Human α-Synuclein (αSyn) is a natively unfolded protein whose aggregation into amyloid fibrils is involved in the pathology of Parkinson disease. A full comprehension of the structure and dynamics of early intermediates leading to the aggregated states is an unsolved problem of essential importance to researchers attempting to decipher the molecular mechanisms of αSyn aggregation and formation of fibrils. Traditional bulk techniques used so far to solve this problem point to a direct correlation between αSyn's unique conformational properties and its propensity to aggregate, but these techniques can only provide ensemble-averaged information for monomers and oligomers alike. They therefore cannot characterize the full complexity of the conformational equilibria that trigger the aggregation process. We applied atomic force microscopy–based single-molecule mechanical unfolding methodology to study the conformational equilibrium of human wild-type and mutant αSyn. The conformational heterogeneity of monomeric αSyn was characterized at the single-molecule level. Three main classes of conformations, including disordered and “β-like” structures, were directly observed and quantified without any interference from oligomeric soluble forms. The relative abundance of the “β-like” structures significantly increased in different conditions promoting the aggregation of αSyn: the presence of Cu2+, the pathogenic A30P mutation, and high ionic strength. This methodology can explore the full conformational space of a protein at the single-molecule level, detecting even poorly populated conformers and measuring their distribution in a variety of biologically important conditions. To the best of our knowledge, we present for the first time evidence of a conformational equilibrium that controls the population of a specific class of monomeric αSyn conformers, positively correlated with conditions known to promote the formation of aggregates. A new tool is thus made available to test directly the influence of mutations and pharmacological strategies on the conformational equilibrium of monomeric αSyn.
Natively unstructured proteins defy the classical “one sequence–one structure” paradigm of protein science. In pathological conditions, monomers of these proteins can aggregate in the cell, a process that underlies neurodegenerative diseases such as Alzheimer and Parkinson. A key step in the aggregation process—the formation of misfolded intermediates—remains obscure. To shed light on this process, we characterized the folding and conformational diversity of αSyn, a natively unstructured protein involved in Parkinson disease, by mechanically stretching single molecules of this protein and recording their mechanical properties. These experiments permitted us to observe directly and quantify three main classes of conformations that, under in vitro physiological conditions, exist simultaneously in the αSyn sample. We found that one class of conformations, “β-like” structures, is directly related to αSyn aggregation. In fact, their relative abundance increases drastically in three different conditions known to promote the formation of αSyn fibrils. We expect that a critical concentration of αSyn with a “β-like” structure must be reached to trigger fibril formation. This critical concentration is therefore controlled by a chemical equilibrium. Novel pharmacological strategies can now be tailored to act upstream, before the aggregation process ensues, by targeting this equilibrium. To this end, single-molecule force spectroscopy can be an effective tool to tailor and test new pharmacological agents.
Citation: Sandal M, Valle F, Tessari I, Mammi S, Bergantino E, et al. (2008) Conformational Equilibria in Monomeric α-Synuclein at the Single-Molecule Level. PLoS Biol 6(1): e6. doi:10.1371/journal.pbio.0060006
Academic Editor: Gregory A. Petsko, Brandeis University, United States of America
Received: June 6, 2007; Accepted: November 26, 2007; Published: January 15, 2008
Copyright: © 2008 Sandal et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: This work was supported by Ministero dell'Università e della Ricerca–Fondo per gli Investimenti della Ricerca di Base (MIUR-FIRB) RBNE03PX83/001; MIUR-FIRB Progetto NG-lab (G.U. 29/07/05 n.175); Progetti di Ricerca di Interesse Nazionale (PRIN) 2006 (Prot. 2006034199), EU FP6-STREP program NMP4-CT-2004–013775 NUCAN. LB is supported also by PRIN 2005 and FIRB Progetto RBNE03PX83/006.
Competing interests: The authors have declared that no competing interests exist.
Abbreviations: aa, amino acid; AFM, atomic force microscopy; αSyn, α-synuclein; CD, circular dichroism; FTIR, Fourier transform infrared; NUP, natively unfolded protein; PBS, phosphate buffered saline; SDS, sodium dodecyl-sulfate; SMFS, single-molecule force spectroscopy; WLC, worm-like chain
A significant fraction (possibly as much as 30%) of proteins and segments of proteins in eukaryotic proteomes has been found to lack, at least partially, a well-defined three-dimensional structure. Proteins belonging to this class are usually called natively unfolded proteins (NUPs) . NUPs have been found to play key roles in a wide range of biological processes like transcriptional and translational regulation, signal transduction, protein phosphorylation, and the folding of RNA and other proteins . The conformational heterogeneity of NUPs allows them to adopt conformations that trigger pathogenic aggregation processes. In fact, NUPs are involved in the pathogenesis of some of the most widespread and socially relevant neurodegenerative diseases, such as Alzheimer and Parkinson [3–5]. Despite intensive research, the folding and the aggregation mechanisms of NUPs remain a major unsolved problem.
Theoretical studies depict the apparent structural disorder of NUPs as the result of the coexistence of a complex ensemble of conformers ensuing from a rugged energy landscape . Five clusters of conformations, each with its own characteristic tertiary structure, were identified by molecular dynamics studies on the Alzheimer β peptide . Traditional bulk experiments and spectroscopies have recently been providing experimental evidence of the conformational diversity of these proteins [3,5]. Because of their inherent ensemble averaging, however, these methodologies cannot reveal the full complexity of the conformational equilibria of NUPs. Single-molecule methodologies can single out the structures adopted by individual molecules within a complex conformational equilibrium [8–14].
We decided to approach the problem of the characterization of the conformers of α-synuclein (αSyn), which is a prototype of this class of proteins. αSyn is a 140–amino acid (aa) protein expressed primarily at the presynaptic terminals in the central nervous system, and it is thought to be physiologically involved in endoplasmic reticulum–Golgi vesicle trafficking . αSyn is involved in the pathogenesis of several neurodegenerative diseases, called synucleopathies. Intracellular proteinaceous aggregates (Lewy bodies and Lewy neurites) of αSyn are hallmarks of Parkinson disease  and multiple system atrophy . Three naturally occurring mutations in the αSyn protein sequence—A30P, A53T, and E46K—have been identified so far in human families affected by familial Parkinsonism [18–20]. These mutant proteins display an increased tendency to form nonfibrillar aggregates  and Lewy bodies–like fibrils in vitro .
The fibrils spontaneously formed by αSyn by a nucleation-dependent mechanism are rich in β structure [23,24]. The transition from the natively unfolded monomeric state to fibril is therefore a process of acquiring structure. This process is still under strong debate. Evidence is accumulating that the monomeric αSyn, under in vitro physiological conditions, populates an ensemble of conformations including extended conformers and structures that are more compact than expected for a completely unfolded chain [25–32]. The marked differences between the scenarios depicted in those studies are mostly determined by the different time scales of the ensemble averaging of the different methods used. Moreover, it is difficult for bulk methodologies to single out the monomeric state in the presence of soluble oligomers when they form quickly in solution . On the contrary, the single-molecule force spectroscopy (SMFS) approach reported here describes, by design, the conformational equilibrium of the monomeric form.
The different structures assumed by αSyn have been commonly investigated by adding to its buffer solution different chemicals, such as methanol or trifluoroethanol , metal cations like Cu2+ and Al3+ [35,36], or sodium dodecyl-sulfate (SDS) micelles [37–39] in order to shift the conformational equilibrium toward the form under investigation. A previous force spectroscopy experiment showed that a relevant 12-aa segment of αSyn is conformationally heterogeneous . The approach we report can span the full conformational space of the whole protein and also identify poorly populated conformers of the monomeric αSyn in in vitro physiological conditions. Three distinct classes of structures in equilibrium were identified: random coil, a mechanically weak fold, and “β-like.” Their populations were also monitored under conditions known to influence aggregation, such as the presence of Cu2+, high buffer concentration and, most importantly, the pathogenic mutation A30P.
To stretch an individual αSyn molecule by AFM, we need handles to connect one end of the protein to the tip and the other to the substrate. To this aim, we followed the design proposed by J. Fernandez for the study of the random coiled titin N2B segment . A chimeric polyprotein composed of a single αSyn module flanked on either side by three tandem I27 domains (Figure 1A, 3S3) was expressed [42–44]. These domains act as molecular handles to mechanically stretch a single αSyn molecule. They also introduce well-characterized fingerprint signals into the recorded force curves that make it possible to identify the different αSyn conformations. The design is such that if the number of unfolding signals coming from I27 modules is larger than four, we are sure to have also mechanically stretched the αSyn module in the middle (Figure 1A). Among the curves showing mechanical unfolding events, however, only those featuring at least six unfolding peaks were selected and analyzed. This choice reduced the statistical sample even more, but it allowed us to recognize, in a very stringent way, the signatures of the different conformations of the αSyn moiety on each construct molecule that had been stretched.
Figure 1. The Mechanical Signatures of αSyn Conformational Classes as Recorded by SMFS
(A) Schematic representation of the polyprotein constructs used in this work: 3S3 contains the αSyn sequence (red) flanked on either side by three titin I27 modules (blue), the N-terminal His-tag needed for purification purposes (green), and the C-terminal Cys-Cys tail needed for covalent attachment to the gold surface (yellow). In 1S1, the αSyn moiety is flanked only by one I27 on both sides; the 3T is made up by three I27s. In the αSyn moiety (enlarged), three regions are shown: (i) the amphipathic region, prone to fold in α-helical structures when in contact with phospholipid membranes; (ii) the fibrillogenic NAC region, characteristic of the fibril core of αSyn amyloid; and (iii) the acidic C-terminal tail, strongly charged and not prone to fold. The positions of alanine 30, site of the A30P mutation and histidine 50, which is crucial for the binding of Cu2+, are marked.
(B) Example of curve characterized by a featureless region assigned to the stretching of αSyn moiety having, in this case, the mechanical properties of a random coil (see Results section). This region is followed (from left to right) by six unfolding peaks of about 200 pN, with about 28-nm gaps between each, assigned to the unfolding of I27 domains.
(C) Example of the curves featuring the β-like signature of αSyn (see Results section), showing seven practically indistinguishable unfolding events of similar magnitude and spacing.
(D) Curves featuring the signature of mechanically weak interactions, showing single or multiple small peaks (arrows) superimposed on the purely entropic WLC behavior of the trace preceding the six saw-tooth–like peaks. The right panels show a zoom of the region enclosed by the dashed squares.doi:10.1371/journal.pbio.0060006.g001
To probe the native-like conformer population of αSyn, we performed experiments in a 10 mM Tris buffer solution. We found that the profiles of the selected force curves can be classified into three main classes. Two were unambiguously assigned to well-defined classes of conformers: one with the typical mechanical behavior of random-coil chains and the other of β-like structures. We propose that the profiles of the third class correspond to fairly compact architectures, likely to be sustained also by interactions among different modules of the construct.
The Signature of Disordered Conformers of αSyn with the Mechanical Behavior of an Entropic Random Coil
In the class of traces depicted in Figure 1B, the force curve exhibits (from left to right) a long initial region, without any significant deviation from the worm-like chain (WLC) behavior , followed by a saw-tooth pattern with six consecutive unfolding events, in addition to the last one that corresponds to the final detachment of the molecule from the tip. The initial region corresponds to the extension of a chain that occurs at low force and without significant energy barriers limiting its extensibility.
The six unfolding peaks are spaced by ~28 nm. This spacing between the peaks corresponds to an 89-aa chain (0.36 nm per amino acid ), i.e., to the increase in length of the protein after the unfolding of one I27 domain. These six unfolding peaks correspond to the characteristic fingerprint of the mechanical unfolding of the I27 modules . We can therefore infer that, in this case, the AFM tip picked up the 3S3 construct molecules at the His-tag terminus, while the other end was tethered to the gold surface by the C-terminal cysteines.
The location of the first unfolding peak of I27, corresponding to the contour length of the construct molecules prior to any unfolding event, proves that the preceding featureless part of the trace can be unambiguously assigned to the αSyn chain. In fact, the measured contour length that fits this peak is 77 ± 4 nm. Subtracting the length of the six, still folded, I27 domains from this value (4.5 nm each ), a value of 48 ± 4 nm is obtained. This length corresponds to the chain of 140 aa of the αSyn. Therefore, this featureless initial part is the signature of αSyn conformers with the mechanical properties of a random coil. Their average persistence length was estimated by fitting the WLC model at 0.36 ± 0.05 nm. About 38% of the molecules showed this mechanical behavior in Tris/HCl buffer 10 mM (Figure 2).
Figure 2. Population Shift of αSyn Conformers in Different Conditions
Population of αSyn conformers in the four different conditions tested in the present work. Percentages observed for each curve type (see Figure 1) at 10 mM Tris/HCl (n = 55), 10 mM Tris/HCl with 1 μM Cu2+ (n = 34), the A30P mutant in 10 mM Tris/HCl (n = 56), and 500 mM Tris/HCl (n = 61).doi:10.1371/journal.pbio.0060006.g002
The Signature of αSyn Conformers with the Mechanical Behavior of a Chain Containing a β-Like Structured Segment
A significant proportion of force curves with seven regularly spaced unfolding peaks in the 200-pN range (in addition to the last one corresponding to the final detachment) (Figure 1C) was also recorded.
The presence of a number of unfolding events greater than that of the I27 modules in the construct cannot be ascribed to a possible simultaneous pulling of more than one 3S3 molecule, because pulling two multidomain constructs at the same time would not likely lead to a uniform separation between the I27 unfolding events. Moreover, we never obtained a significant and uniform set of reproducible curves with eight or more unfolding peaks with 28-nm separation. Curves with seven unfolding events were well reproducible, and their statistics were unambiguously modulated by conditions able to trigger aggregation: e.g., ionic strength, the presence of Cu2+ ions and, most importantly, pathogenic mutations (see below). The appearance of seven unfolding events cannot come from a construct accidentally expressed with seven, instead of six, I27 domains because of the cloning strategy (see Materials and Methods). The occurrence of a seventh peak due to the stretching of 3S3 dimers can be also ruled out. Dimers could form in solution via disulfide bonds between the terminal cysteines, but those bonds tend to dissociate into thiols in the presence of gold, because the gold–sulfur bond is more stable than the sulfur–sulfur bond . Each monomer contains two terminal cysteines: one of them could be involved in the dimerization and the other could bind to the gold surface. Even in this unlikely event, the length of the tethered chains extending from the surface is the same as that of a nondimerized construct. Therefore, also in the case of a dimer tethered to the surface, more than six I27 unfolding peaks with the same separation cannot be recorded. We nevertheless tested the sample using dithiothreitol (DTT) to avoid any disulfide-bonded dimer formation. Under these conditions, the statistics of different populations was comparable to those in the standard buffer, and we still recorded a significant proportion (~10%) of seven-peaked curves.
Because of the previous considerations, we therefore assign one of the seven peaks to the unfolding of the αSyn moiety. The length (95 aa) of this αSyn β-like folded section accidentally coincides with that of the I27 domain. This coincidence hinders the possibility to discriminate the peak of the αSyn from the six of the I27 domains. Nevertheless, the assignment of these curves to the unfolding of the αSyn moiety is confirmed by the position of the first unfolding peak, i.e., by the contour length of the construct molecules prior to any unfolding event. As shown in Figure 3, the position values correspond to a chain composed of the six I27 folded modules, plus the αSyn moiety with its C-terminal segment of 50 aa fully unfolded, and the remaining 95 amino acids folded into a structure with the same contour length as a folded I27 domain (solid line). The low propensity to fold of the 50 aa of the very acidic αSyn C-terminal tail has been extensively documented [38,39,49]. Segments of the remaining 95 amino acids are instead known to fold under different conditions into an α helix [38,39] or, in the amyloid, into a β sheet structure . It must be noted that in about 40% of the molecules, the contour length of the same folded section is larger than that corresponding to 95 aa. The αSyn structural diversity therefore includes also β-like chain portions with different lengths. This interpretation is confirmed by comparing the variance of the folded section of seven-peaked curves with that of I27 modules (Figure 3).
Figure 3. Contour Length Analysis of β-Like Force Curves
Values of the first peak position in force curves showing seven unfolding peaks. The height of each bar corresponds to the initial contour length of a single curve, obtained by fitting the first unfolding peak by means of the WLC model. The dashed line is the length corresponding to a protein construct with six I27 folded modules plus 95 aa of αSyn folded into a β-like structure, and the remaining 50 aa of αSyn unstructured (see Discussion section). The dashed-and-dotted line is the length corresponding to a protein construct with six I27 modules plus the 140 aa of αSyn completely unstructured. The lengths of twelve randomly chosen I27 modules have also been reported (dark gray columns) for comparison. The solid line is the nominal I27 contour length. The larger spreading of the αSyn data confirms the higher conformational heterogeneity. Side quotas show the difference between the maximum and minum observed length value for I27 (bottom) and β-like structures (top).doi:10.1371/journal.pbio.0060006.g003
The 200-pN unfolding force of all the seven peaks indicates that the folded section of αSyn has the same mechanical properties of the I27 β-sandwich structure. At the moment, without any independent structural characterization, we consider and label this folded structure of the αSyn moiety just as β-like, in accordance with its mechanical behavior. Nevertheless, its mechanical behavior is in agreement with a β sheet content in the β-like class of conformers. It is unlikely that the α-helical content we observed by means of circular dichroism (CD) (see below) correlates with the “β-like” conformers. In fact, whereas β-structures, like those of titin modules, such as I27 [41,50], or tenascin , unfold at forces in the range of 100–300 pN (at loading rates of the order of 10−5 N/s), the α helix domains, in the same conditions, are always observed to unfold at forces almost one order of magnitude smaller [52–55].
In conclusion, these curve profiles provide clear evidence that in 10 mM Tris/HCl buffer, about 7% of the molecules (Figure 2) contain a segment of the αSyn chain of about 95 aa folded into a structure with the mechanical property of the I27 β-sandwich structure. This percentage of the β-like structures, as we will see below, can be related with conditions leading to pathogenic aggregation.
Signatures of Further Conformational Complexity Probed as Mechanically Weak Interactions
The remaining force spectroscopy curves (Figure 1D) show single or multiple small peaks (sometimes with a plateau- or dome-like appearance) superimposed on the purely entropic WLC behavior of the trace preceding the six saw-tooth–like peaks.
The geometry of our construct made it possible to exclude that those small peaks might correspond to the rupture of aspecific αSyn-gold interactions. In fact, if the unstructured αSyn was adsorbed on the surface, upon pulling the construct, we would have recorded the first event at a distance from the tip contact point corresponding to the length of the three I27 modules (~13.5 nm). The mechanically weak events we observed instead took place at an average distance from the contact point of 60 ± 26 nm with no events below 20 nm. They are therefore not compatible with αSyn-gold interactions. We assign these signals to the rupture of mechanically weak interactions placed at short and long distances along the chain.
The average forces of those single or multiple small peaks of the profiles are in the 64 ± 30–pN range (well above the noise level), without a defined hierarchy; often stronger peaks precede weaker ones, hinting topologically “nested” interactions. From the difference between the contour length estimated at those small peaks and that at the first I27 unfolding peak, one can measure the size of the topological loop enclosed by the interactions whose rupture is monitored by the different peaks. The resulting broad distribution of these distances monitors the ample multiplicity of these interactions as discussed in Protocol S1.
More than 50% of the molecules showed short- and long-distance mechanically weak interactions in 10 mM Tris/HCl buffer (Figure 2). These interactions were also monitored by ensemble-averaged fluorescence spectroscopy. The fluorescence comes from the tryptophan residues of the I27 domains which are absent in αSyn. The fluorescence spectra reported in Figure 4A prove that interactions between the I27 handles and tracts of the αSyn moiety do take place, as shown by the broadening of the spectrum of 1S1 with respect to that of the 3T construct (See Figure 1A and Materials and Methods section for constructs description) and by the 5-nm shift of the λmax. The possibility of partial I27 unfolding leading to Trp exposure and broadening of the spectrum is ruled out by the CD data and by our force curves, which show that I27 domains are as tightly folded in the 3S3 construct as in an I27 homopolymer. A broadening due to subtle conformational effects on the I27 domain that expose the I27 Trp residue is possible, but even in this case, the fact that this broadening happens only when the αSyn moiety is inserted in the construct proves that direct interaction is taking place.
Figure 4. Circular Dichroism and Fluorescence Spectroscopy
(A) Fluorescence spectra of αSyn, 3T, and 1S1 (dotted, dashed, and solid line, respectively).
(B) Circular dichroism spectra in PBS buffer of 3T, 1S1 (solid lines). The αSyn contribution in 1S1 (dashed line) is calculated by subtracting the relative contribution of the I27 domains from the CD spectrum of 1S1.
(C) CD spectra of αSyn in PBS (solid line) and 250 mM SDS (dotted line). The αSyn contribution in 1S1 (dashed line) is reported as in (B).doi:10.1371/journal.pbio.0060006.g004
CD spectra of 1S1 and 3T were recorded in which 1S1 shows some α-helical content in the αSyn moiety (Figure 4B). . Subtraction of the contribution of the I27 linkers (2/3 of the CD of 3T recorded in the same 10 mM Tris/HCl buffer) from the CD spectrum of 1S1 reveals a profile that is different from that of αSyn in the same buffer condition (Figure 4C) but similar to that of the same protein in the α helix structure induced by the addition of SDS . This α-helical content might be induced by the interactions between the αSyn moiety and the I27 domains as discussed below and in Protocol S1.
Low Concentrations of Cu2+ Affect the Conformational Equilibrium of αSyn
It is well known that multivalent metal cations like Cu2+ can accelerate αSyn aggregation [35,36]. To validate our approach and to investigate how metal cations influence the conformer equilibrium of αSyn, we performed SMFS experiments on the 3S3 construct in 10 mM Tris/HCl buffer in the presence of 1 μM CuCl2. The low concentration of copper was chosen to target the His 50 specific copper binding site of αSyn (dissociation constant Kd = 0.1 μM) .
The presence of 1-μM Cu2+ moderately, but significantly (χ2 statistical significance p < 0.01), alters the relative distribution of the αSyn conformers with respect to plain 10 mM Tris/HCl (see Figure 2). In particular, the relative population of the β-like conformers more than doubles (from 7.2% to almost 18%), with a parallel decrease of the signals coming from mechanically weak interactions. An increase (from 38% to 47%) of random coil-like curves is also observed.
The Conformational Equilibrium of the Pathological A30P αSyn Mutant Is Drastically Shifted Toward the β-Like Conformers
The A30P mutation is a pathogenic, naturally occurring human αSyn variant, that correlates with familial Parkinsonism . The mutant protein displays an increased rate of oligomerization  and impaired degradation by chaperone-mediated autophagy . We tested the 3S3 αSyn-A30P construct to evaluate the capability of our methodology to probe different conformational propensities in mutants of the same protein. We found that the A30P mutation induces a striking shift in the conformational equilibrium of αSyn with β-like curves being around 37% of the sample and again, a corresponding decrease of signals coming from mechanically weak interactions (Figure 2). In contrast with wild-type αSyn incubated with Cu2+, the A30P mutant does not induce an increase of random coil curves that are exactly in the same proportion observed in wild-type αSyn.
The Relative Population of the Three Classes of Conformers Is Modified by the Buffer Concentration
Another condition known to speed up αSyn aggregation is high ionic strength [26,28]. SMFS experiments on the 3S3 wild type construct were performed also in 500 mM Tris/HCl buffer. As reported in Figure 2, the frequency of the three types of profiles radically changed in different ionic strength conditions. The most remarkable result is, again, the significant increase in the population of the β-like structures with buffer concentration (up to about 28%) and the parallel decrease of the percentage of the mechanically weak structures. An increase of random coil curves is also observed, as occurs in the presence of Cu2+, but unlike the case of the A30P mutant.
We have identified the signatures of three classes of conformers in monomeric αSyn at the single-molecule level. One of these classes includes structures that are mechanically indistinguishable from a random coil; the other two classes include β-like structures and structures kept together by short- and long-distance mechanically weak interactions (Figure 1). We have also observed that their equilibrium shifts significantly depending on solution conditions or sequence variants related to pathological aggregation. The important result that emerges from these data is the direct correlation between conditions known to increase the αSyn aggregation propensity and the relative size of the β-like population (Figure 2).
The β-Like Conformers Are Structured Conformations Directly Related to the Aggregation Propensity
We observed a marked increase of the population of “β-like” conformers under three very different conditions known to accelerate αSyn aggregation. This result links the population of those αSyn monomeric conformers to the process of αSyn aggregation. The first condition is the presence of a μM concentration of Cu2+. Our results in this condition agree with the observation of a metal-induced partially folded intermediate by Uversky, Li, and Fink . Also Rasia et al. suggested a compact set of metal-induced conformations, noticing that the specific binding of Cu2+ to the αSyn N terminus requires the formation of a metal-binding interface (pivoted on His 50), which possibly involves residues that are widely separated in the primary amino acid sequence .
The second condition is the A30P mutation. Nuclear magnetic resonance (NMR) experiments have observed a much more flexible average conformation of the αSyn mutants A30P and A53T. The increased average flexibility of αSyn allows the protein to sample a larger conformational space. . Interestingly, the mean hydrodynamic radius of αSyn is not affected by the A30P and A53T mutations [21,59], thus showing that the increased flexibility is compatible with the population of compact folded structures like those singled out by our experiments.
The third condition is a radical increase of the ionic strength. Our results in 500 mM Tris/HCl can be reconciled with the model proposed by Hoyer et al.  and by Bernado et al.  to explain the well-documented phenomenon of the increased αSyn fibril formation with increasing ionic strength. According to that model, the increased fibril formation is explained just on the basis on an increased freedom of the fibrillogenic NAC region caused by the release of its interaction with the negatively charged C-terminal tail. The increased ionic strength of the buffer leads to a more efficient charge shielding of the strongly acidic C-terminal tail, thus relieving its electrostatic self-repulsion. This in turn leads to the lowering of the protein-excluded volume and increases its flexibility. According to our data in Figure 2, we should add to this model a shift of the conformational equilibrium toward the β-like structures that takes place on increasing the charge shielding.
Are β-like structures really β?
Any assignment of force spectroscopy signals to a definite secondary canonical structure must be supported by independent structural data. We have labeled as β-like those conformers with a mechanical behavior closely matching those of structures rich in β sheets. The correlation of the population of these structures with aggregation conditions, which enrich β sheet content in αSyn, supports this labeling. Evidence of some β sheet content in the monomeric state of αSyn was previously reported in the literature. Most recently by means of NMR spectroscopy in supercooled water at minus 15 °C, it was found that the αSyn chain, cold-denatured to an hydrodynamic radius equivalent to that displayed by the same protein in 8-M urea, retains a surprising amount of unpacked β strand content that correlates with the amyloid fibril β structure . The packing of these β strands into compact structures like those observed by us is thus likely to occur in nondenaturing conditions and at physiological temperatures. This NMR result supports our observation of β-like conformers in the monomeric state of αSyn and links them to the amyloid β structure. The presence of β sheet structures was indicated also by Raman spectra of this protein in aqueous solution. In the same investigation, CD spectroscopy proved unable to detect any β content. Correspondingly, the CD spectra of αSyn recorded by us in 10 mM and 500 mM Tris were practically superimposable. We conclude that CD is not a technique sensitive enough to detect partial β-sheet content in the αSyn sample. A fraction of β-sheet/extended structure of about 19% was also detected, again not by CD, but by Fourier transform infrared (FTIR) spectroscopy in dried films of αSyn . This fraction is much larger than that estimated by our experiments in 10 mM Tris/HCl buffer (see Figure 2). However, the conditions of the SMFS and FTIR experiments were markedly different, and in the latter case, some template-mediated formation of β structures due to the packing of the αSyn molecules in the dried films required by the FTIR measurements cannot be ruled out.
In conclusion, despite the fact that force spectroscopy data cannot directly assign a specific secondary structure to the conformers we have labeled as β-like, it is most likely that they have significant β sheet content.
The Mechanically Weak Interactions Can Be Both within the αSyn Moiety and between αSyn and the I27 Domains
By now, any structural characterization of the mechanically weak interactions events monitored by the small peaks in force curves as in Figure 1D (right panels) is at best tentative and falls outside the focus of the present work. A more detailed characterization of these events is, however, within the range of capabilities of the techniques proposed here and is being currently addressed in our laboratory (see Protocol S1 for preliminary measurements). A plausible explanation of the short- and long-distance mechanically weak interactions we observed cannot exclude the interaction between positively charged residues on the αSyn N terminal and the negatively charged surface of I27 modules . It has been documented that αSyn in contact with negatively charged surfaces assumes an α helix structure [37–39,62,63]. We might expect a similar structural transition in the αSyn moiety also from the contact with the I27 modules within the 3S3 or 1S1 constructs (see Protocol S1). This transition is indicated by the CD spectra of the 1S1 construct in 10 mM Tris/HCl (see Figure 4B). We propose that the small peaks like those shown in Figure 1D and assigned to the mechanically weak interactions can be the signature of the interaction between αSyn, possibly in α helical form, and the flanking I27 modules. It is not surprising that more than one of those signals are present in the same force curves, because multiple interactions of this type can occur at the same time in the same molecule. It should be noted that the same transition does not take place when free αSyn is mixed in solution with I27 modules of the 3T construct (see Protocol S1). An electrostatic model, based on the interaction lengths calculated from the positions of the small peaks in the force curves like those displayed in Figure 1D (right panels), is proposed in Protocol S1.
Notably, these short- and long-distance mechanically weak interactions are observed to be in equilibrium with the β-like structures. The population of the former always decreases while that of the latter increases. This result is in accord with the observation by Zhu et al. that a driving force to α helical structures inhibits αSyn fibril formation  and also rule out any template-mediated β sheet imprinting by the I27 linkers. This conclusion is confirmed by the data on 500 mM Tris/HCl buffered solutions showing that when electrostatic interactions between the αSyn moiety and the flanking I27 linkers are decreased, the population of β-like conformers increase. We can also expect entropic effects due to the presence of the flanking I27 domains to drive the protein toward more extended conformations rather than compact conformations [64,65].
These considerations indicate that the design and use of alternative linkers or experimental strategies may prove useful in the future to further discriminate the effective conformational distribution of αSyn from alterations due to the interaction with the linkers.
For the first time, to our knowledge, we applied the AFM-based single-molecule mechanical unfolding methodology to a multimodular protein containing the αSyn moiety. This approach brings into play three main methodological capabilities inaccessible to the bulk ensemble–averaged spectroscopies previously applied to study the structure of αSyn and other natively unstructured proteins.
The first is the possibility to work strictly at the single-molecule level, thus ensuring that the conformer distribution of the monomeric αSyn is detected and quantified without interference from oligomeric soluble forms of the protein and therefore of any possible intermolecular imprinting toward the amyloidogenic β structures.
The second capability is that of spanning the conformational space of the protein under investigation and of directly catching and quantifying all of its conformers with a lifetime longer than 10−3 s. These conformers, because of their longer life time, might be the most biologically relevant. Three classes of the monomeric αSyn conformations, including random coil, mechanically weakly folded and β-like, were characterized by our experiments. They could be detected even in low concentration without the necessity of selectively enhancing one of them by adding specific agents to unbalance the conformational equilibrium, as most commonly done so far with bulk ensemble–averaged experiments.
The third capability is that of following shifts in the population of these classes of conformers in response to changing the solution conditions or the protein sequence and to detect them even if scarcely populated. In the case of αSyn, conditions known to promote oligomerization and aggregation—like the presence of Cu2+, the A30P mutation, or a radical increase of ionic strength—markedly shift its conformational equilibrium toward the β-like form at the expense of other structures. These results indicate that the β-like curves contain the signature of the structural precursor to αSyn oligomerization. We suggest that the different aggregation propensities and, ultimately, the pathogenicity displayed by αSyn under different environmental conditions or point mutations can be triggered by unbalancing the delicate equilibria among αSyn conformers.
These capabilities suggest that in the near future, single-molecule methodologies will play a crucial role in studies of the folding equilibria of the NUP monomers and, in particular, in the detection and quantification of the conformers that can lead to aggregation of those proteins. Our results suggest the feasibility of single-molecule approaches to the testing of novel pharmacological or biophysical therapies for pathologies involving the conformational equilibria of NUPs.
Materials and Methods
Polyprotein design and expression.
We followed the protein construct design proposed by J. Fernandez for the study of the random coiled titin N2B segment . Chimeric polyproteins were obtained starting from pAFM1–4, pAFM5–8, and pAFM(I27)3mer vectors, kindly provided by Professor Jane Clarke (Cambridge University, United Kingdom) and constructed according to . αSyn or its A30P mutated sequences were amplified by PCR using two different pairs of primers, each containing unique restriction sites. A first pair contained KpnI and XbaI sites, and a second one contained SacI and BssHII sites. The original eight I27 module plasmid was reconstituted from pAFM1–4 and pAFM5–8, obtaining the pAFM8m vector. pAFM8m was then digested with KpnI and XbaI and ligated to the amplified αSyn sequence, then cleaved by the same enzymes in substitution of the two central titin modules to give the pAFM3s3 vector (see Protocol S1). By a similar strategy, the pAFM(I27)3mer vector was digested with SacI and BssHII, and the central titin module replaced by αSyn sequence, obtaining the pAFM1s1 vector. The obtained expression plasmids, pAFM3s3 and pAFM1s1, code for two chimeric polyproteins composed of a single αSyn module flanked on either side by three tandem I27 domains or by just one, named 3S3 and 1S1, respectively. The two pAFM8m and pAFM(I27)3mer vectors (coding for two recombinant poly(I27) proteins named 8T and 3T) were transformed into Escherichia coli C41(DE3) cells  (obtained from Professor John E. Walker [Medical Research Council–Dunn Human Nutrition Unit, Cambridge, United Kingdom] with the agreement of the Medical Research Council center of Cambridge). The cells were grown and the expression of proteins was induced as described in . Recombinant proteins were purified by Ni2+-affinity chromatography in 20 mM sodium phosphate buffer pH 8, 500 mM NaCl; the elution from the resin was obtained with 20 mM imidazole. After dialysis, proteins were kept at −80 °C in phosphate buffered saline (PBS) with 15% glycerol. The purification gel is shown in Protocol S1.
CD measurements were carried out on a JASCO J-715 spectropolarimeter interfaced with a personal computer. The CD spectra were acquired and processed using the J-700 program for Windows. All experiments were carried out at room temperature using HELLMA quartz cells with Suprasil windows and an optical path length of 0.1 cm. Spectra were recorded in the 190–260 nm wavelength range using a bandwidth of 2 nm and a time constant of 2 s at a scan speed of 50 nm/min. The signal-to-noise ratio was improved by accumulating at least four scans. All spectra are reported in terms of mean residue molar ellipticity [Θ]R (deg cm2 dmol−1).
Fluorescence emission spectra were recorded on a Perkin-Elmer LS 50 spectrofluorimeter equipped with a thermostated cell compartment and interfaced with a personal computer using the FL-WinLab program for Windows. Sample measurements were carried out using a HELLMA ultra-micro cell with Suprasil windows and an optical path length of 10 × 2 mm. Fluorescence spectra were obtained at 25 °C using an excitation wavelength of 288 nm, with an excitation bandwidth of 4 nm and emission bandwidth of 4 nm. Emission spectra were recorded between 290–380 nm at a scan rate of 60 nm/min.
Buffer elemental analysis.
Due to the well-known structuring effects of divalent metal ions on αSyn , an accurate elemental analysis of the buffer was performed to exclude artifacts in our results due to metal contamination. The high concentration Tris-buffer solution (500 mM) was analyzed for metal contents by atomic absorption spectroscopies. The measured concentrations were Cu = 0.2 ± 0.1 nM, Zn = 3.5 ± 0.1 nM, Fe = 0.9 ± 0.1 nM, and Ca = 22.5 ± 0.1 nM. These values are two orders of magnitude lower than the concentration required to induce structural effects on αSyn .
Gold (Alfa Aesar, 99.99%) was deposited onto freshly cleaved mica substrates (Mica New York Corp., clear ruby muscovite) in a high-vacuum evaporator (Denton Vacuum, model DV502-A) at 10−5 Torr. Before deposition, the mica was preheated to 350 °C by a heating stage mounted behind the mica to enhance the formation of terraced Au(111) domains. The typical evaporation rate was 3 Å/s, and the thickness of the gold films ranged around 300 nm. The mica temperature was maintained at 350 °C for 2 h after deposition for annealing. This method produced samples with flat Au(111) terraces. These films were fixed to a glass substrate with an epoxy (EPO-TEK 377, Epoxy Tech.). They were then separated at the gold–mica interface by peeling immediately before functionalization with the desired molecules. This procedure produced gold substrates with a flat surface morphology due to the templating effect of the atomically flat mica surface [68,69].
Force spectroscopy experiments.
For each experiment, a 20 μl drop of 3S3 construct solution (160 μg/ml) was deposited on the freshly peeled gold surface for about 20 min. SMFS experiments were performed using a commercially available AFM system: Picoforce AFM with Nanoscope IIIa controller (Digital Instruments) using V-shaped silicon nitride cantilevers (NP; Digital Instruments) with a spring constant calibrated by the thermal noise method . The pulling speed was 2.18 μm/s for all experiments. The buffer used was Tris/HCl (10 mM or 500 mM, pH 7.5; the 10 mM buffer was obtained by diluting the 500 mM buffer with milliQ ultrapure water). For CuCl2 experiments, the protein was deposited in a drop with the addition of a final concentration of 1 μM CuCl2 and left on the surface for about 20 min, and the experiments were carried out in 10 mM Tris/HCl with 1 μM CuCl2. Control experiments in DTT were made in 50 mM DTT Tris/HCl buffer.
The force curves were analyzed using the commercially available software from Digital Instrument (Nanoscope v6.12r2), custom Origin scripts and Hooke, a Python-based home coded force spectroscopy data analysis program (M. Sandal, unpublished work). Force curves were analyzed fitting each peak with a simple WLC force versus extension model  with two free parameters: the contour length L and the persistence length p (Equation 1). The I27 modules were characterized in terms of the length of the polypeptide chain extended after each unfolding event.
To assess the statistical validity of the comparison between data obtained in 10 mM Tris/HCl buffer and those obtained in other conditions, standard chi square tests were performed. The differences between the 10 mM Tris data set and the other data sets are significant, with p < 0.01.
Protocol S1. Supplementary Results, Discussion, and Figure
Characterization of the rupture events attributed to mechanically weak interaction and an electrostatic model that explains the observed mechanically weak interactions are given.
(4.9 MB DOC)
The UniProt KB (http://www.ebi.ac.uk/trembl/index.html) accession number for α-synuclein (αSyn) is P37840 (SYUA_HUMAN). The Protein Data Bank (http://www.pdb.org) entry for the I27 domains included in the polyprotein is 1tit. The Online Mendelian Inheritance in Man (OMIM) reference number for familial Parkinsonism is 163890.0002.
We thank Dr. J. Clarke for kindly providing the vectors for constructs expression and Professor J.E. Walker for supplying us the E. coli C41(DE3) cells. We thank Professor G. Legname for critical reading of the manuscript as well for advice and support. We thank Dr. Mark R. Cookson (National Institutes of Health) for providing the A30P αSyn plasmid.
BS, MS, FV, and LB conceived and designed the experiments. MS, FV, IT, and MB performed the experiments. MS, FV, FM, LB, BS, and MB analyzed the data. IT, SM, and EB contributed reagents/materials/analysis tools. MS, FV, LB, and BS wrote the paper.
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