Mutant Protein A30P α-Synuclein Adopts Wild-type Fibril Structure, Despite Slower Fibrillation Kinetics*

Background: A30P α-synuclein is associated with the familial form of Parkinson disease. Results: The secondary structure and chemical shifts of A30P α-synuclein fibrils are in high agreement with wild-type. Conclusion: A30P α-synuclein fibrils adopt the same structure as the wild-type. Significance: This work is an important step toward elucidating the association between the early onset Parkinson disease mutants of α-synuclein fibrils and Parkinson disease pathology. α-Synuclein (AS) is associated with both sporadic and familial forms of Parkinson disease (PD). In sporadic disease, wild-type AS fibrillates and accumulates as Lewy bodies within dopaminergic neurons of the substantia nigra. The accumulation of misfolded AS is associated with the death of these neurons, which underlies many of the clinical features of PD. In addition, a rare missense mutation in AS, A30P, is associated with highly penetrant, autosomal dominant PD, although the pathogenic mechanism is unclear. A30P AS fibrillates more slowly than the wild-type (WT) protein in vitro and has been reported to preferentially adopt a soluble, protofibrillar conformation. This has led to speculation that A30P forms aggregates that are distinct in structure compared with wild-type AS. Here, we perform a detailed comparison of the chemical shifts and secondary structures of these fibrillar species, based upon our recent characterization of full-length WT fibrils. We have assigned A30P AS fibril chemical shifts de novo and used them to determine its secondary structure empirically. Our results illustrate that although A30P forms fibrils more slowly than WT in vitro, the chemical shifts and secondary structure of the resultant fibrils are in high agreement, demonstrating a conserved β-sheet core.

␣-Synuclein (AS) is associated with both sporadic and familial forms of Parkinson disease (PD). In sporadic disease, wild-type AS fibrillates and accumulates as Lewy bodies within dopaminergic neurons of the substantia nigra. The accumulation of misfolded AS is associated with the death of these neurons, which underlies many of the clinical features of PD. In addition, a rare missense mutation in AS, A30P, is associated with highly penetrant, autosomal dominant PD, although the pathogenic mechanism is unclear. A30P AS fibrillates more slowly than the wild-type (WT) protein in vitro and has been reported to preferentially adopt a soluble, protofibrillar conformation. This has led to speculation that A30P forms aggregates that are distinct in structure compared with wild-type AS. Here, we perform a detailed comparison of the chemical shifts and secondary structures of these fibrillar species, based upon our recent characterization of full-length WT fibrils. We have assigned A30P AS fibril chemical shifts de novo and used them to determine its secondary structure empirically. Our results illustrate that although A30P forms fibrils more slowly than WT in vitro, the chemical shifts and secondary structure of the resultant fibrils are in high agreement, demonstrating a conserved ␤-sheet core.
The unifying feature of the "synucleinopathies" is aggregation and accumulation of AS protein within intracellular inclusions (2). Although these diseases are typically sporadic, several mutations in the SNCA gene encoding AS are associated with familial PD, including single-point mutations A53T (3), A30P (4), and E46K (5), and allele duplication (6) or triplication (7). Although the PD-associated AS mutations are extremely rare, analysis of their pathogenicity could significantly illuminate the mechanisms underlying sporadic disease. The normal function of AS is not precisely known, but it shares conserved structural features with the exchangeable apolipoproteins (8), and several lines of evidence suggest a role for AS in presynaptic vesicle trafficking (9 -11). Like the wild-type (WT) protein, all mutant forms of AS are intrinsically unfolded in aqueous solution but adopt an ␣-helical secondary structure within their N-termini upon binding to phospholipid vesicles or detergent micelles (12,13). Within A30P, the helical domain is partially disrupted by proline substitution, with a consequent decrease in lipid affinity (12), whereas the A53T and E46K mutants exhibit similar or enhanced lipid binding compared with WT AS (12,14). Thus, altered lipid affinity is not a unifying phenotype for disease-associated mutants.
One hypothesis to account for the pathogenicity of the PDrelated mutations is that they promote pathological AS aggregation. However, A30P AS has been reported to fibrillate more slowly than WT AS in vitro (15) and to populate a soluble, protofibrillar intermediate preferentially, whereas WT readily progresses to mature, insoluble fibrils (16). This has fueled speculation that the mechanism of A30P toxicity may be fundamentally different from that of WT AS. Only recently has tissue from a familial PD patient with the A30P mutation become available for analysis. This individual displayed neuropathology typical of idiopathic PD but with a greater than typical load of insoluble fibrillar aggregates (17). This is a surprising result that strongly implicates fibrillar AS in the pathogenesis of A30P-dependent PD.
A30P and WT AS fibrils have similar morphologies when viewed by low resolution techniques, like electron microscopy (18). Although recent solution NMR studies of quenched hydrogen/deuterium (H/D) exchange have suggested that the A30P mutation does not perturb the location or arrangement of ␤-strands in WT AS fibrils (19), it is not possible to draw sitespecific conclusions regarding structure from H/D exchange experiments alone; for example, some ␤-sheet regions may be more exposed than others, or protected regions may not exhibit a ␤-sheet secondary structure. In addition, these indirect measurements rely on low molecular mass samples, which require fibrils to be broken down to smaller units. In contrast, solidstate NMR (SSNMR) is uniquely positioned to obtain atomic resolution structural information of systems (like AS fibrils) that are noncrystalline, insoluble, and of high molecular weight; these results are achieved without altering sample integrity. In this study, we sought to determine whether A30P AS fibrils differ from WT AS fibrils at the atomic level of secondary structure. Our results, based on chemical shift analysis obtained with multidimensional SSNMR experiments, illustrate that A30P and WT AS fibrils are highly similar in secondary structural details.

EXPERIMENTAL PROCEDURES
Protein Sample Preparation-Natural abundance and uniformly 13 C, 15 N-labeled WT and A30P full-length, monomer samples were expressed and purified as described previously (20). Briefly, recombinant protein was expressed in Escherichia coli BL21(DE3), while grown in minimal medium supplemented with 13 C, 15 N BioExpress (Cambridge Isotopes). Purification was performed by thermal lysis, hydrophobic interaction, and size exclusion chromatography resulting in high yield (Ͼ40 mg/liter). The sample purity was confirmed by gel electrophoresis and mass spectrometry. To verify that the mutation was present, the plasmid was sequenced and 1 H-15 N heteronuclear single-quantum correlation (HSQC) spectra of the purified monomer samples were acquired (see supplemental Fig. S1).
Thioflavin T Fluorescence-Solutions of monomeric WT and A30P AS (1 mM, 10 mM phosphate buffer, 2.7 mM KCl, 137 mM NaCl, pH 7.4) were filtered, and fibril formation was measured by monitoring Thioflavin T (15 M, Sigma-Aldrich) fluorescence using established protocols (21). Control wells were prepared to account for light scatter and possible quenching. 96-well plates were incubated at 37°C and agitated for 16 min prior to each reading with 4 min of no agitation. Seven replicates were performed for both A30P and WT AS.
Electron Microscopy-WT and A30P AS fibril samples were treated with Karnovsky's fixative and negatively stained with 2% ammonium molybdate (w/v). Samples were applied on Formvar carbon-coated grids (300 mesh) and were viewed with a Hitachi H600 transmission electron microscope, operating at 75 kV.
Solution NMR Spectroscopy-Solution NMR spectroscopy is discussed in the supplemental text.
Solid-state NMR Spectroscopy-An initial solution of monomeric, natural abundance A30P AS (1 mM protein, 50 mM phosphate buffer, pH 7.5, 0.02% azide, and 0.1 mM EDTA) was filtered with a 0.22-m syringe filter. This solution was incubated with shaking (200 rpm) at 37°C for 3 weeks to produce mature fibrils. These fibrils were then used to seed future uniformly 13 C, 15 N-labeled A30P AS fibrils. After the allotted time, fibril solutions were washed, dried, packed into 3.2-mm standard or thin wall rotors (Varian, Fort Collins, CO), and rehydrated with 36% (m/v) water according to previously described protocols (22 (23) and SPINAL-64 (24, 25) 1 H decoupling with a field strength of ϳ75 kHz during evolution and acquisition periods. For three-dimensional 15 N-13 C-13 C and 13 C-15 N-13 C correlation experiments, band-selective SPECIFIC cross-polarization (26) was utilized for heteronuclear polarization transfer between 15 N and 13 C and DARR (27) mixing for 13 C homonuclear polarization transfer. All experiments were acquired under 13.3-kHz MAS and at a cooling gas temperature of 10°C with 90 standard cubic feet per hour flow, resulting in an actual sample temperature of 18 Ϯ 5°C. The adamantane downfield peak was assumed to resonate at 40.48 ppm as an external chemical shift reference (28). The two-and three-dimensional spectra used for chemical shift assignments are listed in supplemental Table S1.
Data were processed with back linear prediction applied to the direct dimension. Zero filling, Lorentzian-to-Gaussian apodization and/or cosine bells were applied for each dimension before Fourier transformation using NMRPipe (29). Peak picking, assignments, and peak heights were obtained with SPARKY software (30) using the approximation of Gaussian line shapes for peak integration.

RESULTS AND DISCUSSION
A30P AS Fibrillates More Slowly than WT-WT and A30P AS solutions were prepared, as described previously (20), to monitor fibril formation with Thioflavin T fluorescence. An increase in lag time indicates a decrease in the fibrillation rate, as shown for A30P compared with WT (Fig. 1a). Our data show WT AS to propagate fibrils after 24 h and A30P after 72 h. These results are in agreement with those of Li et al. (31) and Meuvis et al. (32). Although A30P and WT fibrillate at different rates, a comparison of electron micrographs of mature fibrils, formed after 3 weeks of incubation, exhibit no distinguishable changes in the fibril morphology upon mutation (Fig. 1b).
A30P AS Fibril Morphology Is Highly Reproducible-SSNMR has proven to be a useful structural biology technique in exploring the structure and dynamics of amyloid fibrils, like AS fibrils (33)(34)(35). Certain amino acids (i.e. Gly, Ala, Thr, Ser, Ile, and Pro) are distinctively identifiable by their unique chemical shift patterns and are highly sensitive to secondary structure (36 -40). Therefore, to evaluate slight variations between one fibril batch to the next, 13 C-13 C two-dimensional spectra with 50-ms DARR (27) mixing were acquired of three different batches of A30P AS fibrils, prepared as described previously for uniformly 13 C, 15 N-labeled WT AS fibrils (20,22). The linear regression analysis of two individual batches showed R 2 values of 0.996, 0.999, and 0.999 for 13 CЈ, 13 CA and 13 CB, respectively (Fig. 1,  c-e). Independent batches also exhibit average chemical shift variations of less than 0.2 ppm. Our A30P fibril samples are microscopically well ordered, evidenced by the narrow hetero-geneous line widths, averaging 0.2 ppm (Fig. 1f). Many of the spectral fingerprints of A30P AS fibrils are identical to those of WT; for example, the highly resolved Thr and Ser regions, shown in Fig. 1, g and h. A30P AS Fibril Chemical Shift Assignments-SSNMR heteronuclear ( 15 N-13 C) and homonuclear ( 13 C-13 C) two-dimen-sional experiments with longer DARR mixing times were acquired on uniformly 13 C, 15 N-labeled A30P AS fibrils to detect intra-and interresidue correlations and confirm pairwise assignments. Some signal patterns could be assigned immediately, but the majority of correlation patterns were degenerate due to the presence of sequential, imperfect repeats FIGURE 1. In vitro fibrillation conditions provide microscopically well ordered A30P AS fibrils that form slower than WT. a, average fibril formation assay of (red triangles) and A30P AS fibrils (blue circles) monitored by Thioflavin T fluorescence. Error bars were determined from seven replicates for each. b, comparison of the electron micrographs of WT (left) and A30P AS (right) fibrils. 13 CЈ (c), 13 CA (d), and 13 CB (e) chemical shift plots between two individual batches of A30P AS fibrils. f, 13 C-13 C two-dimensional with 50-ms DARR mixing of A30P AS fibrils. Overlaid expansions of WT (red) on to A30P (blue) AS fibrils for the Thr/Ser (CB-CЈ) (g) and Thr/Ser (CB-CA) (h) regions.

A30P ␣-Synuclein Fibrils Adopt Wild-type Structure
(KTKEGV) in the AS sequence. Accordingly, three-dimensional experiments (supplemental Table S1) were acquired to obtain unambiguous, site-specific chemical shift assignments. 15 N-13 C-13 C three-dimensional experiments detect a common nitrogen frequency to associate two neighboring residues (the i and iϪ1 residues). Additionally, 13 C-15 N-13 C three-dimensional experiments can be used to gain an added common frequency such as 13 CA or 13 CЈ in the second dimension. For example, a CAN(CO)CX starts with 13 C polarization on 13 CA nuclei and is transferred to 15 N nuclei; this is followed by a polarization transfer from 15 N to 13 CЈ nuclei (where no chemical shift evolution takes place) using specific cross-polarization (26). Once these cross-polarization transfers have occurred, the resulting polarization on the 13 CЈ nucleus is transferred through space to the side chain 13 C nuclei using the DARR mixing scheme. Using these three multidimensional experiments, we conducted chemical shift assignments of sequential residues using well established techniques for making de novo site-specific chemical shift assignments (22,(43)(44)(45)(46)(47)(48)(49). Fig. 2 illustrates how the backbone walk method is used to assign seven consecutive residues in A30P AS fibrils. Sequential backbone assignments were achieved for the stretches of Val 40 -Val 49 , Gly 51 -Val 55 , and Glu 57 -Asp 98 (supplemental Figs. S2 and S3). A total of 63 unique de novo resonance assignments were possible for A30P AS fibrils (supplemental Table S2) without relying upon the WT AS chemical shift lists.
The resolution and sensitivity of A30P AS fibril spectra were in some instances better than those observed with WT fibrils; for example, a number of signals (corresponding to residues Glu 57 , Glu 61 , and Asp 98 ) were detected in the loop regions that were not evident in comparable spectra of WT AS fibrils. In previous studies of the WT AS fibrils, residues Tyr 39 to Lys 43 , Lys 58 to Lys 60 , Gln 62 , and Lys 97 (highlighted in supplemental Table S2) could only be assigned using data acquired with 13 Csparsely labeled samples (22), which provide higher resolution data compared with uniformly 13 C-labeled samples (50). For A30P, these residues were detected and assigned using uniformly 13 C-labeled samples, which we attribute to technical improvements in the data collection and potential differences in the dynamics of the loop regions. Some of these signals show slight chemical shift perturbations relative to WT (see below), consistent with small conformational differences and/or chemical exchange effects.
A30P ␣-Synuclein Forms Fibrils That Are Structurally Similar to Wild Type-We applied linear regression analysis to the complete set of WT (22) and A30P AS fibril chemical shifts (Fig.  3). The chemical shifts of 13 CA and 13 CB, which report primarily upon secondary structure, showed a high agreement (R 2 values of 0.999 and 0.998, respectively) and confirm nearly identical secondary structures between A30P and WT AS fibrils. The 15 N and 13 C' chemical shifts exhibit R 2 values of 0.998 and 0.991, respectively, which are consistent with modest perturbations in hydrogen bonding and electrostatics upon mutation (51,52).
As demonstrated previously (53), the dipolar-based CANCO experiment produces a correlation for the most rigid residues in a given sample. Amyloid fibrils contain a rigid core, where dipolar-based experiments transfer polarization with high effi- ciency, and mobile regions, where polarization transfer is inefficient in dipolar-based experiments (34,54). Thus, the signal intensities report qualitatively on rigidity. Sixty-one correlations were identified in the CANCO spectrum of A30P AS fibrils, of a possible maximum of 139 backbone pair correlations from 140 residues. Of the correlations detected in the CANCO spectra, 91% were unambiguously assigned, as described in Fig. 2. Fig. 4c demonstrates the trend in signal intensity by residue number for A30P AS fibrils. The region with the greatest intensity is found for residues 68 -94, which includes the most hydrophobic stretch, 71-82 (55). Signals from mobile regions, such as the termini, are not observed in these spectra, due to the low efficiency of dipolar-mediated polarization transfer for mobile residues. SSNMR detects differences in chemical environments with high sensitivity (37)(38)(39)(40)56). This allows for the identification of amino acids and prediction of backbone dihedral angles ( and ) and secondary structure with the TALOSϩ program, illustrated in Fig. 4, a and b (38, 57). Our results pertaining to A30P AS fibrils indicate a highly similar ␤-sheet secondary structure relative to the WT (22) (Fig. 4a). This is consistent with the localization of A30 outside the stable ␤-sheet core for the WT fibril structure, thus exerting no major effect on the ␤-sheet secondary structure of the core upon mutation (22).
The improvement in data quality of A30P AS fibrils allowed for the detection of additional residues and extended empirical determination of secondary structure compared with the WT in the Val 55 -Val 63 region. In addition, when the chemical shifts of this region were compared between A30P and WT AS fibrils, perturbations greater than 0.5 ppm for Val 55 , Lys 58 , Lys 60 , and Val 63 were observed; this variation significantly exceeds the batch-to-batch variations in individual sample preparations (ϳ0.2 ppm). These localized chemical shift perturbations support the idea that this region somehow interacts with residue 30 in the AS fibril structure. We envision three possible scenarios. (i) The region Val 55 -Val 63 is proximate to A30 in the folded WT structure; these interactions are modified as a direct result of the A30P mutation. (ii) The region Val 55 -Val 63 of one molecule is proximate to A30 of a neighboring molecule, due to the qua-  ternary arrangement of the fibril; such interactions would also change as a direct result of the A30P mutation. (iii) The region Val 55 -Val 63 interacts with the N-terminal domain of the WT fibrils, and the mutation A30P disrupts the organization of this N-terminal domain; thus the perturbations in the region Val 55 -Val 63 would be an indirect consequence of the mutation. These three scenarios are not mutually exclusive.
Furthermore, our SSNMR results demonstrate that the N-terminus of A30P is more dynamic than the fibril core, based upon the absence of N-terminal signals in the dipolar spectra. Perhaps significantly, Goedert and co-workers report that the truncation of the N-terminal domain of AS causes an increase in the fibrillation lag time of WT AS (42). This demonstrates that the intact N-terminal domain plays a role in promoting fibrillation and suggests a mechanism whereby disruption of the N-terminal domain (via the A30P mutation) might inhibit fibrillation kinetics without altering the fibril structure. These observations are consistent with the hypothesis that the A30P mutation affects the susceptibility to form fibrils in vitro, hence the propensity to form more oligomeric species than mature fibrils (31).
Although the propensity to fibrillize more slowly in vitro is well documented for A30P, a recent report of neuropathology in a familial PD patient with the A30P mutation demonstrated a greater than typical load of insoluble fibrillar aggregates as compared with sporadic PD patients (17). This seeming paradox remains to be explained, although it is plausible that relative fibrillation kinetics might differ significantly in a cellular environment. The A30P mutation decreases lipid affinity and disrupts the structure of the lipid-bound protein relative to WT (12), which could alter the trafficking, localization, and turnover of A30P or its interactions with chaperone molecules. Elucidation of the cellular factors that modulate AS fibrillation are a subject of ongoing research.

CONCLUSIONS
We have performed a site-specific comparison between the secondary structures of full-length WT and A30P AS fibrils. Chemical shift assignments and the empirically determined secondary structure demonstrate that A30P adopts the wildtype fibril structure, despite the fact that A30P forms fibrils more slowly. Our results show that the A30P mutation does not substantially perturb the resulting AS fibril secondary structure at an atomic level.