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Secondary nucleation of monomers on fibril surface dominates α-synuclein aggregation and provides autocatalytic amyloid amplification

Published online by Cambridge University Press:  20 March 2017

Ricardo Gaspar ,
Georg Meisl ,
Alexander K. Buell ,
Laurence Young ,
Clemens F. Kaminski ,
Tuomas P. J. Knowles ,
Emma Sparr  and
Sara Linse
Ricardo Gaspar
Affiliation:
Department of Physical-Chemistry, Lund University, Lund, Sweden Department of Biochemistry and Structural Biology, Lund University, Lund, Sweden
Georg Meisl
Affiliation:
Department of Chemistry, University of Cambridge, Cambridge, UK
Alexander K. Buell
Affiliation:
Department of Chemistry, University of Cambridge, Cambridge, UK Institute of Physical Biology, University of Düsseldorf, Düsseldorf, Germany
Laurence Young
Affiliation:
Department of Chemical Engineering and Biotechnology, University of Cambridge, Cambridge, UK
Clemens F. Kaminski
Affiliation:
Department of Chemical Engineering and Biotechnology, University of Cambridge, Cambridge, UK
Tuomas P. J. Knowles
Affiliation:
Department of Chemistry, University of Cambridge, Cambridge, UK
Emma Sparr*
Affiliation:
Department of Physical-Chemistry, Lund University, Lund, Sweden
Sara Linse*
Affiliation:
Department of Biochemistry and Structural Biology, Lund University, Lund, Sweden
*
*Authors for correspondence: Emma Sparr, Department of Physical-Chemistry, Lund University, Lund, Sweden and Sara Linse, Department of Biochemistry and Structural Biology, Lund University, Lund, Sweden. Email: emma.sparr@fkem1.lu.se and sara.linse@biochemistry.lu.se
*Authors for correspondence: Emma Sparr, Department of Physical-Chemistry, Lund University, Lund, Sweden and Sara Linse, Department of Biochemistry and Structural Biology, Lund University, Lund, Sweden. Email: emma.sparr@fkem1.lu.se and sara.linse@biochemistry.lu.se
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Abstract

Parkinson's disease (PD) is characterized by proteinaceous aggregates named Lewy Bodies and Lewy Neurites containing α-synuclein fibrils. The underlying aggregation mechanism of this protein is dominated by a secondary process at mildly acidic pH, as in endosomes and other organelles. This effect manifests as a strong acceleration of the aggregation in the presence of seeds and a weak dependence of the aggregation rate on monomer concentration. The molecular mechanism underlying this process could be nucleation of monomers on fibril surfaces or fibril fragmentation. Here, we aim to distinguish between these mechanisms. The nature of the secondary processes was investigated using differential sedimentation analysis, trap and seed experiments, quartz crystal microbalance experiments and super-resolution microscopy. The results identify secondary nucleation of monomers on the fibril surface as the dominant secondary process leading to rapid generation of new aggregates, while no significant contribution from fragmentation was found. The newly generated oligomeric species quickly elongate to further serve as templates for secondary nucleation and this may have important implications in the spreading of PD.

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Quarterly Reviews of Biophysics , Volume 50 , 2017 , e6
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Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution, and reproduction in any medium, provided the original work is properly cited.
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Copyright © Cambridge University Press 2017

1. Introduction

Protein misfolding and aberrant aggregation processes that elude cellular maintenance mechanisms can result in major disturbances of cellular processes. This may lead to protein aggregation diseases, for example Parkinson's disease (PD), the prevalence of which is increasing (Dobson, Reference Dobson2003). In PD, the formation and deposition of amyloid fibrils by the protein α-synuclein (α-syn) is the pathological hallmark associated with degeneration of dopaminergic neurons in the substantia nigra (Fink, Reference Fink2006), and other brain regions. Neurodegeneration is believed to initiate at the synapse, and once started, the disease spreads without remission until reaching a terminal phase (Danzer et al. Reference Danzer, Krebs, Wolff, Birk and Hengerer2009; Schulz-Schaeffer, Reference Schulz-Schaeffer2010). Cell death appears to result from the aggregation process per se or the presence of oligomeric aggregates that impair neurotransmission (Lesné et al. Reference Lesné, Koh, Kotilinek, Kayed, Glabe, Yang, Gallagher and Ashe2006; Shankar et al. Reference Shankar, Li, Mehta, Garcia-Munoz, Shepardson, Smith, Brett, Farrell, Rowan, Lemere, Regan, Walsh, Sabatini and Selkoe2008; Wakabayashi et al. Reference Wakabayashi, Tanji, Mori and Takahashi2007; Winner et al. Reference Winner, Jappelli, Maji, Desplats, Boyer, Aigner, Hetzer, Loher, Vilar, Campioni, Tzitzilonis, Soragni, Jessberger, Mira, Consiglio, Pham, Masliah, Gage and Riek2011). Indeed, toxic forms may arise in a reaction involving both monomeric and fibrillar species (Jan et al. Reference Jan, Adolfsson, Allaman, Buccarello, Magistretti, Pfeifer, Muhs and Lashuel2011), generating oligomers at the fibril surface (Cohen et al. Reference Cohen, Linse, Luheshi, Hellstrand, White, Rajan, Otzen, Vendruscolo, Dobson and Knowles2013).

α-Syn is a natively unfolded 140 amino acid protein that exists abundantly in neuronal cells, where it is located in the proximity of vesicles within the presynaptic terminals (Izawa et al. Reference Izawa, Tateno, Kameda, Hirakawa, Hato, Yagi, Hongo, Mizobata and Kawata2012). α-Syn comprises 1% of total cytosolic protein in the nervous system (Stefanis, Reference Stefanis2012) with an estimated intracellular concentration ranging from 30 to 60 µM (Rabe et al. Reference Rabe, Soragni, Reynolds, Verdes, Liverani, Riek and Seeger2013). The physiological functions of α-syn are still unclear, but are likely related to vesicle trafficking and release (Bisaglia et al. Reference Bisaglia, Mammi and Bubacco2009). The onset of PD is also unclear, but has been suggested to be related to α-syn levels above a critical aggregation concentration (Galvagnion et al. Reference Galvagnion, Buell, Meisl, Michaels, Vendruscolo, Knowles and Dobson2015; Pinotsi et al. Reference Pinotsi, Michel, Buell, Laine, Mahou, Dobson, Kaminski and Schierle2016; Rabe et al. Reference Rabe, Soragni, Reynolds, Verdes, Liverani, Riek and Seeger2013). The amyloid fibrils formed from recombinant α-syn in vitro are highly similar to those extracted from PD patients in terms of morphology and size (Conway et al. Reference Conway, Harper and Lansbury1998). In vitro experiments have shown that the aggregation of α-syn is very sensitive to solution conditions, such as temperature (Uversky et al. Reference Uversky, Li and Fink2001), pH (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014), salt concentration (Munishkina et al. Reference Munishkina, Henriques, Uversky and Fink2004) and the presence of cofactors (Ashmad et al. Reference Ashmad, Chen and Lapidus2012). In addition, the presence of surfaces, e.g. air–liquid interface for which α-syn has high affinity, has been shown to influence aggregation kinetics in vitro (Campioni et al. Reference Campioni, Carret, Jordens, Nicoud, Mezzenga and Riek2014). The primary nucleation of α-syn can be accelerated by the presence of lipid membranes (Galvagnion et al. Reference Galvagnion, Buell, Meisl, Michaels, Vendruscolo, Knowles and Dobson2015; Grey et al. Reference Grey, Dunning, Gaspar, Grey, Brundin, Sparr and Linse2015), surfactant micelles (Giehm & Otzen, Reference Giehm and Otzen2010) and nanoparticles (Vácha et al. Reference Vácha, Linse and Lund2014). Mechanical agitation enhances fibril fragmentation and increases the air–water interfacial area, which may promote heterogeneous primary nucleation (Campioni et al. Reference Campioni, Carret, Jordens, Nicoud, Mezzenga and Riek2013; Giehm & Otzen, Reference Giehm and Otzen2010). Quiescent conditions may therefore be preferred in mechanistic studies.

The formation of amyloid fibrils occurs through a nucleation-dependent polymerization reaction. Underlying the macroscopically observable sigmoidal growth curves are several possible microscopic steps occurring simultaneously: primary nucleation of monomers in solution or on surfaces, elongation of fibrils through the addition of monomers to fibril ends, secondary nucleation of monomers on the surface of already existing fibrils and fibril breakage (Arosio et al. Reference Arosio, Cukalevski, Frohm, Knowles and Linse2014; Pinotsi et al. Reference Pinotsi, Buell, Galvagnion, Dobson, Schierle and Kaminski2014). In each case, detailed kinetic studies are needed to reveal the relative importance of these steps. For α-syn, mechanistic studies under quiescent conditions are difficult because homogeneous primary nucleation in bulk solution is undetectably slow, a behavior very different from that observed for many other aggregating proteins, including Aβ42 (Arosio et al. Reference Arosio, Knowles and Linse2015; Cohen et al. Reference Cohen, Linse, Luheshi, Hellstrand, White, Rajan, Otzen, Vendruscolo, Dobson and Knowles2013), Aβ40 (Meisl et al. Reference Meisl, Yang, Hellstrand, Frohm, Kirkegaard, Cohen, Dobson, Linse and Knowles2014), actin (Oosawa & Asakura, Reference Oosawa and Asakura1975) and some prions (Collins et al. Reference Collins, Douglass, Vale and Weissman2004; Tanaka et al. Reference Tanaka, Collins, Toyama and Weissman2006). Therefore, the initiation of in vitro aggregation requires the presence of seeds or other surfaces that enhance nucleation; here we have used pre-formed α-syn fibrils.

2. Outline of the problem

The formation of amyloid fibrils by the intrinsically disordered protein α-syn is a hallmark of PD. There is a correlation between spreading of amyloid and neuronal death. It is therefore of utmost importance to characterize the underlying microscopic steps of the assembly reaction that lead to the conversion of soluble α-syn into its insoluble amyloid fibrils. At mildly acidic pH, mimicking specific cellular environments, such as endosomes and lysosomes, the aggregation of α-syn is greatly accelerated compared with neutral pH, and this effect has been attributed to a strongly pH-dependent autocatalytic process. The molecular mechanism of this process could be nucleation of monomers on fibril surfaces or fibril fragmentation as outlined in Fig. 1. Here, we address the problem of elucidating the α-syn aggregation mechanism, with an aim to distinguish between nucleation on fibril surfaces or fibril fragmentation. We have used seeded aggregation kinetics together with a filter trap assay, differential sedimentation analysis, quartz crystal microbalance studies and two-color super-resolution microscopy using dSTORM to distinguish between these two possibilities. Our data imply that the secondary process consists of nucleation of monomers on the surfaces of existing fibrils, hence rationalizing the autocatalytic nature of the aggregation process.

Fig. 1.

Schematic depictions of the two possible secondary processes in the aggregation of α-syn at mildly acidic pH conditions. (a) Fibrils multiply through fragmentation. (b) Fibrils catalyze the formation of new aggregates from monomer on their surface. In a saturated secondary nucleation reaction the initial monomer-dependent (attachment) step is so fast that the second monomer-independent (rearrangement or detachment) step becomes the rate determining step (RDS).

3. Results

3.1. Non-seeded aggregation kinetic experiments

α-Syn aggregation is strongly influenced by intrinsic and extrinsic factors. In order to obtain a well-controlled system, all kinetic studies were here performed under quiescent conditions at mildly acidic pH (10 mM MES buffer pH 5·5). To investigate the role of surfaces, reactions starting from monomeric α-syn were monitored in untreated polystyrene (PS) plates as well as non-binding PS plates coated with polyethylene glycol (PEG). Interestingly, no aggregation of α-syn was detected during the time frame of the experiment (up to 100 h) in the PEGylated plates, whereas reproducible kinetic traces with typical sigmodal curves were observed in PS plates (S3A). This highlights the importance of heterogeneous nucleation of α-syn on the PS surface as previously found when adding PS nanoparticles to α-syn in the PEGylated plates (Vácha et al. Reference Vácha, Linse and Lund2014). Another striking observation from the current experiments in PS plates is that α-syn aggregation kinetics appear independent of the peptide concentration at high monomer concentrations (above ca. 30 µM, S3B). To characterize the aggregation mechanism of α-syn in the absence of catalyzing foreign surfaces, all further experiments presented here were conducted in non-binding PEGylated plates in the presence of seeds.

3.2. Seeded kinetic experiments

It is well established that by using preformed fibrils as seeds, the primary nucleation reaction can be bypassed (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014; Giehm & Otzen, Reference Giehm and Otzen2010). Therefore, the reaction was here monitored in the presence of controlled amounts of α-syn seeds. As the reaction is very sensitive to the concentration and size of the seeds, it is vital to handle all seed solutions in the same manner, as described in the materials and methods section. Initial seeded kinetic experiments were conducted by systematically varying monomer (1–50 µM) and seed (0·3–3 µM) concentrations (Figs 2 and 3). The monomer concentrations fall within the physiologically relevant range (Rabe et al. Reference Rabe, Soragni, Reynolds, Verdes, Liverani, Riek and Seeger2013). Strikingly, for each seed concentration, the α-syn aggregation rate appears to be independent of the initial monomer concentration above ca. 10 µM, as evident from the overlapping curves at early times in Fig. 2a–c. This implies that the processes contributing to the aggregation reaction under these conditions, elongation and secondary nucleation are saturated.

Fig. 2.

Seeded α-syn aggregation kinetics. The monomer concentration was systematically varied in the range of 1–50 µM in the presence of three different seed concentrations: (a) 3 µM, (b) 1 µM and (c) 0·3 µM in 10 mM MES pH 5·5 at 37 °C under quiescent conditions. For each solution condition three traces are shown in bold circles. The figures show ThT intensity as a function of time (non-normalized raw data). Different microscopic mechanistic events lead to overall different observable macroscopic kinetic profiles, as shown through simulated traces for the case of monomer concentration variation in the presence of 1 µM seed (experimental data shown in 2b) for the different kinetic models tested, (d) only primary nucleation and elongation, (e) dominant fragmentation and (f) dominant saturated secondary nucleation.

Fig. 3.

Seeding efficiency in α-syn aggregation. (a–c) Representative seeded aggregation kinetic traces in the presence of fixed (3, 1, 0·3 and 0 µM) seed concentrations incubated with (a) 50 µM, (b): 10 µM and (c) 5 µM α-syn monomer. For each condition three traces are shown in bold circles. (d) Aggregation with systematic variation of α-syn seed concentration from 0 to 20% in the presence of a fixed α-syn monomer concentration (20 µM). Averages of three traces are shown as solid lines. All figures show ThT intensity as a function of time (non-normalized raw data). Therefore, experiments in the presence of seeds show elevated ThT intensity at time zero. All experiments were performed in 10 mM MES pH 5·5 in non-binding PEGylated plates at 37 °C and under quiescent conditions.

Comparing the kinetic curves at a fixed monomer concentration and varied amount of preformed seeds (Fig. 3), it is clear that increasing concentration of seed fibrils leads to a decrease in lag time, and that no aggregation is observed in the absence of seed fibrils. This behavior is observed at all monomer concentrations studied. The formation of new fibrils is thus strongly enhanced by the presence of seed fibrils, which is the definition of a secondary process (Cohen et al. Reference Cohen, Vendruscolo, Dobson and Knowles2012). In addition, most of the aggregation curves have concave shapes, i.e. an accelerating rate of aggregation at early times, indicating the existence of a process that significantly increases the number of growth competent ends (i.e. aggregates) (S5).

A number of kinetic models were globally fitted to the experimental data (Meisl et al. Reference Meisl, Kirkegaard, Arosio, Michaels, Vendruscolo, Dobson, Linse and Knowles2016a) and only models that include secondary processes were found to produce reasonable fits. There are some remaining deviations that may be due to higher-order assembly events (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014) not included in the existing model. Simulated macroscopic traces for the case of monomer concentration variation in the presence of 1 µM seed concentration (experimental data shown in Fig. 2b), for the different kinetic models tested are shown in Fig. 2d–f (Meisl et al. Reference Meisl, Kirkegaard, Arosio, Michaels, Vendruscolo, Dobson, Linse and Knowles2016a). Two models were most consistent with the data: having either fragmentation or saturated secondary nucleation as the dominant processes of fibril multiplication (Fig. 2e, f). This is manifested in the very weak dependence of the overall aggregation rate on the monomer concentration observed in our seeded kinetic data. We next designed experiments to distinguish between fragmentation and nucleation of monomers on fibril surface as the dominant secondary process.

3.3. Sedimentation analysis of fibril size development

The fragmentation of fibrils would lead to a change in fibril size distribution, even after the monomer concentration has reached the solubility limit (Michaels et al. Reference Michaels, Yde, Willis, Jensen, Otzen, Dobson, Buell and Knowles2015). α-Syn aggregates at different times after the aggregation process was completed were investigated using differential sedimentation analysis (Arosio et al. Reference Arosio, Cedervall, Knowles and Linse2016). The method relies on the fact that aggregates of different sizes travel through a sucrose gradient at different speeds. The results show that the retention time profile of the samples remains unaltered over up to 20 days (Fig. 4a), implying that the fragmentation rate is undetectably low under quiescent conditions.

Fig. 4.

Experiments designed to identify the dominant secondary process of α-syn aggregation at mildly acidic pH conditions. (a) Time-dependent differential sedimentation analysis performed on fibrils incubated at 37 °C under quiescent conditions in 10 mM MES buffer pH 5·5 for 1–20 days. Aggregates sediment within a sucrose gradient on a rotating disc where longer retention times correspond to smaller size aggregates. The raw data is shown to the left and processed data to the right. The calculations of relative weight and size are made under the assumption of spherical particles, which leads to an underestimation of the size and relative weight for a fibrillar particle. Nevertheless, changes in size distribution can be detected, which was the purpose of this experiment. The figures show representative traces of each condition that was repeated at least two times. (b) Trap and seed kinetic experiment. Fibrils made from 20 µM α-syn monomer supplemented with 3 µM seed fibrils in 10 mM MES pH 5·5 were trapped by filtration in filter plates and the flow-through (filtrate 1) was collected in non-binding PEGylated plates, supplemented with ThT and monitored in a plate reader (B1). The trapped fibrils were then incubated for 2 h with concentrations ranging from 10 to 50 µM α-syn monomer or 10 mM MES buffer pH 5·5 and newly filtered (filtrates 2 and 3, respectively). Again, the flow-through was collected in non-binding PEGylated plates, supplemented with ThT and monitored (B2 and B3). The figures show averages of at least four traces that are shown in bold with individual traces dotted below and are plotted as ThT intensity as a function of time (non-normalized data).

3.4. Trap and seed kinetic experiment

As a further test as to whether fragmentation or surface catalysis are the major sources of new aggregates, a set of experiments, referred to as the trap and seed kinetic approach (Arosio et al. Reference Arosio, Cukalevski, Frohm, Knowles and Linse2014) was performed at 37 °C under quiescent conditions (Fig. 4b). Mature fibrils were trapped in low-binding GHP membrane filter plates (Nasir et al. Reference Nasir, Linse and Cabaleiro-Lago2015) with 200 nm cutoff (retentate), and the flow through was collected in non-binding PEGylated plates (filtrate 1). Purified α-syn monomer at different concentrations or buffer alone was added and incubated with the trapped fibrils for 2 h and again filtered (filtrates 2 and 3, respectively). The aggregation kinetics of filtrates 1, 2 and 3 were followed by ThT fluorescence (Fig. 4b). For filtrate 1, no enhanced fluorescence was detected within the time frame of the experiment (90 h), which indicates that seeds were trapped in the GHP membrane filter, and that any monomer or smaller species in the filtrate are present at too low concentration to give rise to any significant aggregation (Fig. 4B1). This control is relevant to show that the system has reached equilibrium. When 16 µM of monomeric α-syn was added to wells with filtrate 1, aggregation was detected. This implies that some catalyzing species are present in filtrate 1 (Fig. 4B1). For filtrate 2, sigmoidal ThT fluorescence curves are seen within ca. 15 h at all monomer concentrations (Fig. 4B2). In contrast, no fluorescence increase is observed for filtrated monomer that has been incubated in the filter plate without seeds (negative control) (Fig. 4B2). Together, this indicates that during incubation of monomer with trapped fibrils, a fibril-catalyzed reaction generates a significant concentration of aggregates that are small enough to pass through the filter together with the remaining monomer. We conclude that the trapped fibrils present catalytic surfaces promoting aggregation of the added monomeric α-syn. ThT was added to filtrate 3 and the fluorescence was monitored for approximately 70 h (Fig. 4B3). The ThT intensity was close to background suggesting either that fibril fragmentation did not occur to any significant extent, or that fragments were larger than the membrane cutoff. After ca. 70 h, 16 µM monomer was added to filtrate 3, but no fluorescence increase was detected over the following 80 h, confirming the absence of small catalyzing species that could have been present as a result of fibril fragmentation (Fig. 4B3).

3.5. Surface affinity of monomers is pH dependent

The interaction between monomeric and fibrillar α-syn as a function of pH was studied by means of quartz crystal microbalance with dissipation (QCM-D) to monitor the association and dissociation of monomers to and from surface-attached fibrils. This experimental strategy relies on the observation that fibril elongation occurs at significant rates over a much larger pH range than secondary nucleation (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014). The QCM-D measurements provide information on the total amount of adsorbed material (including the coupled solvent) from the change in frequency (ΔF), as well as the viscoelastic properties of the attached layer from the dissipation (ΔD). Figure 5a shows typical QCM-D data where the decrease in frequency is due to added mass, albeit the relation between frequency and mass addition can be non-linear for viscoelastic layers. Gold coated sensor crystals with covalently immobilized and elongated α-syn fibrils were exposed to 20 µM α-syn monomer in 10 mM MES buffer at pH 5·5, 5·7, 5·9, 6·1 and 6·5 to allow for monomer adsorption and fibril elongation in different proportions. After a certain frequency shift (~420 Hz) was obtained for each pH condition, each sensor was washed with 10 mM MES buffer pH 6·5 to monitor dissociation. We observe a strong pH dependence of monomer association with the fibrils. A sharp decrease in frequency was observed during incubation with monomer at pH < 6·0, followed by a rapid increase during washing at pH 6·5 (Fig. 5a). This indicates that the majority of mass that was added at pH < 6·0 is reversibly associated. A less sharp decrease in frequency was observed during incubation with monomer at pH > 6·0, followed by a smaller increase during washing, indicating that the majority of the mass added is unaffected by washing at pH 6·5 (Fig. 5a). We interpret this behavior as evidence for two types of mass addition, the relative importance of which depends on the pH. At pH > 6·0 mostly elongation occurs, and monomers are very slowly dissociating upon washing. At pH < 6·0, surface binding becomes significant, and the mass addition is reversible upon washing at pH > 6·0. Therefore, reversible surface binding has a similar pH dependence as the secondary process (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014), providing additional support for the hypothesis that the secondary process consists of nucleation of monomers on the surface of existing fibrils.

Fig. 5.

The surface of α-syn amyloid fibrils shows a pH-dependent affinity for monomeric α-syn. (a) Fibrils of α-syn were immobilized on gold-coated QCM-D sensor crystals and incubated with 20 µM monomeric α-syn in 10 mM MES buffer at different pH values until a certain frequency shift was reached (ca. −420 Hz for overtone N = 3). The sensors were then washed with 10 mM MES pH 6·5 (indicated by arrows), leading to different levels of dissociation of the previously attached material. (b) Scheme of what is postulated to occur on the sensors for the conditions of pH < 6·0 and pH > 6·0. The orange stars represent binding to the surface of the fibrils.

3.6. Imaging of amyloid growth from seed fibrils

In order to investigate amyloid growth from seed fibrils at mildly acidic pH conditions, we imaged samples with super-resolution microscopy. The approach employed was a two-color dSTORM strategy previously reported (Pinotsi et al. Reference Pinotsi, Buell, Galvagnion, Dobson, Schierle and Kaminski2014). This technique relies on labeling two samples of an α-syn cysteine variant (N122C) with two different Alexa Fluor dyes, namely Alexa Fluor 647 (AF647) and Alexa Fluor 568 (AF568). Preformed seeds of α-syn-AF647 (purple) were incubated with α-syn-AF568 (green) monomer at pH 5·5 (Fig. 6). Comparing with images taken at neutral pH (Pinotsi et al. Reference Pinotsi, Buell, Galvagnion, Dobson, Schierle and Kaminski2014), it is again clear that the aggregation mechanism is pH dependent. Two scenarios were discerned from these images: at mildly acidic pH monomer showed affinity for the surface along the sides of the existing seeds (co-localization of purple and green in Fig. 6), while for neutral pH conditions elongation dominated and monomer showed greater affinity for the growth-competent fibril ends (Pinotsi et al. Reference Pinotsi, Buell, Galvagnion, Dobson, Schierle and Kaminski2014). It should be noted here that, irrespective of the conditions during sample preparation, the dSTORM imaging was performed in a dedicated imaging buffer at pH 8·2. As the majority of the mass added at mildly acidic pH is reversibly associated, as inferred from the QCM-D data (Fig. 5), it is likely that the majority of the mass added to the fibril seeds at pH 5·5 detach from the fibrils when they are placed in buffer of higher pH due to repulsive electrostatic interactions. This might then lead to an underestimation of the amount of associated α-syn-AF568 species at the fibril surface. Still, it is evident that the surfaces along the α-syn-AF647 fibrils contain along their length α-syn-AF568 species.

Fig. 6.

dSTORM images of amyloid growth from seed fibrils at mildly acidic pH conditions. (a) Imaged preformed seed fibrils of α-syn N122C labeled with 1:20 AF647 used for the self-seeding experiment. (b, c) α-Syn monomer labeled with AF568 (green) was incubated with 50% seed fibrils labeled with AF647 (purple). The top panel is imaged in the red channel, middle panel imaged in the green channel and the bottom panel is the merge between both channels. Scale bar corresponds to 1 µm.

4. Discussion

Alterations in the balance of protein synthesis and clearance may lead to the formation of toxic oligomers and trigger a neurodegenerative cascade (Lee et al. Reference Lee, Desplats, Lee, Spencer and Masliah2012). No clear correlation has been found between the amount of α-syn inclusions and the stage of PD (Chaudhary et al. Reference Chaudhary, Stefanovi, Subramaniam and Claessens2014), although larger areas of the brain contain aggregated α-syn as the disease progresses (Braak et al. Reference Braak, Tredici, Bratzke, Hamm-Clement, Sandmann-Keil and Rüb2002).

In a previous study, we have shown that the α-syn aggregation is dominated by secondary processes under mildly acidic conditions (pH < 6·0) (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014). It was also shown that at neutral pH, there is a linear relation between the elongation rate and monomer concentration at low monomer concentrations, and that the elongation rate becomes saturated at high monomer concentrations (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014). Similar overall behavior has been observed for other amyloid proteins, including Sup35 yeast protein (Collins et al. Reference Collins, Douglass, Vale and Weissman2004), S6 (Lorenzen et al. Reference Lorenzen, Cohen, Nielsen, Herling, Christiansen, Dobson, Knowles and Otzen2012), insulin (Buell et al. Reference Buell, Blundell, Dobson, Welland, Terentjev and Knowles2010a) and α-lactalbumin (Buell et al. Reference Buell, Blundell, Dobson, Welland, Terentjev and Knowles2010a).

In the current work, we aim to understand the nature of the dominant secondary process at mildly acidic pH. As a first strategy we studied the monomer dependence of the aggregation kinetics in the presence of low concentrations of preformed seed fibrils. Two different scenarios are consistent with the observation that the aggregation kinetics is only weakly dependent on the concentration of monomeric α-syn: (a) fibrils multiply through fragmentation or (b) fibrils catalyze the formation of new aggregates from monomers on their surface, but this reaction is saturated at the monomer concentrations investigated. Secondary nucleation consists of an initial attachment of monomers to the surface, followed by nucleus formation and detachment. However, secondary nucleation may saturate at high enough monomer concentrations, where the initial attachment becomes very fast. The fibril is then fully covered in monomer and the second, monomer-independent (rearrangement or detachment) step, becomes rate limiting (Meisl et al. Reference Meisl, Yang, Hellstrand, Frohm, Kirkegaard, Cohen, Dobson, Linse and Knowles2014). The two models lead to the same overall scaling of the kinetic behavior with monomer and fibril concentration. To distinguish the nature of the dominant secondary mechanism, additional and complementary experiments were performed including: (i) differential sedimentation, (ii) the trap and seed kinetic approach, (iii) QCM-D biosensing studies and (iv) two-color super-resolution microscopy using dSTORM.

Fragmentation and secondary nucleation mechanisms may lead to different final states. If fragmentation is the dominant mechanism, then the mature fibrils will keep fragmenting even after completion of the aggregation reaction. However, the differential sedimentation analysis shows that the mature fibrils do not become shorter over time, implying that spontaneous fragmentation occurs very slowly. This makes fragmentation of fibrils less likely to be the dominant secondary mechanism.

The trap and seed kinetic approach was used to probe whether new oligomeric aggregates smaller than 200 nm are formed during a reaction involving both monomer and fibrils. We found that α-syn aggregation is clearly faster in samples of filtrates from reactions where α-syn monomers had been incubated with trapped fibrils compared with samples where α-syn monomers had been incubated for the same time in the same type of filters with no preformed seeds, confirming again the importance of secondary processes. Moreover, since shedding/fragmentation of the trapped fibrils when incubated with buffer alone under the same experimental conditions was undetectable, alongside the observation that spontaneous fragmentation does not occur during the time frame studied, we propose that the newly formed oligomeric species are most likely generated by a secondary nucleation process of α-syn monomer at the surface of existing fibrils. As with the seeded kinetic experiments, in the trap and seed assay, we also observed that the aggregation kinetics are to a large extent independent of the monomer concentration, likely a result of saturated secondary nucleation.

QCM-D experiments were set up with changes in pH between the association and dissociation phases to probe whether the added aggregate mass would be reduced at different rates upon washing with buffer at pH 6·5, depending on the pH value during mass association. The QCM-D results reveal that part of the mass associated with the surface-bound fibrils at low pH, dissociates upon pH increase, which is likely due to release of protein that is relatively weakly attached to the surface of the fibrils, i.e. monomeric protein or indeed already formed secondary nuclei. On the other hand, at pH > 6·0 mostly elongation occurs, and monomers dissociate very slowly upon washing due to the high thermodynamic stability of the fibrils (Baldwin et al. Reference Baldwin, Knowles, Tartaglia, Fitzpatrick, Devlin, Shammas, Waudby, Mossuto, Meehan, Gras, Christodoulou, Anthony-Cahill, Barker, Vendruscolo and Dobson2011). The QCM-D experiments, also support that nucleation of new fibrils from surface-bound monomers is the most likely secondary process at mildly acidic pH. The dependence on pH of α-syn monomer surface affinity was also evident in the two-color dSTORM images. Here, it was clearly shown that at mildly acidic pH conditions, a larger proportion of monomer is bound at the surface along the seed fibrils, opposing to neutral conditions, where monomer has higher affinity for the growth-competent fibril-free ends (Pinotsi et al. Reference Pinotsi, Buell, Galvagnion, Dobson, Schierle and Kaminski2014).

In summary, the combination of experiments presented here very strongly suggests that the nucleation of monomers on fibril surfaces is the secondary process that dominates the aggregation mechanism for α-syn at pH < 6·0. Thus, at mildly acidic pH the aggregation of α-syn follows the same mechanism as previously found for insulin (Foderà et al. Reference Foderà, Librizzi, Groenning, van de Weert and Leone2008), IAPP (Padrick & Miranker, Reference Padrick and Miranker2002) and the amyloid β peptide, Aβ (Cohen et al. Reference Cohen, Linse, Luheshi, Hellstrand, White, Rajan, Otzen, Vendruscolo, Dobson and Knowles2013; Meisl et al. Reference Meisl, Yang, Hellstrand, Frohm, Kirkegaard, Cohen, Dobson, Linse and Knowles2014). Although surface catalyzed secondary nucleation dominates the aggregation process for Aβ also at basic pH, a reduction in pH lowers the electrostatic repulsion between monomers and fibrils leading to enhanced secondary nucleation (Meisl et al. Reference Meisl, Yang, Frohm, Knowles and Linse2016b). α-Syn has a pI of 4·7 (Uversky et al. Reference Uversky, Li and Fink2001) and carries a net negative charge at neutral pH. The sequence is separated into three distinct regions, with a large number of charged residues in the N- and C-terminal regions and a higher fraction of hydrophobic residues in the central region. Interactions involving hydrophobic groups may play a significant role at all pH values, but at neutral pH, there is significant electrostatic repulsion between monomers, as well as, between monomers and fibrils. The charge of the residues in the termini is modulated by pH and therefore the electrostatic interactions between monomers and fibrils are likely to have strong pH dependence. This may underlie the observed pH dependence of secondary nucleation (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014).

It can be postulated that changes in pH between different cellular environments may affect the rate of formation of potentially cytotoxic oligomeric species, as observed under the conditions studied here. Mildly acidic pH is found in many intracellular compartments, linked to the endocytic and exocytic pathways, making this set of conditions physiologically relevant. In vitro studies at mildly acidic pH can thus bring new insights into the microscopic steps underlying the aggregation mechanism of α-syn, and in particular, aggregate multiplication in the brain (Buell et al. Reference Buell, Galvagnion, Gaspar, Sparr, Vendruscolo, Knowles, Linse and Dobson2014). The secondary nucleation process of α-syn monomers on fibril surfaces described here is an autocatalytic process, which constitutes a double threat; it increases rapidly both the total load of fibril mass and the amount of smaller oligomeric species that are thought to be the main responsible agents for cytotoxicity (Xue et al. Reference Xue, Hellewell, Gosal, Homans, Hewitt and Radford2009). Since secondary nucleation appears as the dominant route to α-syn aggregation at mildly acidic pH, this reaction can be considered a future therapeutic target for development of small molecular inhibitors or using certain chaperones that have been successfully shown to inhibit this specific microscopic process for the Aβ peptide (Cohen et al. Reference Cohen, Arosio, Presto, Kurudenkandy, Biverstål, Dolfe, Dunning, Yang, Frohm, Vendruscolo, Johansson, Dobson, Fisahn, Knowles and Linse2015).

5. Material and method section

5.1. Recombinant α-syn peptide expression and purification

Human α-syn WT and α-syn cysteine variant (N122C) were expressed and purified using heat treatment, ion exchange and gel filtration chromatography as described previously (Grey et al. Reference Grey, Linse, Nilsson, Brundin and Sparr2011) (S1). Labeling of α-syn cysteine variant (N122C) with Alexa Fluor 647 and Alexa Fluor 568 was performed as previously reported (Pinotsi et al. Reference Pinotsi, Buell, Galvagnion, Dobson, Schierle and Kaminski2014) (S6).

5.2. ThT kinetic experiments

A key factor in achieving reproducible kinetics is to use pure monomeric α-syn as starting material. Prior to setting up any kinetic measurement, the frozen aliquots were purified with a final size exclusion chromatography run in 10 mM MES pH 5·5 (standard condition) were the central region of the peak is collected in order to assure the presence of only monomeric species (S1). The protein concentration was determined by measuring the UV absorbance at 280 nm and using the extinction coefficient ε 280 = 5800 l mol−1 cm−1. Buffer solutions were filtered and degassed before each run. The isolated monomeric α-syn was always kept on ice to prevent aggregation.

To follow the fibrillation process, samples were aliquoted in 96-well plates with a non-binding surface (black PS plates treated with a PEGylated surface, half-area, 3881 Corning), supplemented with 20 µM of ThT and sealed with a plastic film to avoid evaporation. With the exception being for the experiment to investigate the role of surfaces on α-syn aggregation shown in S3, were also non-treated surface (black PS plates, full volumes, 3631 Costar) were used. The optimal concentration for ThT (20 µM) was accessed to have a linear relationship between fluorescence intensity and aggregate concentration (S2). Plates were incubated at 37 °C up to 100 h in a plate reader (FluoStar Omega or FluoStar Galaxy, BMG Labtech, Offenburg, Germany) under quiescent conditions (excitation filter 440 nm and emission filter 480 nm).

5.3. Preparation of α-syn seed fibrils

α-Syn seed fibrils were formed in Eppendorf tubes (Axygen low-bind tubes) at 37 °C, with low stirring speed (300 rpm) with a teflon bar and left fibrillating for up to 48 h. Parallel kinetic ThT measurements were performed to assure that the plateau was reached during this time period. Before each kinetic experiment, seed fibrils were pre-treated by 1 min continuous sonication at maximum power in a sonicator bath (Struer, Copenhagen, DK) to disperse lumped fibrils. The concentration of seeds is counted as monomer equivalents.

5.4. Differential sedimentation method

In order to measure retentions times of the main populations of mature fibrils as a function of time a sedimentation analysis was performed using a CPS disc centrifuge instrument model DC24000. The instrument was operated at 13 782 rpm and a 4 to 12% sucrose gradient was cast in the spin fluid (Milli-Q water). Dodecane was added last to the gradient to extend its lifetime. Calibration was done with polyvinyl chloride particles with a weight-average diameter of 483 nm, and 100 µl samples were injected.

5.5. Trap and seed

Fibrils were made from 20 µM monomeric α-syn in the presence of 3 µM seeds under quiescent conditions at 37 °C in non-binding PEGylated plates. The fibrils were trapped on the filter membranes (retentate) by filtration applying vacuum for 10 s on a low-binding AcroPrep 96-well filter plate (plate housing – Polypropylene) embedded with a Versatile GH Polypro membrane (GHP – hydrophilic Polypropylene membrane) (Pall Life Sciences, Ann Arbor, MI). The flow through was collected in a 96-well non-binding PEGylated plate (filtrates). The filtration was done using a MultiScreenHTS vacuum (Millipore) manifold. Before loading the seed samples, the GHP filter membrane of the multi-well plate was washed with experimental buffer. The fluorescence intensity of ThT of each filtrate collected in the non-binding PEGylated plates was monitored in a plate reader at 37 °C under quiescent conditions.

5.6. QCM-D measurements

The QCM-D measurements were performed with an E4 instrument (Q-Sense, Västra Frölunda, Sweden). α-Syn fibrils were produced and attached to the gold-coated surface of a quartz sensor (QSX 301) as previously described (Buell et al. Reference Buell, White, Meier, Welland, Knowles and Dobson2010b, Reference Buell, Dobson and Welland2012) (S4). For the main experiments, the sensors were incubated with solutions of 20 µM monomeric α-syn in 10 mM MES buffer at the pH values of 5·5, 5·7, 5·9, 6·1 and 6·5. When the frequency shift had reached approximately 420 Hz in the frequency overtone N = 3, the sensor surface was washed with 10 mM MES buffer at pH 6·5.

5.7. Two-color super-resolution microscopy using dSTORM

Two-color super-resolution microscopy was performed on an inverted total internal reflectance fluorescence microscope which was custom-built for dSTORM imaging, as described previously (Kaminski Schierle et al. Reference Kaminski Schierle, van de Lind, Erdely, Esbjörner, Klein, Rees, Bertoncini, Dobson, Sauer and Kaminski2011; Pinotsi et al. Reference Pinotsi, Buell, Galvagnion, Dobson, Schierle and Kaminski2014). Alexa Fluor 647 and 568 dyes were excited using a 640 nm diode laser (Toptica) and a 561 nm DPSS laser (Oxxius), respectively with an irradiance between 1 and 5 kW cm−2, and a 405 nm laser diode was used as a reactivation source. The fluorescence was collected with a 100X/1·49 NA objective (Nikon) onto an EMCCD camera (iXon3 897, Andor). To induce photoswitching of the dye the fibrils were immersed in a switching buffer consisting of 100 mM mercaptoethylamine (Sigma) in PBS at pH 8·2 supplemented with an oxygen scavenger to reduce photobleaching (40 mg ml−1 glucose, 50 µg ml−1 glucose oxidase, 1 µg ml−1 catalase). The red and green channels were imaged sequentially, and for each field of view, a series of 10–15 000 frames was acquired with 15 ms exposure time. The acquired dSTORM datasets were analyzed using rapidSTORM 3·3 (Wolter et al. Reference Wolter, Löschberger, Holm, Aufmkolk, Dabauvalle, van de Linde and Sauer2012) and super-resolution images were generated using a pixel size of 30 nm pixel−1 for both channels. Seeds with different labeling densities were tested for image optimization. Also, these dye labels were evaluated in terms of interfering with the aggregation process using ThT kinetics studies. It was shown that a 1:20 ratio of labeled α-syn to unlabeled peptide was the optimal in terms of labeling density and unperturbed aggregation kinetics (S7).

Supplementary Material

To view supplementary material for this article, please visit https://doi.org/10.1017/S0033583516000172

Acknowledgements

This work was supported by the Swedish Research Council and its Linneaus Centers for Organizing Molecular Matter (E. Sparr and S. Linse), the European Research Council (S. Linse), Nanolund (S. Linse), Multipark (S. Linse and R. Gaspar), the Leverhulme Trust (A. Buell), Magdalene College, Cambridge (A. Buell), the Parkinson's and Movement Disorder Foundation (A. Buell), EPSRC (C.F. Kaminski), MRC (C.F. Kaminski) and Wellcome Trust UK (C.F. Kaminski). We thank Gunnel Karlsson for the expert help with Cryo-TEM, C. Galvagnion and C.M. Dobson for kindly providing the plasmid for α-syn cysteine variant (N122C) expression, G. Schierle Kaminski for helpful inputs and discussions concerning the dSTORM experiments and we would also like to acknowledge K. Sanagavarapu, X. Yang, M. Tornqvist, N. Yu and W.Y. Chen for the support given during the dStorm imaging. We also acknowledge T. Cedervall and S. Gunnarsson for expert help with the fibril sedimentation analysis.

Author Contributions

R.G., A.K.B, C.K., T.P.J.K., E.S. and S.L. designed the experiments. R.G., A.K.B. and L.Y. performed the experiments. R.G., A.K.B., G.M., L.Y., T.P.J.K, E.S. and S.L. analyzed data. R.G., E.S. and S.L. wrote the paper. All authors contributed to the manuscript writing and revision.

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Figure 0

Fig. 1. Schematic depictions of the two possible secondary processes in the aggregation of α-syn at mildly acidic pH conditions. (a) Fibrils multiply through fragmentation. (b) Fibrils catalyze the formation of new aggregates from monomer on their surface. In a saturated secondary nucleation reaction the initial monomer-dependent (attachment) step is so fast that the second monomer-independent (rearrangement or detachment) step becomes the rate determining step (RDS).

Figure 1

Fig. 2. Seeded α-syn aggregation kinetics. The monomer concentration was systematically varied in the range of 1–50 µM in the presence of three different seed concentrations: (a) 3 µM, (b) 1 µM and (c) 0·3 µM in 10 mM MES pH 5·5 at 37 °C under quiescent conditions. For each solution condition three traces are shown in bold circles. The figures show ThT intensity as a function of time (non-normalized raw data). Different microscopic mechanistic events lead to overall different observable macroscopic kinetic profiles, as shown through simulated traces for the case of monomer concentration variation in the presence of 1 µM seed (experimental data shown in 2b) for the different kinetic models tested, (d) only primary nucleation and elongation, (e) dominant fragmentation and (f) dominant saturated secondary nucleation.

Figure 2

Fig. 3. Seeding efficiency in α-syn aggregation. (a–c) Representative seeded aggregation kinetic traces in the presence of fixed (3, 1, 0·3 and 0 µM) seed concentrations incubated with (a) 50 µM, (b): 10 µM and (c) 5 µM α-syn monomer. For each condition three traces are shown in bold circles. (d) Aggregation with systematic variation of α-syn seed concentration from 0 to 20% in the presence of a fixed α-syn monomer concentration (20 µM). Averages of three traces are shown as solid lines. All figures show ThT intensity as a function of time (non-normalized raw data). Therefore, experiments in the presence of seeds show elevated ThT intensity at time zero. All experiments were performed in 10 mM MES pH 5·5 in non-binding PEGylated plates at 37 °C and under quiescent conditions.

Figure 3

Fig. 4. Experiments designed to identify the dominant secondary process of α-syn aggregation at mildly acidic pH conditions. (a) Time-dependent differential sedimentation analysis performed on fibrils incubated at 37 °C under quiescent conditions in 10 mM MES buffer pH 5·5 for 1–20 days. Aggregates sediment within a sucrose gradient on a rotating disc where longer retention times correspond to smaller size aggregates. The raw data is shown to the left and processed data to the right. The calculations of relative weight and size are made under the assumption of spherical particles, which leads to an underestimation of the size and relative weight for a fibrillar particle. Nevertheless, changes in size distribution can be detected, which was the purpose of this experiment. The figures show representative traces of each condition that was repeated at least two times. (b) Trap and seed kinetic experiment. Fibrils made from 20 µM α-syn monomer supplemented with 3 µM seed fibrils in 10 mM MES pH 5·5 were trapped by filtration in filter plates and the flow-through (filtrate 1) was collected in non-binding PEGylated plates, supplemented with ThT and monitored in a plate reader (B1). The trapped fibrils were then incubated for 2 h with concentrations ranging from 10 to 50 µM α-syn monomer or 10 mM MES buffer pH 5·5 and newly filtered (filtrates 2 and 3, respectively). Again, the flow-through was collected in non-binding PEGylated plates, supplemented with ThT and monitored (B2 and B3). The figures show averages of at least four traces that are shown in bold with individual traces dotted below and are plotted as ThT intensity as a function of time (non-normalized data).

Figure 4

Fig. 5. The surface of α-syn amyloid fibrils shows a pH-dependent affinity for monomeric α-syn. (a) Fibrils of α-syn were immobilized on gold-coated QCM-D sensor crystals and incubated with 20 µM monomeric α-syn in 10 mM MES buffer at different pH values until a certain frequency shift was reached (ca. −420 Hz for overtone N = 3). The sensors were then washed with 10 mM MES pH 6·5 (indicated by arrows), leading to different levels of dissociation of the previously attached material. (b) Scheme of what is postulated to occur on the sensors for the conditions of pH < 6·0 and pH > 6·0. The orange stars represent binding to the surface of the fibrils.

Figure 5

Fig. 6. dSTORM images of amyloid growth from seed fibrils at mildly acidic pH conditions. (a) Imaged preformed seed fibrils of α-syn N122C labeled with 1:20 AF647 used for the self-seeding experiment. (b, c) α-Syn monomer labeled with AF568 (green) was incubated with 50% seed fibrils labeled with AF647 (purple). The top panel is imaged in the red channel, middle panel imaged in the green channel and the bottom panel is the merge between both channels. Scale bar corresponds to 1 µm.

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