggested in Ref.(38).
As the time scale probed by neutron spans from pico-to nanoseconds, it is too fast to allow us to directly “see” structural relaxations of the protein around Ton. However, “freezing” of the structural relaxation beyond the equilibrium time (∼100 - 1000 s), i.e., the measurement time of neutron experiments at each temperature, will turn the system into a “frozen” solid form, which can significantly suppress the fast dynamics measured by neutron and cause the transition probed (32-34,38). Moreover, water can be considered here as lubricant or plasticizer which facilitates the motion of the biomolecule (28,39,40). As widely observed in polymeric systems (41-43), adding water as plasticizer will significantly reduce the glass transition temperature of the polymers. This rationalizes the hydration effect on TDSC and Ton, both decreasing with increase of h.
Dynamics in hydration water
Figs. 3a-b and c-e show the temperature dependence of S(q, Δt) measured on perdeuterated GFP and CYP in dry and H2O-hydrated forms. In these samples, the measured signal reflects primarily the motions of water molecules. Two important observations arise from the data. Firstly, Ton of hydration water for these two proteins strongly depends on the resolution of the spectrometer, increasing drastically from 200 K to 250 K when reducing Δt from 1 ns to 10 ps. Similar conclusions are obtained when we analyzed the temperature dependence of <x2(Δt)> (see Fig. S4). The observation of a dependence of Ton on Δt is typical for a thermally activated process, which occurs when the characteristic relaxation time becomes comparable to the instrumental resolution, and the relaxation process is said to enter the time window of the instrument (29,44). In this case, it means that the relaxation time, τ, of hydration water is 10 ps at 250 K, 40 ps at 234 K and 1 ns at 200 K. Assuming an Arrhenius-type process, 
Resolution dependence of the anharmonic onset of hydration water. Neutron spectrometers with different resolutions (1, 25.4 and 100 □eV) were applied. S(q, Δt) of (a, b) dry D-GFP and D-GFP in H2O at h = 0.4, and (c-e) dry D-CYP and D-CYP in H2O at h = 0.4.
Furthermore, the hydration dependence of the anharmonic onset of the water is presented in Fig. 4, which shows that Ton remains constant with h as long as the instrument resolution is fixed. This behavior is drastically different from that of the protein (Fig. 2). The same conclusions can be obtained when analyzing <x2(Δt)> (see Figs. S5).
Hydration dependence of the anharmonic onset of hydration water. S(q, Δt), for dry D-CYP and D-CYP in H2O at h = 0.2 and 0.4, measured using HFBS neutron instrument with an energy resolution of 1 □eV.
Conclusion and Discussion
By combining elastic neutron scattering with isotopic labelling, we have been able to probe the dynamics of the protein and surface water separately, as a function of temperature, protein structural composition, hydration level and time scale. We found that the anharmonic onsets of the two components around 200 K are clearly decoupled and different in origin. The protein shows an intrinsic transition, whose temperature depends on the structure of the protein and the hydration level, and not on the instrument used to measure it. It has a thermodynamic signature similar to the glass transition in polymers as confirmed by DSC, and thus can be assigned to the freezing of the structural relaxation of the protein beyond the experimental equilibrium time (100 to 1000 s). In contrast, the temperature at which the onset of anharmonicity happens in the hydration water is given by the instrument resolution, independent of both the biomolecular structure and the level of hydration.
Based on our findings, we can infer that, in some cases, the dynamical transition of a protein can coincide with the anharmonic onset of its surface water if one characterizes the system using a single neutron instrument with a fixed resolution. But such coincidence will be torn apart if the measurements were conducted by using instruments of different resolutions or at different amounts of hydration, such as in the present work. This rationalizes the seemingly contradictive results reported in the literature (7,21,25).
The protein dynamical transition has long been thought to connect to the thermal onset of the functionality of the biomolecule. Our experiments suggest that this transition in protein is an intrinsic property of the hydrated protein that its structural relaxation is activated upon heating above the onset temperature. This structural relaxation might be associated with conformational jumps of the biomolecules among different functional states, such as the states with the ligand-binding pocket being opened or closed. Unfreezing of the protein structural relaxation might facilitate these conformational jumps, turning on its functionality. However, as revealed by Ref (48), the denatured form of lysozyme also exhibits a dynamical transition, similar to that seen in its folded native form. Hence, one can argue that the activation of the structural relaxation of the biomolecule above the dynamical transition temperature is a necessary but insufficient condition for the protein to function, as the latter also requires the biomolecule assuming the correctly folded 3-dimensional structure. The findings in this work help further the understanding of the microscopic mechanism governing the dynamics in proteins and their hydration water, as well as their interactions at the cryogenic temperature. More importantly, we demonstrated that the protein dynamical transition is a real transition, connecting to unfreezing of the biomolecular structural relaxation, which could be crucial for activating the function.
Acknowledgements
This work is supported by the National Natural Science Foundation of China (11974239; 62302291), the Innovation Program of Shanghai Municipal Education Commission (2019-01-07-00-02-E00076). H.O’N. and Q.Z. acknowledge the support of Center for Structural Molecular Biology (FWPERKP291) funded by the U.S. Department of Energy (DOE) Office of Biological and Environmental Research. Access to the HFBS was provided by the Center for High-Resolution Neutron Scattering, a partnership between the National Institute of Standards and Technology and the National Science Foundation under Agreement No. DMR-1508249. The neutron experiment at the Materials and Life Science Experimental Facility of the J-PARC was performed under a user program (Proposal No. 2019A0020). We thank STFC for access to neutron scattering facilities at RB1800112. The original data is accessible via data cite: htpps://doi.10.5286/ISIS.E.RB1800112.
References
- 1.The hunting of the SrcNature Reviews Molecular Cell Biology 2:467–475
- 2.Direct Determination of Vibrational Density of States Change on Ligand Binding to a ProteinPhysical Review Letters 93
- 3.Good vibrations in enzyme-catalysed reactionsNature Chemistry 4:161–168
- 4.Protein hydration and functionAdvances in Protein Chemistry 41:37–172
- 5.Solvent mobility and the protein ‘glass’ transitionNature Structural Biology 7:34–38
- 6.Crystalline ribonuclease A loses function below the dynamicaltransition at 220 KNature 357:423–424
- 7.Coincidence of Dynamical Transitions in a Soluble Protein and Its Hydration Water: Direct Measurements by Neutron Scattering and MD SimulationsJournal of the American Chemical Society 130:4586–4587
- 8.Onsets of Anharmonicity in Protein DynamicsPhysical Review Letters 95
- 9.How soft is a protein? A protein dynamics force constant measured by neutron scatteringScience 288:1604–1607
- 10.Dynamical transition of myoglobin revealed by inelastic neutron scatteringNature 337:754–756
- 11.Elastic and Conformational Softness of a Globular ProteinPhysical Review Letters 110
- 12.Physical origin of anharmonic dynamics in proteins: new insights from resolution-dependent neutron scattering on homomeric polypeptidesPhysical Review Letters 109
- 13.Dynamics of ligand binding to myoglobinBiochemistry 14:5355–5373
- 14.Direct Structural Observation of an Acyl-Enzyme Intermediate in the Hydrolysis of an Ester Substrate by ElastaseBiochemistry 33:9285–9293
- 15.Thermal motions and function of bacteriorhodopsin in purple membranes: effects of temperature and hydration studied by neutron scatteringProceedings of the National Academy of Sciences 90:9668–9672
- 16.Slaving: Solvent fluctuations dominate protein dynamics and functionsProceedings of the National Academy of Sciences 99:16047–16051
- 17.A unified model of protein dynamicsProceedings of the National Academy of Sciences 106:5129–5134
- 18.Dynamics and mechanism of ultrafast water–protein interactionsProceedings of the National Academy of Sciences 113:8424–8429
- 19.Direct observation of hierarchical protein dynamicsScience 348:578–581
- 20.Translational Hydration Water Dynamics Drives the Protein Glass TransitionBiophysical Journal 85:1871–1875
- 21.Dynamics of Protein and its Hydration Water: Neutron Scattering Studies on Fully Deuterated GFPBiophysical Journal 103:1566–1575
- 22.Dynamical Transition of Collective Motions in Dry ProteinsPhysical Review Letters 119
- 23.Using polarization analysis to separate the coherent and incoherent scattering from protein samplesBiochimica et Biophysica Acta (BBA) - Proteins and Proteomics 1804:76–82
- 24.de Gennes Narrowing Describes the Relative Motion of Protein DomainsPhysical Review Letters 112
- 25.Low-Temperature Decoupling of Water and Protein Dynamics Measured by Neutron ScatteringThe Journal of Physical Chemistry Letters 8:4883–4886
- 26.Influence of Hydration on the Dynamics of LysozymeBiophysical Journal 91:2573–2588
- 27.Translational diffusion of hydration water correlates with functional motions in folded and intrinsically disordered proteinsNature Communications 6
- 28.Surface Hydration Amplifies Single-Well Protein Atom Diffusion Propagating into the Macromolecular CorePhysical Review Letters 108
- 29.Direct Experimental Characterization of Contributions from Self-Motion of Hydrogen and from Interatomic Motion of Heavy Atoms to Protein AnharmonicityThe Journal of Physical Chemistry B 122:9956–9961
- 30.Coupling of protein and hydration-water dynamics in biological membranesProceedings of the National Academy of Sciences 104:18049–18054
- 31.Interactions of Hydration Water and Biological Membranes Studied by Neutron ScatteringThe Journal of Physical Chemistry B 103:8036–8050
- 32.Why the fast relaxation in the picosecond to nanosecond time range can sense the glass transitionPhilosophical Magazine 84:1341–1353
- 33.The microscopic basis of the glass transition in polymers from neutron scattering studiesScience 267:1939–1945
- 34.Boson peak and fast relaxation process near the glass transition in polystyreneColloid and Polymer Science 273:413–420
- 35.Glass Transition Behavior of a Microphase Segregated Polyurethane Based on PFPE and IPDI. A Calorimetric StudyMacromolecules 36:8015–8023
- 36.Salt-Concentration Dependence of the Glass Transition Temperature in PEO–NaI and PEO–LiTFSI Polymer ElectrolytesMacromolecules 46:8580–8588
- 37.The protein glass transition as measured by dielectric spectroscopy and differential scanning calorimetryBiochimica et Biophysica Acta (BBA) - Proteins and Proteomics 1804:20–26
- 38.Change of caged dynamics at Tg in hydrated proteins: Trend of mean squared displacements after correcting for the methyl-group rotation contributionThe Journal of Chemical Physics 138
- 39.Dynamics of tRNA at Different Levels of HydrationBiophysical Journal 96:2755–2762
- 40.Hydration-Dependent Dynamical Modes in Xyloglucan from Molecular Dynamics Simulation of 13C NMR Relaxation Times and Their DistributionsBiomacromolecules 19:2567–2579
- 41.The physico-chemical characterization of poly (2-hydroxyethyl methacrylate-co-methacrylic acid: 2. Effect of water, PEG 400 and PEG 6000 on the glass transition temperaturePolymer 30:1946–1950
- 42.Water absorption in EVOH films and its influence on glass transition temperatureJournal of Polymer Science Part B: Polymer Physics 37:691–699
- 43.Dielectric Investigation of the Low-Temperature Water Dynamics in the Poly(vinyl methyl ether)/H2O SystemMacromolecules 38:7056–7063
- 44.Direct Evidence of the Amino Acid Side Chain and Backbone Contributions to Protein AnharmonicityJournal of the American Chemical Society 132:1371–1376
- 45.Conductivity in Hydrated Proteins: No Signs of the Fragile-to-Strong CrossoverPhysical Review Letters 100
- 46.Influence of Hydration on Protein Dynamics: Combining Dielectric and Neutron Scattering Spectroscopy DataThe Journal of Physical Chemistry B 112:14273–14280
- 47.Dynamical Transition of Protein-Hydration WaterPhysical Review Letters 104
- 48.Mean-squared atomic displacements in hydrated lysozyme, native and denaturedJournal of biological physics 36:291–297
- 49.ASTM International
Metrics
- views
- 53
- download
- 1
- citations
- 0
Views, downloads and citations are aggregated across all versions of this paper published by eLife.
