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MAK33 antibody light chain amyloid fibrils are similar to oligomeric precursors

MAK33 antibody light chain amyloid fibrils are similar to oligomeric precursors Little structural information is available so far on amyloid fibrils consisting of immunoglobulin light chains. It is not understood which features of the primary sequence of the protein result OPENACCESS in fibril formation. We report here MAS solid-state NMR studies to identify the structured Citation: Hora M, Sarkar R, Morris V, Xue K, Prade core ofκ-type variable domain light chain fibrils. The core contains residues of the CDR2 E, Harding E, et al. (2017) MAK33 antibody light and theβ-strands D, E, F and G of the native immunoglobulin fold. The assigned core region chain amyloid fibrils are similar to oligomeric precursors. PLoS ONE 12(7): e0181799. https:// of the fibril is distinct in comparison to the core identified in a previous solid-state NMR study doi.org/10.1371/journal.pone.0181799 on AL-09 by Piehl at. al, suggesting that V fibrils can adopt different topologies. In addition, Editor: Patrick van der Wel, University of we investigated a soluble oligomeric intermediate state, previously termed the alternatively Pittsburgh School of Medicine, UNITED STATES folded state (AFS), using NMR and FTIR spectroscopy. The NMR oligomer spectra display Received: April 9, 2017 a high degree of similarity when compared to the fibril spectra, indicating a high structural similarity of the two aggregation states. Based on comparison to the native state NMR Accepted: July 9, 2017 chemical shifts, we suggest that fibril formation via domain-swapping seems unlikely. More- Published: July 26, 2017 over, we used our results to test the quality of different amyloid prediction algorithms. Copyright:© 2017 Hora 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. Introduction Data Availability Statement: NMR data are Antibody light chain amyloidosis (AL amyloidosis) is a rare disease caused by amyloid forma- available from the BioMagResBank (BMRB ID 27065; URL: http://www.bmrb.wisc.edu/). tion of immunoglobulin light chains (LCs) [1,2]. An underlying B-cell dyscrasia causes over- production and secretion of LCs. In the case of an aggregation-prone LC sequence, this can Funding: This work was supported by a grant from result in formation of oligomeric intermediates and further of fibrils, which deposit in the the German Bundesministerium fu Èr Bildung und Forschung (BMBF) within the network GERAMY. inner organs, causing systemic amyloidosis. Heart failure is the dominant cause of death [3,4]. We acknowledge support of the Helmholtz- The 4-year overall-survival rate is on the order of 33% [5]. Gemeinschaft, the German Research Foundation Non-fibrillar oligomers have aroused interest of the research community due to their cyto- (DFG, Grant Re1435, to B.R.) and the Center for toxicity as well as their role as folding intermediates [6]. Oligomers have been reported for sev- Integrated Protein Science Munich (CIPS-M). The eral amyloid-forming proteins and peptides [7]. In many cases, these oligomers appear to be DFG and the Technical University of Munich (TUM) supported the open access publication in the the most cytotoxic species [8,9]. The mechanism of cytotoxicity is likely due to membrane PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 1 / 14 AL fibrils are similar to AL oligomers framework of the Open Access Publishing pore formation [10,11]. Nonetheless, fibrils also exhibit toxicity [12]. In AL amyloidosis, both Program. The funders had no role in study design, oligomers and fibrils have been found to be cytotoxic, affecting the cardiomyocyte metabolism data collection and analysis, decision to publish, or [13,14]. preparation of the manuscript. Despite the relevance of LC oligomers and fibrils for disease, little is known about their Competing interests: The authors have declared structures. AL fibrils are composed of proteins containing mostly variable domain (V ) resi- that no competing interests exist. dues [1]. However, aggregates can also contain LC protein including constant domain (C ) residues [1]. The N-terminal part of the V domain seems to be structured in the fibrils [15,16]. Cryo-EM has been used to determine the steric zipper structure of an AL-protein derived 12-residue peptide fibril [17]. Recently, magic-angle-spinning solid-state NMR (MAS ssNMR) chemical shift assignments and a secondary structure analysis were reported for the κI sequence AL-09 [18,19]. We report here a MAS ssNMR spectroscopic analysis of amyloid fibrils and oligomers formed by the V domain of MAK33. The murineκ-type V domain of MAK33 has been stud- L L ied extensively regarding its native structure [20], biophysical properties and folding pathways [21,22]. Several point mutations facilitate fibril formation [23±26]. We employed the amyloi- dogenic mutant MAK33 V S20N [25] to study amyloid fibrils with MAS ssNMR. We were able to identify the structured hydrophobic core region, which comprises mainly residues 60± 87. Oligomeric intermediates tend to be short-lived and thus difficult to investigate. In con- trast, the MAK33 V domain forms stable high-molecular weight oligomers at pH 2, which were previously referred to as alternatively folded state (AFS) [21]. These non-fibrillar oligo- mers were studied with MAS ssNMR, Fourier-transform infrared spectroscopy (FTIR) and transmission electron microscopy (TEM). MAS ssNMR revealed an astonishing similarity of the oligomer and the fibril chemical shifts, indicating a high degree of structural similarity. In contrast, secondary chemical shifts of the fibrils show no correlation with those of the native state, suggesting that fibril formation does not proceed via a domain swapping mechanism. Results In order to investigate AL fibril structure, we employed seeded fibrils of the MAK33 V S20N protein. Two independent fibril preparations yielded highly reproducible MAS ssNMR spectra 13 15 (Fig 1). Fig 1A shows a 2D-N(CA)CX correlation spectrum obtained from uniformly C, N 13 13 labeled protein and Fig 1B a 2D-NCA spectrum for a C-spin dilute sample. Due to sparse C labeling of the 2- C-glycerole labeled sample, fewer cross peaks were obtained [27]. Except for this observation, however, the two preparations produced identical NMR spectra. In Fig 1B, assignments were transferred directly from the spectrum of the uniformly C labeled sample without moving the position of the crosses. Considering the common problem of fibril poly- morphism [28], such reproducibility is an important prerequisite for further structural analysis. The assignment of the structured parts of the MAK33 V S20N fibrils was accomplished using a variety of MAS ssNMR experiments: PDSD [29], NCACX, NCOCX [30], NCACB, N (CO)CACB, NCOCA and CANCO [31]. A detailed list of all experimental settings is given in the Supporting Information (S1 Table). In total, 36 residues were assigned sequentially, com- prising residues 49±52 (located in the complementarity determining region 2 (CDR2) of the native state), residues 60±87 (β-strands D, E and F) and residues 98±101 (β-strand G). For all these residues, only a single set of resonances was observed, indicating that the preparations contained only one fibril polymorph. Chemical shift assignments were deposited in the Bio- 13 15 MagResBank (BMRB ID 27065). The C and N linewidths were both on the order of 1 ppm at a 750 MHz spectrometer. In particular, the N transverse relaxation time of 9 ms indicated PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 2 / 14 AL fibrils are similar to AL oligomers 13 15 13 15 13 Fig 1. C, N correlations of MAK33 V S20N fibrils. A) N(CA)CX spectrum of a u- C, N labeled sample. B) NCA spectrum of a 2- C-glycerole isotope labeled sample. Peak positions are identical in A) and B), indicating good reproducibility. The resolution in B) is increased due to sparse isotope labeling. https://doi.org/10.1371/journal.pone.0181799.g001 a high quality of the sample, i.e. a high degree of homogeneity. Representative strip plots of the assignment are shown in S1 Fig. The secondary chemical shift analysis indicates that MAK33 V S20N populates mostlyβ- strands in the fibril state, as expected for amyloid fibers. Using TALOS+ [32], we identified fourβ-strands, with regions of random coil conformation in between them (Fig 2, for Cα, Cβ and CO secondary chemical shifts, see S2 Fig). Twenty additional spin systems could be observed, but not assigned, due to low signal intensities. As signal intensity correlates with rigidity in dipolar-based MAS ssNMR experiments, we assumed that these twenty residues were less structured and located in the flanking region of the core structure. Dynamic residues cannot be observed with the dipolar-based MAS ssNMR experiments employed here. For complementarity, we conducted an INEPT experiment based on scalar couplings, which is suited to detect highly flexible residues. The resulting spectrum did not yield observable cross peaks (S3 Fig). Therefore, we assume that the remaining residues exhibit dynamics on an intermediate time scale, which can be observed neither with INEPT nor with dipolar-coupling based experiments. Alternatively, the respective residues might be structur- ally heterogeneous. Having identified the core of the fibrils, we aimed at a comparison with the oligomeric intermediates that are formed during aggregation. While oligomers are typically short-lived and thus difficult to study, MAK33 V forms stable oligomers at acidic pH (Fig 3A) [21]. An electron microscopic analysis of the oligomers revealed an irregular morphology, but a rather homogeneous size distribution (Fig 3B). The mean diameter of the particles was 9.9 ± 1.5 nm, suggesting in average 30 monomers per oligomer (S4 Fig). This is in excellent agreement with previous studies using analytical ultracentrifugation, which yielded 17 to 42 monomers per oligomer [22]. Upon shaking at 37ÊC, the oligomers transform to well-structured fibrils within 24 hours (Fig 3C). Using FTIR (Fig 3D), both samples displayed similar peaks, with maxima at PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 3 / 14 AL fibrils are similar to AL oligomers Fig 2. Secondary structure analysis of MAK33 V in the fibril state. A)β-sheet propensity calculated with TALOS+ [32]. B) Sequence and secondary structure elements of the native V fold. Green and red bars indicateβ-strands and CDRs of the native structure, respectively. Red arrows below the sequence indicateβ-strands in the fibril state. The expansion shows the assigned atoms in the aggregated state. https://doi.org/10.1371/journal.pone.0181799.g002 -1 -1 1619 cm (oligomers) and 1621 cm (fibrils). Amyloid fibrils yield characteristic FTIR max- -1 -1 ima between 1611 cm and 1630 cm , whereas peaks of nativeβ-sheet proteins are typically -1 -1 found in the range from 1630 cm to 1643 cm [33,34]. Hence, the oligomers differ from the native state and resemble the fibrils at the level of secondary structure. The oligomer FTIR -1 spectrum also displayed a less pronounced peak at 1697 cm . This peak is characteristic for oligomers [35]. We employed MAS solid-state NMR to investigate the V oligomer structure. Using FROS- 13 13 TY-NMR [36], a PDSD C, C-correlation of the MAK33 V WT oligomers was acquired. The similarity between the oligomer and the fibril spectrum is striking (Fig 3E). The chemical PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 4 / 14 AL fibrils are similar to AL oligomers Fig 3. Comparison of MAK33 V oligomers and fibrils. A) Procedure to form oligomers and fibrils. B), C) Electron micrographs of MAK33 V L L S20N oligomers (B) and fibrils (C). The scale bar denotes 200 nm. D) FTIR spectra of MAK33 V S20N oligomers and fibrils. The peak maxima -1 -1 -1 were 1619 cm (oligomers) and 1621 cm (fibrils), respectively. The oligomer spectrum displayed an additional peak at 1697 cm . E) PDSD 13 13 C, C-intraresidue correlations of MAK33 V S20N fibrils and MAK33 V WT oligomers. The proline spin system, which is more intense in the L L oligomers, is highlighted in blue. https://doi.org/10.1371/journal.pone.0181799.g003 shift patterns for many spin systems were very similar. The oligomer resonances were broader in general, which is in good agreement with a less well-defined structure. Some fibril reso- nances are missing in the oligomer spectrum, which is presumably due to dynamics, resulting in reduced sensitivity. Spectral differences are expected, since oligomers and fibrils show clearly distinct morphologies. The resonances of residues I75, S77, V78, E79 and T80 are miss- ing in the oligomer spectrum and the presence of N76 is unclear due to spectral overlap. In the fibrils, this region corresponds to a loop connecting twoβ-strands (Fig 2). In the oligomers, this loop might adopt a different conformation or experiences a different chemical environment. Nevertheless, the similarity of both spectra indicates that the secondary and tertiary struc- tures of the oligomeric and the fibril state are highly similar. We could identify only one spin system, which clearly has a higher signal intensity in the oligomer state than in the fibril state. This spin system corresponded to a proline residue. The proline is presumably in a trans con- formation, as the Cβ and Cγ shifts were approximately 30.3 ppm and 25.5 ppm, respectively [37]. MAK33 V contains five prolines, at positions 8, 15, 44, 59 and 95. However, due to lack of sequential connectivities, we could not assign this proline spin system to one of the five PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 5 / 14 AL fibrils are similar to AL oligomers prolines in the primary structure of MAK33 V . Considering which regions of the sequence were assigned, it is likely to be either P44, P59 or P95. The change in NMR signal intensity of this residue suggests that the dynamics of this proline residue increase when the oligomer structure is converted into the fibril state. Proline isomerisation is critical during the initial folding of MAK33 V [38,39]. Prolines have been reported previously as important switches for amyloid formation in the case ofβ2-microglobulin [40]. In the case of the amyloidogenic V domain AL-103, the presence of two consecutive prolines at positions 95 and 95a affects both the kinetic stability and fibril formation [41]. Further analysis of the proline isomerisation states are needed to yield a better understanding of their role in AL amyloid formation. Discussion Here we reported on the structured core residues of an immunoglobulin V -κ sequence in the amyloid fibril and oligomeric state. Considering the tremendous variability of antibody sequences, it is interesting whether these results are transferable to other light chain sequences. In the AL-09 fibril sample studied by Piehl et al. [18,19], the structured regions comprised mostly the first 30 N-terminal residues as well as residues 94±107 at the C-terminus. In between, only a few residues could be assigned. It is surprising that the assigned regions differ considerably compared to our sequence (Fig 4A). In both studies, several residues could not be assigned sequentially, so there might be more overlap in the hydrophobic core regions. We emphasise however, that intense resonances, which are easier to assign, correlate with rigid structure. In this regard, the differences with respect to assigned regions are meaningful and indicate distinct topologies for the fibril states of both V sequences. Recently, LC amyloid deposits with distinct morphologies were found in ex vivo tissue samples of one individual patient [42]. In this sense, the V fibril structure is polymorphic due to growth conditions and tissue specific factors, in addition to the structural diversity which is presumably induced by differences in the sequence. Piehl et al. have previously pointed out that most of the non-conservative mutations in AL- 09 are located outside of the assigned and thus structured regions [18]. Similarly, the amyloid- enhancing mutation S20N employed here for MAK33 is not part of the hydrophobic core identified in our study. These findings emphasise that point mutations, which are relevant for fibril formation, are not necessarily structured in the fibril state. On the other hand, the critical residue D70, which is part of a conserved salt bridge is located within the assigned regions [25]. Similarly, the highly amyloidogenic V -λ6 subtype differs from less amyloidogenic vari- ants by an insertion at positions 68 and 69 [43,44], which, according to our findings, is located in the fibril core. Understanding of amyloidogenicity of antibody LC sequences cannot be complete without considering the fibril structure and requires further ssNMR studies. In this study, we investigated a murine VL sequence. To find out if the murine framework is comparable to human pathological sequences, we compared the MAK VL with human VL sequences. The sequence identity between MAK33 VL and other patient-derived or patient- related sequences ranges from 40% to 60%. E. g. the sequence identity is 57% with respect to Sma [45], 44% in comparison to 6aJL2 [46], and 42% for Wil [47]. While these values might seem low, they are actually in the same order as the identities between different pathological human sequences: The identity between Sma and 6aJL2 is 46%, 45% for Sma and Wil, and 89% for the quite similarλ6 sequences 6aJL2 and Wil. Hence, the differences between our murine sequence and pathological sequences are not larger than the differences between patient-derived AL sequences of different light chain subgroups. We prepared our fibrils deliberately at pH 2, since acidic conditions are known to stabilise fibrils. pH 2 is necessary to form stable oligomers. Recently, ssNMR experiments have been PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 6 / 14 AL fibrils are similar to AL oligomers Fig 4. Comparison with AL-09, amyloid prediction algorithms and native state chemical shifts. A) Sequence alignment of MAK33 V S20N and AL-09 V : Identical residues are marked in blue. Residues assigned in MAS ssNMR spectra are indicated by bars above and below the corresponding sequence. B) Predictions of MAK33 V S20N amyloid propensity and experimentally observedβ-strands. C) Secondary chemical shift correlation of MAK33 V S20N in the solid-state (fibrils, pH 2) and solution-state (native, pH 6.5) for Cα, Cβ, CO and N chemical shifts. The cross-correlation coefficients r are indicated in each plot. https://doi.org/10.1371/journal.pone.0181799.g004 performed to identify the structured core residues in the VL-κ protein AL-09 fibril. Also in this study, fibrils were prepared at pH 2 [18,19]. Piehl et al compared those in vitro fibrils formed at acidic conditions with ex vivo fibrils derived from human spleen tissue. It is dis- cussed that NMR spectra from both samples are comparable. Hence, while acidic conditions PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 7 / 14 AL fibrils are similar to AL oligomers are not physiological, they represent a necessary experimental requirement for the investiga- tion of fibrillised VL protein by ssNMR. The vast number of different V sequences that can form fibrils makes a structural charac- terisation of all antibody fibrils by ssNMR impractical. Therefore, predictions of amyloido- genic regions can be a precious tool to study a multitude of sequences. We compared our MAS ssNMR results with the predictions from three web tools (Fig 4B). In our benchmark, we included Aggrescan [48], Tango [49] and Zyggregator [50]. Of the fourβ-strands identified by MAS ssNMR, all algorithms identified the two longer C-terminalβ-strands between residues 70 and 90. Our first N-terminalβ-strand was only predicted by Aggrescan, the second one only with low propensity by Zyggregator. All programs predicted moderate aggregation pro- pensities in the N-terminal region (residues 1±30), where we could not assign any resonances. Our assignments are incomplete and we cannot exclude the presence of further structured regions. In fact, a structured N-terminus of V fibrils has also been suggested for other V L L sequences [15,16]. To summarise, all three algorithms could correctly predict the two longer β-strands. We therefore believe that prediction of amyloid propensity will be a valuable tool to study VL sequences in the future. In the past, domain swapping has been suggested as a mechanism to explain immunoglobu- lin light chain deposition [51,52]. In this context, it has been shown that the amyloid core of transthyretin consists of native-likeβ-sheets [53]. We analysed NMR secondary chemical shifts, which report on secondary structure elements. If the conformation of MAK33 V S20N in the fibril state resembled the conformation of this point mutant in the native structure, the secondary chemical shifts of the solid-state and solution-state preparations should be similar. Fig 4C shows correlation plots of the Cα, Cβ, CO and N secondary chemical shifts. We can not observe a correlation between native and fibril secondary structure for any of the nuclei assigned in both conformations. Hence, we conclude the fibrils studied here were not formed by domain swapping. Similar discrepancies between native and fibril states were reported recently for AL-09 V [19], supporting the hypothesis that AL fibrils do not form via a domain-swapping mechanism. Our data alternatively indicate that the native MAK33 V at least partially unfolds and undergoes a transformation to a distinct oligomeric state. While the morphology according to TEM differs from mature fibrils, the local chemical environment is rather similar, as reflected by the NMR chemical shifts. Along the same lines, NMR spectra for oligomer and protofibril preparations have been reported for amyloid-β [54]. Our FTIR experiment with the oligomers -1 displayed a characteristic peak at 1697 cm . While there are still disputes about determination ofβ-sheet arrangements with FTIR [35], according to theoretical derivations, this band might indicate anti-parallelβ-sheets [55]. The fibrils, in contrast, do not produce this FTIR peak and thus likely contain the typical parallelβ-sheets [56]. Different orientations ofβ-strands in olig- omers and fibrils are in agreement with literature [35,57,58]. It will be interesting to see, whether these observations on MAK33 V oligomers and fibrils are also true for other light chain amyloid sequences. With the recent advances in MAS ssNMR structure determinations of fibrils [59,60] and the now available assignments of V fibrils, a structure comes within reach. We expect this will be an important contribution to predict which V sequences are prone to fibril formation and how the oligomers and fibrils can be cleared. Material and methods If not specified otherwise, all chemicals were purchased from Sigma Aldrich (Taufkirchen, Germany). PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 8 / 14 AL fibrils are similar to AL oligomers Recombinant protein production MAK33 V WT and S20N were purified as described previously [25]. Briefly, E.coli BL21 with a pET28 vector containing the MAK V gene were grown in M9 minimal medium supple- L Kan 13 15 mented with 2 g/l C-glucose and 0.5 g/l NH Cl. Expression was induced with 1 mM IPTG at OD 0.6±0.8. After over night expression at 37ÊC, cells were harvested and inclusion bodies were isolated. The inclusion bodies were dissolved in a buffer consisting of 50 mM Tris, 5 mM EDTA, 8 M urea and 1%β-mercaptoethanol (pH 8). The dissolved protein was subjected to anion exchange chromatography, using a 16 / 10 Q Sepharose High Performance column (GE Healthcare, Munich, Germany) using a buffer consisting of 25 mM Tris, 5 mM EDTA and 5 M urea (pH 8). The V protein eluted in the flowthrough. Refolding was achieved by over- night dialysis into a buffer containing 250 mM Tris, 5 mM EDTA, 100 mM L-arginine, 1mM oxidised glutathione und 0.5 mM reduced glutathione (pH 8, 4ÊC). Finally, the protein was purified using gel filtration chromatography with a HiLoad 16/600 Superdex 75 prep grade column (GE Healthcare, Munich, Germany) and a buffer consisting of 20 mM sodium phos- phate and 50 mM NaCl (pH 6.5). Total yield was 15±20 mg protein per liter of culture. Oligomer and fibril preparation The buffer was thoroughly exchanged to 25 mM acetic acid, 25 mM phosphoric acid and 50 mM NaCl (pH 2). Protein monomer concentration was set to 50 μM. 0.05% NaN was supple- mented to protect against bacterial growth. In order to obtain non-fibrillar oligomers, the solu- tion was incubated at room temperature under quiescent conditions. For fibril formation, the solution was incubated at 37ÊC at 350 rpm. Fibrils formed within one week. The outcome was confirmed by TEM. To enrich a single polymorph, fibrils were seeded for several generations. Approximately 2% of preformed fibrils were added to a new batch set up for fibril formation. th Samples used for MAS ssNMR analysis were from 7 or later generation of continuous seed- ing, with each seeding step incubating for one week. MAS solid-state NMR sample preparation An OptimaL-100 XP ultracentrifuge (Beckman Coulter, Krefeld, Germany) equipped with an SW 32 Ti swinging bucket rotor and a rotor filling device (Giotto Biotech, Florence, Italy) were used to pack the protein aggregate into an MAS rotor. The rotation frequency of the centrifuge was set to 28,000 rpm. Samples were packed into 3.2 mm thin wall ZrO rotors with vespel caps (CortecNet, Voisins Le Bretonneux, France) employing house-made teflon spacers. MAS solid-state NMR experiments All MAS ssNMR experiments were recorded using a 750 MHz Bruker Avance III spectrometer (Bruker BioSpin, Karlsruhe) equipped with a triple-resonance MAS probe for 3.2 mm rotors. The set temperature of the probe was adjusted to 273 K. The MAS frequency was set to 10 kHz (for PDSD, NCACX, NCOCX) or 17 kHz (NCOCA, CANCO, NCACB, NCOCAB, INEPT). Detailed settings for the experiments are given in the Supplementary Information (S1 Table). The building blocks for the experiments were PDSD, SPECIFIC-CP [61], BSH-CP [62], DREAM [63] and INEPT. The pulse sequences were implemented as described by Szeverenyi et al. [29] and Schu È tz et al. [31]. NCACX, NCOCX and NCACB were acquired with non-uni- form sampling to increase sensitivity [64]. Sparsity was set to 50% with exponentially decreas- ing sampling density, matched to the transverse relaxation time according to a spin echo experiment [65]. Experiments were acquired using Topspin 3.2 (Bruker BioSpin, Karlsruhe, Germany). Uniformly sampled experiments were processed with Topspin 3.2, nonuniformly PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 9 / 14 AL fibrils are similar to AL oligomers sampled spectra were processed either with the compressed sensing plugin of Topspin 3.2 or with hmsIST [66] in combination with NMRPipe [67]. All spectra were zero-filled to double the number of measured points and then the next power of two. Shifted squared cosine func- tions were employed for apodisation. Secondary chemical shifts were calculated as observed random coil Dd ˆ d d with random coil chemical shifts taken from the BMRB [68]. Negative-stain transmission electron microscopy Copper grids with 300 meshes coated with formvar/carbon film (Electron Microscopy Sci- ences, Hatfield, USA) were glow-discharged in argon atmosphere for 30 s at 3 mA. 5 μl of a 50 μM protein sample were incubated for 60 s on the grid. After removing the protein solution, the grid was washed with water. 5 μl uranyl acetate solution (2% w/v) were applied on the grid for staining and removed after 30 s. Photographs of the oligomers and fibrils converted from oligomers were measured on a Jeol JEM 1400 Plus transmission electron microscope (Jeol, Tokyo, Japan). Fourier-transform infrared spectroscopy Oligomer and fibril samples, 50 μM in fibril buffer (25 mM phosphoric acid, 25 mM acetic acid, 50 mM NaCl, 0.05% NaN , pH 2), were recorded on a JASCO FT/IR-4100 FT-IR spec- trometer (JASCO, Gross-Umstadt, Germany) with attenuated total reflectance (ATR) attach- -1 ment. The samples were measured with 128 scans at a resolution of 2 cm at room temperature. Spectra were buffer subtracted and smoothed using a Savitzky-Golan algorithm. Supporting information S1 Fig. Sequential walks from residues G64 to G68. (PDF) S2 Fig. Secondary chemical shifts of MAK33 V S20N fibrils. (PDF) 1 15 S3 Fig. H- N-INEPT experiment of MAK33 V S20N fibrils. (PDF) S4 Fig. Electron microscopic analysis of MAK33 V S20N oligomers. (PDF) S1 Table. ssNMR parameters. (XLS) Acknowledgments We thank Carsten Peters and Sevil Weinkauf for assistance with electron microscopy. Author Contributions Conceptualization: Manuel Hora, Johannes Buchner, Bernd Reif. Data curation: Manuel Hora. Formal analysis: Manuel Hora, Vanessa Morris. PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 10 / 14 AL fibrils are similar to AL oligomers Funding acquisition: Johannes Buchner, Bernd Reif. Investigation: Manuel Hora, Vanessa Morris, Elke Prade, Emma Harding. Methodology: Manuel Hora, Riddhiman Sarkar, Kai Xue. Project administration: Manuel Hora, Johannes Buchner, Bernd Reif. Supervision: Bernd Reif. Validation: Manuel Hora. Visualization: Manuel Hora. Writing ± original draft: Manuel Hora, Bernd Reif. Writing ± review & editing: Manuel Hora, Vanessa Morris, Elke Prade, Johannes Buchner, Bernd Reif. References 1. Desport E, Bridoux F, Sirac C, Delbes S, Bender S, Fernandez B, et al. AL Amyloidosis. Orphanet J Rare Dis. 2012; 7(54). 2. Ramirez-Alvarado M. Amyloid Formation in Light Chain Amyloidosis. Curr Top Med Chem. 2012; 12 (22):2523±33. PMID: 23339305 3. Merlini G, Seldin DC, Gertz MA. Amyloidosis: Pathogenesis and New Therapeutic Options. J Clin Oncol. 2011; 29(14):1924±33. https://doi.org/10.1200/JCO.2010.32.2271 PMID: 21483018 4. Huang X, Wang Q, Jiang S, Chen W, Zeng C, Liu Z. The clinical features and outcomes of systemic AL amyloidosis: a cohort of 231 Chinese patients. 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MAK33 antibody light chain amyloid fibrils are similar to oligomeric precursors

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Abstract

Little structural information is available so far on amyloid fibrils consisting of immunoglobulin light chains. It is not understood which features of the primary sequence of the protein result OPENACCESS in fibril formation. We report here MAS solid-state NMR studies to identify the structured Citation: Hora M, Sarkar R, Morris V, Xue K, Prade core ofκ-type variable domain light chain fibrils. The core contains residues of the CDR2 E, Harding E, et al. (2017) MAK33 antibody light and theβ-strands D, E, F and G of the native immunoglobulin fold. The assigned core region chain amyloid fibrils are similar to oligomeric precursors. PLoS ONE 12(7): e0181799. https:// of the fibril is distinct in comparison to the core identified in a previous solid-state NMR study doi.org/10.1371/journal.pone.0181799 on AL-09 by Piehl at. al, suggesting that V fibrils can adopt different topologies. In addition, Editor: Patrick van der Wel, University of we investigated a soluble oligomeric intermediate state, previously termed the alternatively Pittsburgh School of Medicine, UNITED STATES folded state (AFS), using NMR and FTIR spectroscopy. The NMR oligomer spectra display Received: April 9, 2017 a high degree of similarity when compared to the fibril spectra, indicating a high structural similarity of the two aggregation states. Based on comparison to the native state NMR Accepted: July 9, 2017 chemical shifts, we suggest that fibril formation via domain-swapping seems unlikely. More- Published: July 26, 2017 over, we used our results to test the quality of different amyloid prediction algorithms. Copyright:© 2017 Hora 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. Introduction Data Availability Statement: NMR data are Antibody light chain amyloidosis (AL amyloidosis) is a rare disease caused by amyloid forma- available from the BioMagResBank (BMRB ID 27065; URL: http://www.bmrb.wisc.edu/). tion of immunoglobulin light chains (LCs) [1,2]. An underlying B-cell dyscrasia causes over- production and secretion of LCs. In the case of an aggregation-prone LC sequence, this can Funding: This work was supported by a grant from result in formation of oligomeric intermediates and further of fibrils, which deposit in the the German Bundesministerium fu Èr Bildung und Forschung (BMBF) within the network GERAMY. inner organs, causing systemic amyloidosis. Heart failure is the dominant cause of death [3,4]. We acknowledge support of the Helmholtz- The 4-year overall-survival rate is on the order of 33% [5]. Gemeinschaft, the German Research Foundation Non-fibrillar oligomers have aroused interest of the research community due to their cyto- (DFG, Grant Re1435, to B.R.) and the Center for toxicity as well as their role as folding intermediates [6]. Oligomers have been reported for sev- Integrated Protein Science Munich (CIPS-M). The eral amyloid-forming proteins and peptides [7]. In many cases, these oligomers appear to be DFG and the Technical University of Munich (TUM) supported the open access publication in the the most cytotoxic species [8,9]. The mechanism of cytotoxicity is likely due to membrane PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 1 / 14 AL fibrils are similar to AL oligomers framework of the Open Access Publishing pore formation [10,11]. Nonetheless, fibrils also exhibit toxicity [12]. In AL amyloidosis, both Program. The funders had no role in study design, oligomers and fibrils have been found to be cytotoxic, affecting the cardiomyocyte metabolism data collection and analysis, decision to publish, or [13,14]. preparation of the manuscript. Despite the relevance of LC oligomers and fibrils for disease, little is known about their Competing interests: The authors have declared structures. AL fibrils are composed of proteins containing mostly variable domain (V ) resi- that no competing interests exist. dues [1]. However, aggregates can also contain LC protein including constant domain (C ) residues [1]. The N-terminal part of the V domain seems to be structured in the fibrils [15,16]. Cryo-EM has been used to determine the steric zipper structure of an AL-protein derived 12-residue peptide fibril [17]. Recently, magic-angle-spinning solid-state NMR (MAS ssNMR) chemical shift assignments and a secondary structure analysis were reported for the κI sequence AL-09 [18,19]. We report here a MAS ssNMR spectroscopic analysis of amyloid fibrils and oligomers formed by the V domain of MAK33. The murineκ-type V domain of MAK33 has been stud- L L ied extensively regarding its native structure [20], biophysical properties and folding pathways [21,22]. Several point mutations facilitate fibril formation [23±26]. We employed the amyloi- dogenic mutant MAK33 V S20N [25] to study amyloid fibrils with MAS ssNMR. We were able to identify the structured hydrophobic core region, which comprises mainly residues 60± 87. Oligomeric intermediates tend to be short-lived and thus difficult to investigate. In con- trast, the MAK33 V domain forms stable high-molecular weight oligomers at pH 2, which were previously referred to as alternatively folded state (AFS) [21]. These non-fibrillar oligo- mers were studied with MAS ssNMR, Fourier-transform infrared spectroscopy (FTIR) and transmission electron microscopy (TEM). MAS ssNMR revealed an astonishing similarity of the oligomer and the fibril chemical shifts, indicating a high degree of structural similarity. In contrast, secondary chemical shifts of the fibrils show no correlation with those of the native state, suggesting that fibril formation does not proceed via a domain swapping mechanism. Results In order to investigate AL fibril structure, we employed seeded fibrils of the MAK33 V S20N protein. Two independent fibril preparations yielded highly reproducible MAS ssNMR spectra 13 15 (Fig 1). Fig 1A shows a 2D-N(CA)CX correlation spectrum obtained from uniformly C, N 13 13 labeled protein and Fig 1B a 2D-NCA spectrum for a C-spin dilute sample. Due to sparse C labeling of the 2- C-glycerole labeled sample, fewer cross peaks were obtained [27]. Except for this observation, however, the two preparations produced identical NMR spectra. In Fig 1B, assignments were transferred directly from the spectrum of the uniformly C labeled sample without moving the position of the crosses. Considering the common problem of fibril poly- morphism [28], such reproducibility is an important prerequisite for further structural analysis. The assignment of the structured parts of the MAK33 V S20N fibrils was accomplished using a variety of MAS ssNMR experiments: PDSD [29], NCACX, NCOCX [30], NCACB, N (CO)CACB, NCOCA and CANCO [31]. A detailed list of all experimental settings is given in the Supporting Information (S1 Table). In total, 36 residues were assigned sequentially, com- prising residues 49±52 (located in the complementarity determining region 2 (CDR2) of the native state), residues 60±87 (β-strands D, E and F) and residues 98±101 (β-strand G). For all these residues, only a single set of resonances was observed, indicating that the preparations contained only one fibril polymorph. Chemical shift assignments were deposited in the Bio- 13 15 MagResBank (BMRB ID 27065). The C and N linewidths were both on the order of 1 ppm at a 750 MHz spectrometer. In particular, the N transverse relaxation time of 9 ms indicated PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 2 / 14 AL fibrils are similar to AL oligomers 13 15 13 15 13 Fig 1. C, N correlations of MAK33 V S20N fibrils. A) N(CA)CX spectrum of a u- C, N labeled sample. B) NCA spectrum of a 2- C-glycerole isotope labeled sample. Peak positions are identical in A) and B), indicating good reproducibility. The resolution in B) is increased due to sparse isotope labeling. https://doi.org/10.1371/journal.pone.0181799.g001 a high quality of the sample, i.e. a high degree of homogeneity. Representative strip plots of the assignment are shown in S1 Fig. The secondary chemical shift analysis indicates that MAK33 V S20N populates mostlyβ- strands in the fibril state, as expected for amyloid fibers. Using TALOS+ [32], we identified fourβ-strands, with regions of random coil conformation in between them (Fig 2, for Cα, Cβ and CO secondary chemical shifts, see S2 Fig). Twenty additional spin systems could be observed, but not assigned, due to low signal intensities. As signal intensity correlates with rigidity in dipolar-based MAS ssNMR experiments, we assumed that these twenty residues were less structured and located in the flanking region of the core structure. Dynamic residues cannot be observed with the dipolar-based MAS ssNMR experiments employed here. For complementarity, we conducted an INEPT experiment based on scalar couplings, which is suited to detect highly flexible residues. The resulting spectrum did not yield observable cross peaks (S3 Fig). Therefore, we assume that the remaining residues exhibit dynamics on an intermediate time scale, which can be observed neither with INEPT nor with dipolar-coupling based experiments. Alternatively, the respective residues might be structur- ally heterogeneous. Having identified the core of the fibrils, we aimed at a comparison with the oligomeric intermediates that are formed during aggregation. While oligomers are typically short-lived and thus difficult to study, MAK33 V forms stable oligomers at acidic pH (Fig 3A) [21]. An electron microscopic analysis of the oligomers revealed an irregular morphology, but a rather homogeneous size distribution (Fig 3B). The mean diameter of the particles was 9.9 ± 1.5 nm, suggesting in average 30 monomers per oligomer (S4 Fig). This is in excellent agreement with previous studies using analytical ultracentrifugation, which yielded 17 to 42 monomers per oligomer [22]. Upon shaking at 37ÊC, the oligomers transform to well-structured fibrils within 24 hours (Fig 3C). Using FTIR (Fig 3D), both samples displayed similar peaks, with maxima at PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 3 / 14 AL fibrils are similar to AL oligomers Fig 2. Secondary structure analysis of MAK33 V in the fibril state. A)β-sheet propensity calculated with TALOS+ [32]. B) Sequence and secondary structure elements of the native V fold. Green and red bars indicateβ-strands and CDRs of the native structure, respectively. Red arrows below the sequence indicateβ-strands in the fibril state. The expansion shows the assigned atoms in the aggregated state. https://doi.org/10.1371/journal.pone.0181799.g002 -1 -1 1619 cm (oligomers) and 1621 cm (fibrils). Amyloid fibrils yield characteristic FTIR max- -1 -1 ima between 1611 cm and 1630 cm , whereas peaks of nativeβ-sheet proteins are typically -1 -1 found in the range from 1630 cm to 1643 cm [33,34]. Hence, the oligomers differ from the native state and resemble the fibrils at the level of secondary structure. The oligomer FTIR -1 spectrum also displayed a less pronounced peak at 1697 cm . This peak is characteristic for oligomers [35]. We employed MAS solid-state NMR to investigate the V oligomer structure. Using FROS- 13 13 TY-NMR [36], a PDSD C, C-correlation of the MAK33 V WT oligomers was acquired. The similarity between the oligomer and the fibril spectrum is striking (Fig 3E). The chemical PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 4 / 14 AL fibrils are similar to AL oligomers Fig 3. Comparison of MAK33 V oligomers and fibrils. A) Procedure to form oligomers and fibrils. B), C) Electron micrographs of MAK33 V L L S20N oligomers (B) and fibrils (C). The scale bar denotes 200 nm. D) FTIR spectra of MAK33 V S20N oligomers and fibrils. The peak maxima -1 -1 -1 were 1619 cm (oligomers) and 1621 cm (fibrils), respectively. The oligomer spectrum displayed an additional peak at 1697 cm . E) PDSD 13 13 C, C-intraresidue correlations of MAK33 V S20N fibrils and MAK33 V WT oligomers. The proline spin system, which is more intense in the L L oligomers, is highlighted in blue. https://doi.org/10.1371/journal.pone.0181799.g003 shift patterns for many spin systems were very similar. The oligomer resonances were broader in general, which is in good agreement with a less well-defined structure. Some fibril reso- nances are missing in the oligomer spectrum, which is presumably due to dynamics, resulting in reduced sensitivity. Spectral differences are expected, since oligomers and fibrils show clearly distinct morphologies. The resonances of residues I75, S77, V78, E79 and T80 are miss- ing in the oligomer spectrum and the presence of N76 is unclear due to spectral overlap. In the fibrils, this region corresponds to a loop connecting twoβ-strands (Fig 2). In the oligomers, this loop might adopt a different conformation or experiences a different chemical environment. Nevertheless, the similarity of both spectra indicates that the secondary and tertiary struc- tures of the oligomeric and the fibril state are highly similar. We could identify only one spin system, which clearly has a higher signal intensity in the oligomer state than in the fibril state. This spin system corresponded to a proline residue. The proline is presumably in a trans con- formation, as the Cβ and Cγ shifts were approximately 30.3 ppm and 25.5 ppm, respectively [37]. MAK33 V contains five prolines, at positions 8, 15, 44, 59 and 95. However, due to lack of sequential connectivities, we could not assign this proline spin system to one of the five PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 5 / 14 AL fibrils are similar to AL oligomers prolines in the primary structure of MAK33 V . Considering which regions of the sequence were assigned, it is likely to be either P44, P59 or P95. The change in NMR signal intensity of this residue suggests that the dynamics of this proline residue increase when the oligomer structure is converted into the fibril state. Proline isomerisation is critical during the initial folding of MAK33 V [38,39]. Prolines have been reported previously as important switches for amyloid formation in the case ofβ2-microglobulin [40]. In the case of the amyloidogenic V domain AL-103, the presence of two consecutive prolines at positions 95 and 95a affects both the kinetic stability and fibril formation [41]. Further analysis of the proline isomerisation states are needed to yield a better understanding of their role in AL amyloid formation. Discussion Here we reported on the structured core residues of an immunoglobulin V -κ sequence in the amyloid fibril and oligomeric state. Considering the tremendous variability of antibody sequences, it is interesting whether these results are transferable to other light chain sequences. In the AL-09 fibril sample studied by Piehl et al. [18,19], the structured regions comprised mostly the first 30 N-terminal residues as well as residues 94±107 at the C-terminus. In between, only a few residues could be assigned. It is surprising that the assigned regions differ considerably compared to our sequence (Fig 4A). In both studies, several residues could not be assigned sequentially, so there might be more overlap in the hydrophobic core regions. We emphasise however, that intense resonances, which are easier to assign, correlate with rigid structure. In this regard, the differences with respect to assigned regions are meaningful and indicate distinct topologies for the fibril states of both V sequences. Recently, LC amyloid deposits with distinct morphologies were found in ex vivo tissue samples of one individual patient [42]. In this sense, the V fibril structure is polymorphic due to growth conditions and tissue specific factors, in addition to the structural diversity which is presumably induced by differences in the sequence. Piehl et al. have previously pointed out that most of the non-conservative mutations in AL- 09 are located outside of the assigned and thus structured regions [18]. Similarly, the amyloid- enhancing mutation S20N employed here for MAK33 is not part of the hydrophobic core identified in our study. These findings emphasise that point mutations, which are relevant for fibril formation, are not necessarily structured in the fibril state. On the other hand, the critical residue D70, which is part of a conserved salt bridge is located within the assigned regions [25]. Similarly, the highly amyloidogenic V -λ6 subtype differs from less amyloidogenic vari- ants by an insertion at positions 68 and 69 [43,44], which, according to our findings, is located in the fibril core. Understanding of amyloidogenicity of antibody LC sequences cannot be complete without considering the fibril structure and requires further ssNMR studies. In this study, we investigated a murine VL sequence. To find out if the murine framework is comparable to human pathological sequences, we compared the MAK VL with human VL sequences. The sequence identity between MAK33 VL and other patient-derived or patient- related sequences ranges from 40% to 60%. E. g. the sequence identity is 57% with respect to Sma [45], 44% in comparison to 6aJL2 [46], and 42% for Wil [47]. While these values might seem low, they are actually in the same order as the identities between different pathological human sequences: The identity between Sma and 6aJL2 is 46%, 45% for Sma and Wil, and 89% for the quite similarλ6 sequences 6aJL2 and Wil. Hence, the differences between our murine sequence and pathological sequences are not larger than the differences between patient-derived AL sequences of different light chain subgroups. We prepared our fibrils deliberately at pH 2, since acidic conditions are known to stabilise fibrils. pH 2 is necessary to form stable oligomers. Recently, ssNMR experiments have been PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 6 / 14 AL fibrils are similar to AL oligomers Fig 4. Comparison with AL-09, amyloid prediction algorithms and native state chemical shifts. A) Sequence alignment of MAK33 V S20N and AL-09 V : Identical residues are marked in blue. Residues assigned in MAS ssNMR spectra are indicated by bars above and below the corresponding sequence. B) Predictions of MAK33 V S20N amyloid propensity and experimentally observedβ-strands. C) Secondary chemical shift correlation of MAK33 V S20N in the solid-state (fibrils, pH 2) and solution-state (native, pH 6.5) for Cα, Cβ, CO and N chemical shifts. The cross-correlation coefficients r are indicated in each plot. https://doi.org/10.1371/journal.pone.0181799.g004 performed to identify the structured core residues in the VL-κ protein AL-09 fibril. Also in this study, fibrils were prepared at pH 2 [18,19]. Piehl et al compared those in vitro fibrils formed at acidic conditions with ex vivo fibrils derived from human spleen tissue. It is dis- cussed that NMR spectra from both samples are comparable. Hence, while acidic conditions PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 7 / 14 AL fibrils are similar to AL oligomers are not physiological, they represent a necessary experimental requirement for the investiga- tion of fibrillised VL protein by ssNMR. The vast number of different V sequences that can form fibrils makes a structural charac- terisation of all antibody fibrils by ssNMR impractical. Therefore, predictions of amyloido- genic regions can be a precious tool to study a multitude of sequences. We compared our MAS ssNMR results with the predictions from three web tools (Fig 4B). In our benchmark, we included Aggrescan [48], Tango [49] and Zyggregator [50]. Of the fourβ-strands identified by MAS ssNMR, all algorithms identified the two longer C-terminalβ-strands between residues 70 and 90. Our first N-terminalβ-strand was only predicted by Aggrescan, the second one only with low propensity by Zyggregator. All programs predicted moderate aggregation pro- pensities in the N-terminal region (residues 1±30), where we could not assign any resonances. Our assignments are incomplete and we cannot exclude the presence of further structured regions. In fact, a structured N-terminus of V fibrils has also been suggested for other V L L sequences [15,16]. To summarise, all three algorithms could correctly predict the two longer β-strands. We therefore believe that prediction of amyloid propensity will be a valuable tool to study VL sequences in the future. In the past, domain swapping has been suggested as a mechanism to explain immunoglobu- lin light chain deposition [51,52]. In this context, it has been shown that the amyloid core of transthyretin consists of native-likeβ-sheets [53]. We analysed NMR secondary chemical shifts, which report on secondary structure elements. If the conformation of MAK33 V S20N in the fibril state resembled the conformation of this point mutant in the native structure, the secondary chemical shifts of the solid-state and solution-state preparations should be similar. Fig 4C shows correlation plots of the Cα, Cβ, CO and N secondary chemical shifts. We can not observe a correlation between native and fibril secondary structure for any of the nuclei assigned in both conformations. Hence, we conclude the fibrils studied here were not formed by domain swapping. Similar discrepancies between native and fibril states were reported recently for AL-09 V [19], supporting the hypothesis that AL fibrils do not form via a domain-swapping mechanism. Our data alternatively indicate that the native MAK33 V at least partially unfolds and undergoes a transformation to a distinct oligomeric state. While the morphology according to TEM differs from mature fibrils, the local chemical environment is rather similar, as reflected by the NMR chemical shifts. Along the same lines, NMR spectra for oligomer and protofibril preparations have been reported for amyloid-β [54]. Our FTIR experiment with the oligomers -1 displayed a characteristic peak at 1697 cm . While there are still disputes about determination ofβ-sheet arrangements with FTIR [35], according to theoretical derivations, this band might indicate anti-parallelβ-sheets [55]. The fibrils, in contrast, do not produce this FTIR peak and thus likely contain the typical parallelβ-sheets [56]. Different orientations ofβ-strands in olig- omers and fibrils are in agreement with literature [35,57,58]. It will be interesting to see, whether these observations on MAK33 V oligomers and fibrils are also true for other light chain amyloid sequences. With the recent advances in MAS ssNMR structure determinations of fibrils [59,60] and the now available assignments of V fibrils, a structure comes within reach. We expect this will be an important contribution to predict which V sequences are prone to fibril formation and how the oligomers and fibrils can be cleared. Material and methods If not specified otherwise, all chemicals were purchased from Sigma Aldrich (Taufkirchen, Germany). PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 8 / 14 AL fibrils are similar to AL oligomers Recombinant protein production MAK33 V WT and S20N were purified as described previously [25]. Briefly, E.coli BL21 with a pET28 vector containing the MAK V gene were grown in M9 minimal medium supple- L Kan 13 15 mented with 2 g/l C-glucose and 0.5 g/l NH Cl. Expression was induced with 1 mM IPTG at OD 0.6±0.8. After over night expression at 37ÊC, cells were harvested and inclusion bodies were isolated. The inclusion bodies were dissolved in a buffer consisting of 50 mM Tris, 5 mM EDTA, 8 M urea and 1%β-mercaptoethanol (pH 8). The dissolved protein was subjected to anion exchange chromatography, using a 16 / 10 Q Sepharose High Performance column (GE Healthcare, Munich, Germany) using a buffer consisting of 25 mM Tris, 5 mM EDTA and 5 M urea (pH 8). The V protein eluted in the flowthrough. Refolding was achieved by over- night dialysis into a buffer containing 250 mM Tris, 5 mM EDTA, 100 mM L-arginine, 1mM oxidised glutathione und 0.5 mM reduced glutathione (pH 8, 4ÊC). Finally, the protein was purified using gel filtration chromatography with a HiLoad 16/600 Superdex 75 prep grade column (GE Healthcare, Munich, Germany) and a buffer consisting of 20 mM sodium phos- phate and 50 mM NaCl (pH 6.5). Total yield was 15±20 mg protein per liter of culture. Oligomer and fibril preparation The buffer was thoroughly exchanged to 25 mM acetic acid, 25 mM phosphoric acid and 50 mM NaCl (pH 2). Protein monomer concentration was set to 50 μM. 0.05% NaN was supple- mented to protect against bacterial growth. In order to obtain non-fibrillar oligomers, the solu- tion was incubated at room temperature under quiescent conditions. For fibril formation, the solution was incubated at 37ÊC at 350 rpm. Fibrils formed within one week. The outcome was confirmed by TEM. To enrich a single polymorph, fibrils were seeded for several generations. Approximately 2% of preformed fibrils were added to a new batch set up for fibril formation. th Samples used for MAS ssNMR analysis were from 7 or later generation of continuous seed- ing, with each seeding step incubating for one week. MAS solid-state NMR sample preparation An OptimaL-100 XP ultracentrifuge (Beckman Coulter, Krefeld, Germany) equipped with an SW 32 Ti swinging bucket rotor and a rotor filling device (Giotto Biotech, Florence, Italy) were used to pack the protein aggregate into an MAS rotor. The rotation frequency of the centrifuge was set to 28,000 rpm. Samples were packed into 3.2 mm thin wall ZrO rotors with vespel caps (CortecNet, Voisins Le Bretonneux, France) employing house-made teflon spacers. MAS solid-state NMR experiments All MAS ssNMR experiments were recorded using a 750 MHz Bruker Avance III spectrometer (Bruker BioSpin, Karlsruhe) equipped with a triple-resonance MAS probe for 3.2 mm rotors. The set temperature of the probe was adjusted to 273 K. The MAS frequency was set to 10 kHz (for PDSD, NCACX, NCOCX) or 17 kHz (NCOCA, CANCO, NCACB, NCOCAB, INEPT). Detailed settings for the experiments are given in the Supplementary Information (S1 Table). The building blocks for the experiments were PDSD, SPECIFIC-CP [61], BSH-CP [62], DREAM [63] and INEPT. The pulse sequences were implemented as described by Szeverenyi et al. [29] and Schu È tz et al. [31]. NCACX, NCOCX and NCACB were acquired with non-uni- form sampling to increase sensitivity [64]. Sparsity was set to 50% with exponentially decreas- ing sampling density, matched to the transverse relaxation time according to a spin echo experiment [65]. Experiments were acquired using Topspin 3.2 (Bruker BioSpin, Karlsruhe, Germany). Uniformly sampled experiments were processed with Topspin 3.2, nonuniformly PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 9 / 14 AL fibrils are similar to AL oligomers sampled spectra were processed either with the compressed sensing plugin of Topspin 3.2 or with hmsIST [66] in combination with NMRPipe [67]. All spectra were zero-filled to double the number of measured points and then the next power of two. Shifted squared cosine func- tions were employed for apodisation. Secondary chemical shifts were calculated as observed random coil Dd ˆ d d with random coil chemical shifts taken from the BMRB [68]. Negative-stain transmission electron microscopy Copper grids with 300 meshes coated with formvar/carbon film (Electron Microscopy Sci- ences, Hatfield, USA) were glow-discharged in argon atmosphere for 30 s at 3 mA. 5 μl of a 50 μM protein sample were incubated for 60 s on the grid. After removing the protein solution, the grid was washed with water. 5 μl uranyl acetate solution (2% w/v) were applied on the grid for staining and removed after 30 s. Photographs of the oligomers and fibrils converted from oligomers were measured on a Jeol JEM 1400 Plus transmission electron microscope (Jeol, Tokyo, Japan). Fourier-transform infrared spectroscopy Oligomer and fibril samples, 50 μM in fibril buffer (25 mM phosphoric acid, 25 mM acetic acid, 50 mM NaCl, 0.05% NaN , pH 2), were recorded on a JASCO FT/IR-4100 FT-IR spec- trometer (JASCO, Gross-Umstadt, Germany) with attenuated total reflectance (ATR) attach- -1 ment. The samples were measured with 128 scans at a resolution of 2 cm at room temperature. Spectra were buffer subtracted and smoothed using a Savitzky-Golan algorithm. Supporting information S1 Fig. Sequential walks from residues G64 to G68. (PDF) S2 Fig. Secondary chemical shifts of MAK33 V S20N fibrils. (PDF) 1 15 S3 Fig. H- N-INEPT experiment of MAK33 V S20N fibrils. (PDF) S4 Fig. Electron microscopic analysis of MAK33 V S20N oligomers. (PDF) S1 Table. ssNMR parameters. (XLS) Acknowledgments We thank Carsten Peters and Sevil Weinkauf for assistance with electron microscopy. Author Contributions Conceptualization: Manuel Hora, Johannes Buchner, Bernd Reif. Data curation: Manuel Hora. Formal analysis: Manuel Hora, Vanessa Morris. PLOS ONE | https://doi.org/10.1371/journal.pone.0181799 July 26, 2017 10 / 14 AL fibrils are similar to AL oligomers Funding acquisition: Johannes Buchner, Bernd Reif. Investigation: Manuel Hora, Vanessa Morris, Elke Prade, Emma Harding. 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