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Molecular Alignment within ß-Sheets in Aß_14-23 Fibrils: Solid-State NMR Experiments and Theoretical Predictions

Zimei Bu ^*, Yuan Shi , David J. E. Callaway ^*  and Robert Tycko 

^* Fox Chase Cancer Center, Philadelphia, Pennsylvania; New York University School of Medicine, New York, New York; and Laboratory of Chemical Physics, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, Bethesda, Maryland

Correspondence: Address reprint requests to R. Tycko, E-mail: robertt{at}niddk.nih.gov; or D. Callaway, david.callaway{at}fccc.edu.

	ABSTRACT

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION ACKNOWLEDGEMENTS REFERENCES

 
We report investigations of the molecular structure of amyloid fibrils formed by residues 14–23 of the ß-amyloid peptide associated with Alzheimer's disease (Aß_14-23), using solid-state nuclear magnetic resonance (NMR) techniques in conjunction with electron microscopy and atomic force microscopy. The NMR measurements, which include two-dimensional proton-mediated ¹³C-¹³C exchange and two-dimensional relayed proton-mediated ¹³C-¹³C exchange spectra, show that Aß_14-23 fibrils contain antiparallel ß-sheets with a registry of backbone hydrogen bonds that aligns residue 17+k of each peptide molecule with residue 22–k of neighboring molecules in the same ß-sheet. We compare these results, as well as previously reported experimental results for fibrils formed by other ß-amyloid fragments, with theoretical predictions of molecular alignment based on databases of residue-specific alignments in antiparallel ß-sheets in known protein structures. While the theoretical predictions are not in exact agreement with the experimental results, they facilitate the design of experiments by suggesting a small number of plausible alignments that are readily distinguished by solid-state NMR.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION ACKNOWLEDGEMENTS REFERENCES

 
Amyloid fibrils are filamentous aggregates formed by a large class of peptides and proteins with diverse amino-acid sequences. Current interest in amyloid fibrils arises from their involvement in amyloid diseases (including Alzheimer's disease, type 2 diabetes, dialysis-related amyloidosis, Parkinson's disease, transthyretin amyloidoses, transmissible spongiform encephalopathy, and others (1)), from the fairly recent realization that the propensity to form amyloid fibrils is not restricted to disease-associated peptides and proteins (but is instead a nearly generic property of polypeptides (2)), and from the possibility that amyloid fibrils may be a useful basis for development of self-assembled nanomaterials (3,4). Knowledge of the molecular-level details of amyloid fibril structures would contribute to our understanding of potential mechanisms by which amyloid fibrils contribute to or cause amyloid diseases, to the development of therapeutic agents (5–7), to our understanding of the intermolecular and intramolecular interactions that stabilize amyloid fibrils, and possibly to the development of amyloid-based nanomaterials. These molecular-level structural details are only recently becoming accessible, largely through the application of modern solid-state nuclear magnetic resonance (NMR) techniques such as multiple quantum NMR (8–10), dipolar recoupling (11–21), and various forms of multidimensional spectroscopy (10,18,19,22–26) in conjunction with magic-angle spinning (MAS). Solid-state NMR measurements have revealed that amyloid fibrils, which are known to be primarily ß-sheet structures from x-ray fiber diffraction patterns (27–29), can contain either parallel or antiparallel ß-sheets, depending on the amino-acid sequence. To date, antiparallel ß-sheets have only been observed in fibrils formed by relatively short peptides that contain one ß-strand segment (10,12,19). The precise registry of backbone hydrogen bonds (i.e., the alignment of neighboring ß-strands within a single ß-sheet) can be pH-dependent (19) and is not fully determined by the local amino acid sequence (e.g., by seven-residue segments). Not all short peptides form antiparallel ß-sheets in amyloid fibrils (20,30), and the ß-sheets in fibrils formed by short peptides can be switched from antiparallel to parallel by attachment of N-terminal alkyl chains (31).

Techniques other than solid-state NMR have also contributed greatly to our developing understanding of amyloid structures. These techniques include electron microscopy (32–36), x-ray crystallography (30,37), electron paramagnetic resonance (38–42), hydrogen/deuterium exchange (25,43–47), chemical cross-linking (13,48), limited proteolysis (49,50), and scanning mutagenesis (51–53). Results from these techniques are generally consistent with those from solid-state NMR, especially with regard to the types of ß-sheets contained in amyloid fibrils.

In this article, we report the results of solid-state NMR measurements on fibrils formed by residues 14–23 of the full-length ß-amyloid peptide associated with Alzheimer's disease (Aß_14-23, sequence Ac-HQKLVFFAED-NH₂, with acetyl and amide capping groups at the N- and C-termini). We have chosen to study Aß_14-23 for the following reasons:

1. In earlier work, Tjernberg et al. (54) examined amyloid fibril formation by ß-hairpin peptides containing the Aß_14-23 sequence on both sides of a type 1' ß-turn, constrained to align either residue 17+k with residue 20–k or residue 17+k with residue 21–k (54). Both ß-hairpin peptides were found to form fibrils, raising the question of what alignment is preferred by the unconstrained Aß_14-23 peptide in amyloid fibrils (including the possibility of either antiparallel or parallel ß-sheet structure).
   
2. Although the hexapeptide Ac-KLVFFAE-NH₂ has been shown to form amyloid fibrils (10), other ß-amyloid-derived peptides containing the LVFFA hydrophobic segment and a total of nine or fewer residues were found by Tjernberg et al. not to form fibrils (55), while all peptides examined that contained 11 or more residues did form fibrils (19,55). Residues 14–23 may therefore be considered the minimal segment of the ß-amyloid sequence that is sufficient for fibril formation.
   
3. Given that our current understanding of amyloid structures and the interactions that stabilize these structures is relatively primitive (e.g., compared with our understanding of soluble, monomeric, globular protein structures), structural studies of model systems such as Aß_14-23 fibrils are expected to contribute important information about the variety and sequence dependence of amyloid structures and stabilizing interactions.
   
4. Model systems such as Aß_14-23 fibrils serve as test-beds for the development and demonstration of experimental methods for determining specific features of amyloid structures and theoretical methods for predicting these structural features.
   

The solid-state NMR measurements described below show that Aß_14-23 fibrils contain antiparallel ß-sheets with hydrogen-bond registry that aligns residue 17+k with residue 22–k, for integral k (e.g., V18 of each Aß_14-23 molecule forms hydrogen bonds with A21 of a neighboring molecule in the same ß-sheet). Moreover, the solid-state NMR data indicate a high level of order in the ß-sheets, with no detectable defects in the 17+k 22–k hydrogen-bond registry. We compare these experimental results with theoretical predictions of ß-strand alignment. In particular, we show that simple predictive tools based upon comparisons with known protein structures may be useful in guiding experimental design, although precise prediction of registry may not be possible.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION ACKNOWLEDGEMENTS REFERENCES

 
Peptide synthesis and fibril formation
Isotopically labeled amino acids were obtained from Cambridge Isotope Laboratories (Andover, MA). Aß_14-23 peptides containing labeled amino acids were synthesized on a Symphony/Multiplex solid-phase synthesizer (Protein Technologies, Tucson, AZ), using standard FMOC synthesis and cleavage protocols. Peptides were purified by high performance liquid chromatography using two mobile phases, water with 0.1% trifluoroacetic acid and acetonitrile with 0.1% trifluoroacetic acid, on a C18 reverse phase column (Grace Vydac, Hesperia, CA). Final purity was >95%, as confirmed by a Kompact MALDI TOF mass spectrometer (Kratos, Chestnut Ridge, NY). After lyophilization of the high performance liquid chromatography fraction containing these peptides, Aß_14-23 was dissolved at 5.3 mg/ml in 10 mM phosphate buffer, 0.01% NaN₃, at pH 4.7. Fibrils formed within three weeks at room temperature. Aß_14-23 fibril samples were prepared with uniform ¹³C and ¹⁵N labeling of L17 and F20 (17,20-Aß_14-23), V18 and F20 (18,20-Aß_14-23), V18 and A21 (18,21-Aß_14-23), and L17 and A21 (17,21-Aß_14-23).

Electron microscopy and atomic force microscopy
Fibril formation was confirmed and fibril dimensions were determined using electron microscopy (EM) and atomic force microscopy (AFM). For EM measurements, 10 µl aliquots of incubated Aß_14-23 solutions were placed on specimen grids covered by a formvar/carbon support film. Excess fluid was wicked off after 2 min and the grids were negatively stained with 4 mg/ml uranyl acetate in water. The stained grids were then examined and photographed with a JEOL (Tokyo, Japan) JEM-100CXII transmission electron microscope.

For AFM, fibrils were diluted in 0.5% acetic acid (pH 3) to a peptide concentration of 0.5 mM. Both lyophilized and fully hydrated (i.e., never lyophilized or dried after incubation) fibrils were examined. A 50 µl aliquot was placed on freshly cleaved mica (1 cm² area), allowed to adsorb for several minutes, and drained from the mica surface. The surface was washed twice with 100 µl of 0.5% acetic acid, then dried under a stream of nitrogen gas. AFM images were obtained in air with a MultiMode AFM system (Veeco Instruments, Santa Barbara, CA) in tapping mode, using microactuated probes with a nominal force constant of 3 N/m and a nominal tip radius of curvature of 10 nm. Approximately 100 images of 5 µm x 5 µm areas were recorded for both lyophilized and hydrated samples, with 1024 pixel resolution in each lateral dimension. AFM images in Fig. 1 b are portions of typical 5 µm x 5 µm areas.

View larger version (155K): [in this window] [in a new window]   FIGURE 1  (a) Transmission electron microscope image of Aß14-23 fibrils, with negative staining. (b) Atomic force microscope images of Aß14-23 fibrils with (left) and without (right) lyophilization before dilution in 0.5% acetic acid and deposition on mica. Grayscales indicate height.

Rf pulse sequences used in solid-state NMR measurements are shown in Fig. 2. One-dimensional ¹³C NMR spectra (Fig. 2 a) were recorded with cross-polarization (CP) from protons (56) and with two-pulse phase-modulated proton decoupling (57). Decoupling fields were 110 kHz. ¹³C rf fields were 50 kHz during CP, with tangent-shaped amplitude modulation. Two-dimensional proton-mediated ¹³C-¹³C NMR exchange (2D-PME) spectra were recorded as described previously (19,58), using 150 µs CP periods, 200 µs proton spin diffusion (SD) periods in the exchange period, and MAS frequencies of 20.0–21.4 kHz (Fig. 2 b). Under these conditions, strong crosspeaks are observed between the NMR lines of ¹³C pairs with directly-bonded protons for which the proton-proton distances are <3 Å. In particular, strong intermolecular crosspeaks between NMR lines of ¹³C-labeled -carbons (C) are detected when the corresponding residues are aligned in antiparallel ß-sheets, leading to intermolecular distances of 2.2 Å between -protons (H). Thus, the presence or absence of particular C/C crosspeaks in 2D-PME spectra can be used to determine hydrogen-bond registry in antiparallel ß-sheets (19,58).

View larger version (15K): [in this window] [in a new window]   FIGURE 2  Radio-frequency pulse sequences for one-dimensional 13C MAS NMR measurements (a), 2D-PME measurements (b), and 2D-RPME measurements (c). Radio-frequency-driven recoupling periods consist of one 13C pulse per MAS rotor period. Dephasing delays are 1 ms. Phase cycles are: 1 = x, –x; 2 = x, x, –x, –x; 3 = x or y for real or imaginary signals in t1; 4 = x, x, y, y, –x, –x, –y, –y; 5 = x, x, x, x, y, y, y, y, –x, –x, –x, –x, –y, –y, –y, –y. Receiver phase cycles are x, –x, y, –y, –x, x, –y, y in panel a and x, –x, –x, x, y, –y, –y, y, –x, x, x, –x, –y, y, y, –y in panels b and c.

1. A short ¹³C-¹³C dipolar recoupling period for intraresidue COC transfer.
   
2. A short CP period for one-bond CH transfer.
   
3. A short proton SD period for intermolecular HH transfer.
   
4. A second short CP period for one-bond HC transfer.
   
5. A second short ¹³C-¹³C dipolar recoupling period for intraresidue CCO transfer. CP and SD conditions are the same as in 2D-PME measurements.
   

¹³C-¹³C dipolar recoupling periods employed the radio-frequency-driven recoupling pulse sequence (59,60), with one 8.0 µs ¹³C -pulse per MAS rotation period for a total of 16 rotation periods (1.067 ms at a 15.0 kHz MAS frequency). ¹³C -pulse phases followed the XY-16 pattern (61).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION ACKNOWLEDGEMENTS REFERENCES

 
Electron microscopy and atomic force microscopy
The EM image in Fig. 1 a shows that Aß_14-23 forms fibrils with an apparently flat, ribbonlike morphology, with fibril widths of 30 nm. Fibril widths exceed the 3.5 nm length of a single Aß_14-23 molecule in a fully extended ß-strand conformation, suggesting that each fibril contains many finer filaments with cross-ß structures.

The AFM images in Fig. 1 b show that lyophilization breaks long Aß_14-23 fibrils into shorter fragments, which tend to coalesce into clumps under the conditions of AFM measurements, but otherwise has no detectable effect on fibril morphology. Apparent fibril heights in AFM images of both lyophilized and hydrated fibrils are 2.5 ± 0.5 nm. The fibril heights may correspond to the thickness of between two and four ß-sheets in a laminated cross-ß structure.

Solid-state NMR
Fig. 3 shows one-dimensional ¹³C MAS NMR spectra of the four Aß_14-23 fibril samples examined in this work. ¹³C chemical shift assignments, summarized in Table 1, are based on the known chemical shift ranges for individual carbon sites in amino acids, and are confirmed by the 2D-NMR spectra described below. Chemical shifts for CO, C, and ß-carbon (C_ß) sites are consistent with a ß-strand conformation for residues 17–21 in Aß_14-23 fibrils (i.e., upfield secondary shifts relative to random coil values (62) for CO and C, downfield secondary shifts for C_ß). Only the C line for L17 does not show a strong secondary shift. In the dry, lyophilized state, ¹³C MAS NMR line-widths for resolved single sites are 1.5 to 2.1 ppm (full width at half-maximum). In the rehydrated state (Fig. 3, a and b, bottom spectra), line-widths are 1.0 ppm. The reduction of ¹³C MAS NMR line-widths upon rehydration is attributable to increased molecular motion, which partially averages out the inhomogenous broadening that arises from structural variations within these noncrystalline fibril samples. Structural variations that may contribute to the observed line-widths include variations in backbone torsion angles within the ß-strand segments by ±10°, variations in side-chain conformations, disorder at the extreme N- and C termini of Aß_14-23, variations in contacts between the fine filaments that presumably comprise the fibrils shown in Fig. 1, and variations in the number of or contacts between ß-sheet layers within these filaments. When compared with the 2–3 ppm line-widths observed in ¹³C MAS NMR spectra of other noncrystalline systems, including peptide/antibody complexes (63,64) and helical proteins (65–67) in frozen solutions as well as other amyloid fibrils (17,21,22), the line-widths in Fig. 3 indicate a high degree of structural order, but without true crystallinity.

View larger version (21K): [in this window] [in a new window]   FIGURE 3  One-dimensional 13C MAS NMR spectra of Aß14-23 fibrils with uniform 13C and 15N labeling of L17 and F20 (a), V18 and A21 (b), V18 and F20 (c), and L17 and A21 (d). Spectra were recorded at a 13C NMR frequency of 150.7 MHz, with MAS frequencies of 20 kHz and between 64 and 256 scans.

Fig. 4 shows 2D-PME spectra of the four Aß_14-23 fibril samples. In the 2D-PME spectrum of 18,21-Aß_14-23 fibrils, strong crosspeaks (25% of diagonal peaks) are observed between C NMR lines of V18 and A21. C/C crosspeaks are not observed above the noise level in any of the other 2D-PME spectra. This result implies that Aß_14-23 fibrils contain antiparallel ß-sheets in which V18 aligns with A21, i.e., antiparallel ß-sheets with 17+k 22–k hydrogen-bond registry. C/C crosspeak intensities for 18,21-Aß_14-23 fibrils, relative to diagonal peak intensities, are approximately the same as in previously reported 2D-PME spectra of Aß_16-22 and Aß_11-25 fibrils for the C pairs that are aligned in antiparallel ß-sheets in these fibrils (19,58). For example, under quite similar experimental conditions, C/C crosspeaks for V18/F20 and L17/A21 pairs in 2D-PME spectra of Aß_16-22 fibrils (which have 17+k 21–k registry (10)) were found to have 28% of the volume of V18 and A21 C diagonal peaks (58). The observed crosspeak intensities for 18,21-Aß_14-23 fibrils indicate that all V18 and A21 residues in Aß_14-23 fibrils participate in the 17+k22–k registry. Any putative alternations in registry (e.g., as previously suggested for Aß_34-42 fibrils (12)) or alternations between antiparallel and parallel ß-sheet alignments would reduce the V18/A21 crosspeak intensities by at least a factor of two. Structures with alternating registry or alignment would also necessarily contain two or more inequivalent environments for Aß_14-23 molecules (i.e., more than one molecule in the asymmetric unit), potentially splitting each ¹³C NMR line into two or more components. No splittings are observed in the one- or two-dimensional spectra of Aß_14-23 fibrils.

View larger version (17K): [in this window] [in a new window]   FIGURE 4  (a) Aliphatic regions of 2D-PME spectra of lyophilized Aß14-23 fibrils with the indicated labeled residues. Single-headed arrows indicate assignments of certain intraresidue crosspeaks. Double-headed arrow indicates an interresidue crosspeak. (b) One-dimensional slices at the indicated C chemical shifts. Double-headed arrows indicate the only interresidue crosspeaks observed in these measurements. Spectra were recorded in 24–72 h, using recycle delays of 2 s and maximum t1 periods of 3.8 ms.

Fig. 5 shows 2D-RPME spectra of 17,20-Aß_14-23 and 18,21-Aß_14-23 fibrils. As explained above, the 2D-RPME technique allows hydrogen-bond registry to be investigated in cases where the C NMR lines are not resolved. The 2D-RPME spectrum of 17,20-Aß_14-23 shows only intraresidue crosspeaks, including crosspeaks between the CO line of L17 (172.8 ppm) and aliphatic carbon lines of L17 (53.3, 44.5, and 24.7 ppm) and crosspeaks between the CO line of F20 (169.5 ppm) and aliphatic lines of F20 (54.0 and 43.0 ppm). In contrast, the 2D-RPME spectrum of 18,21-Aß_14-23 fibrils shows both intraresidue and interresidue crosspeaks, including crosspeaks between the CO line of V18 and the CO line of A21, crosspeaks between the CO line of V18 and aliphatic lines of A21, and crosspeaks between the CO line of A21 and aliphatic lines of V18. Although the signal/noise ratio is higher in the 2D-RPME spectrum of 18,21-Aß_14-23 fibrils (due to a larger sample quantity), the signal/noise ratio in the 2D-RPME spectrum of 17,20-Aß_14-23 fibrils is high enough to permit the observation of interresidue crosspeaks if they were present. The data in Fig. 5 confirm the 17+k22–k hydrogen-bond registry in Aß_14-23 fibrils. In addition, these data demonstrate the utility of the 2D-RPME technique in structural investigations of amyloid fibrils.

View larger version (18K): [in this window] [in a new window]   FIGURE 5  (a) 2D-RPME spectra of rehydrated Aß14-23 fibrils with the indicated labeled residues. (b) One-dimensional slices at the indicated CO chemical shifts. Spectra were recorded in 48–72 h, using recycle delays of 1.6 s and maximum t1 periods of 2.3 ms.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION ACKNOWLEDGEMENTS REFERENCES

 
Summary of experimental findings
EM and AFM images in Fig. 1 demonstrate that Aß_14-23 forms amyloid fibrils, as observed previously for many other fragments of the Alzheimer's ß-amyloid peptide (10,12,13,19). As in the case of fibrils formed by other short fragments (10,19), the fibril widths exceed the maximum length of a single peptide chain, suggesting that the observed fibrils are comprised of multiple finer filaments that cannot be resolved in the images. One-dimensional ¹³C NMR spectra of isotopically labeled Aß_14-23 fibrils in Fig. 3 indicate a high degree of structural order at the molecular level. ¹³C NMR chemical shifts indicate that residues 17–21 form a continuous ß-strand. The 2D-PME and 2D-RPME spectra in Figs. 4 and 5 show that the ß-sheets are of the antiparallel type, with a registry that produces a distance <3 Å between H sites of V18 and A21. Given the ß-strand conformation of residues 17–21, this must be an intermolecular distance. Only 17+k 22–k registry is consistent with the data. Any alternation in registry or alignment within the ß-sheets would be inconsistent with the intensity of C-C crosspeaks in the 2D-PME spectrum of 18,21-Aß_14-23 fibrils and the absence of splittings of any ¹³C NMR lines. A molecular model for the antiparallel ß-sheets in Aß_14-23 fibrils is shown in Fig. 6.

View larger version (59K): [in this window] [in a new window]   FIGURE 6  (a) Molecular model for an antiparallel ß-sheet in Aß14-23 fibrils, with the registry of backbone hydrogen bonds indicated by the solid-state NMR data in Figs. 4 and 5. (b) One-letter-code representation, showing hydrogen-bonded (red lines) and non-hydrogen-bonded (yellow lines) interstrand alignments of amino-acid pairs. Two different sets of alignments (i.e., patterns of red and yellow lines) alternate along the hydrogen-bonding direction of the antiparallel ß-sheet, making two distinct contributions to the calculated free energy.

As observed in solid-state NMR studies of amyloid fibrils formed by other peptides (19,20,73), ¹³C NMR chemical shifts in lyophilized and hydrated Aß_14-23 fibrils are indistinguishable, indicating that the molecular structure is not affected significantly by hydration. Hydration produces a reduction in ¹³C NMR line-widths, also as previously observed. From a practical standpoint, lyophilized samples have the advantages of permitting the use of high MAS frequencies, as required for certain solid-state NMR measurements (74–76), and small sample volumes, which in turn permit high rf fields and high sensitivity. Lyophilized samples are not prone to rf-induced heating and to NMR probe tuning instabilities. On the other hand, hydrated samples may be preferred in experiments where the highest possible spectral resolution is required. Similar line-widths have been observed in spectra of samples that are fully hydrated without prior lyophilization (19) and in spectra of samples that were lyophilized and subsequently rehydrated (20,73).

Theoretical predictions
We now compare the experimental results with theoretical predictions of hydrogen-bond registry in antiparallel ß-sheets. These predictions were made in advance of the experiments and were used to select the isotopic labeling patterns and solid-state NMR strategies described above.

The relative probability of a given registry can be estimated from the probability that such an alignment occurs in known protein structures (54). This probability is calculated from the relative probability that individual pairs of residues align in an antiparallel ß-sheet in known protein structures, which we take from the database of Wouters and Curmi (77,78). Specifically, Wouters and Curmi report pair-correlation values and for all pairs of amino acids i and j, representing the ratio of the observed occurrence of i and j in positions of interstrand alignment (in a set of 253 nonredundant protein structures) to the predicted occurrence of i and j in positions of interstrand alignment if all amino acids in the antiparallel ß-sheets were randomly distributed (77). Wouters and Curmi distinguish between hydrogen-bonded (HB) and non-hydrogen-bonded (NHB) alignments, which they find to have significantly different pair correlation values. We calculate the relative probability for a given registry of a given peptide sequence in antiparallel ß-sheets in an amyloid fibril by multiplying the relevant and values for all aligned residue pairs in that registry. Residues that are unpaired in a given registry (i.e., dangling residues) are assigned a pair correlation value of 1. If the calculated probability is denoted by P, the relative free energy of binding for a given peptide registry is then given by G = –RT ln(P), where T is the temperature and R is the gas constant.

Note that each aligned residue pair occurs with both HB and NHB alignments in the antiparallel ß-sheets under consideration here, because all ß-strands have the same amino-acid sequence and because we consider only ß-sheet structures with maximal symmetry. Therefore, we must evaluate two alignment probabilities (for the two combinations of HB and NHB alignments that alternate along the hydrogen-bonding direction of the ß-sheet; see Fig. 6 b and accompanying caption for clarification) and two free energies. The final free energy is taken to be the average of the two.

Fig. 7 shows this free energy as a function of the offset N, defined by requiring that residue 17+k be aligned with residue N–k of neighboring peptide chains in the ß-sheet. For Aß_14-23, the solid-state NMR results indicate that N = 22, so that V18 aligns with A21. Solid-state NMR data indicate that N = 21 for Aß_16-22 fibrils grown at pH 7.4, while for Aß_11-25 fibrils, N = 20 at pH 7.4 and N = 22 at pH 2.4. Calculated free energies predict N = 21 for all three peptides. In all three cases, the experimental offset is within a deep minimum of the predicted relative free energy. Thus, this simple predictive scheme may be useful to guide experimental design (for instance, by suggesting which residues should be isotopically labeled for solid-state NMR investigations), but does not capture all factors that determine the precise hydrogen-bond registries.

View larger version (12K): [in this window] [in a new window]   FIGURE 7  Calculated free energies G/RT as a function of the offset N in antiparallel ß-sheets with 17+k N–k registry, plotted for the three peptides Aß16-22, Aß14-23, and Aß11-25. See text for details of calculations.

We have also used the pair-information values P_i,j+m introduced by Steward and Thornton (79) to evaluate the relative probabilities of various registries, as previously described by Petkova et al. (19) The pair-information values take into account interstrand interactions between residues that are not directly aligned. For a given registry, we evaluate the sum of P_i,j+m values for m = –1, 0, and 1 (i.e., directly aligned residue pairs, and pairs that are shifted by one residue in either direction) and for i being residues 17, 18, 19, 20, and 21. P_i,j+m values for hydrogen-bonded and non-hydrogen-bonded pairs i and j are added together, because both types of pairing are present for each residue in the ß-sheet structures under consideration. Total information scores are 450, 795, 1042, and 576 for N equal to 19, 20, 21, and 22, respectively. Replacing Asp by Asn and Glu by Gln to approximate the effects of low pH, the total scores become 450, 895, 1036, and 653. If we set P_i,j+m = 0, so that only directly aligned residues are considered, the scores are 80, 412, 631, and 204 at neutral pH, and 80, 412, 631, and 416 at low pH. Thus, the most likely registry according to the pair-information value treatment is always 17+k 21–k, in agreement with the free energy calculations in Fig. 7.

More sophisticated and accurate schemes could be formulated by including structural effects or energetics derived from other experimental techniques (80). The approaches described above do not take into account interactions between ß-sheet layers, which have been elucidated experimentally in Aß_1-40 fibrils (81) and GNNQQNY fibrils (30), but not in the fibrils discussed above. In Aß_14-23 and Aß_11-25 fibrils, it is not yet known whether residues at the N- and C-termini are structurally ordered and participate in the antiparallel ß-sheets. The 17+k 22–k registry observed in Aß_14-23 fibrils necessarily leaves H14 and Q15 unpaired and outside the ß-sheets. Entropy associated with these residues may favor the observed registry over the predicted 17+k 21–k registry. In addition, the 17+k 22–k registry results in antiparallel ß-sheets with two equivalent faces. Side chains of F19 and F20 create continuous rows of aromatic rings on each face, as shown in Fig. 6. These and other features may be advantageous from the standpoint of interactions between ß-sheet layers.

	ACKNOWLEDGEMENTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION ACKNOWLEDGEMENTS REFERENCES

 
This work was supported by the Intramural Research Program of the National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, and by a grant to D.J.E.C. from the Alzheimer's Association. Development of solid-state NMR methodology was supported by a grant to R.T. from the Intramural AIDS Targeted Antiviral Program of the National Institutes of Health.

Submitted on June 8, 2006; accepted for publication October 2, 2006.

	REFERENCES

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION ACKNOWLEDGEMENTS REFERENCES

 
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