The extent of protein hydration dictates the preference for heterogeneous or homogeneous nucleation generating either parallel or antiparallel β-sheet α-synuclein aggregates

Camino, José D.; Gracia, Pablo de; Chen, Serene W.; Sot, Jesús; Arada, Igor de la; Sebastián, Víctor; Arrondo, José Luis R.; Goñi, Félix M.; Dobson, Christopher M.; Cremades, Nunilo

doi:10.1101/2020.09.28.315325

Cited by 6 publications

(6 citation statements)

References 83 publications

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“…19,20 In vitro analysis also showed that α-synuclein can self-assemble at room temperature to produce amyloid-like fibrils under several solution conditions such as low pH, 21 orbital shaking, 22 an air−water interface, etc. 23,24 The protein secondary structure and morphological features of these aggregates are quite similar to those found in the patients' samples. Therefore, the prevention of aggregation of α-synuclein and other such proteins and peptides may be one of the possible treatment options for PD, AD, and other similar amyloid diseases which are becoming a huge burden for society.…”

Section: ■ Introductionsupporting

confidence: 64%

Naringenin-Functionalized Gold Nanoparticles and Their Role in α-Synuclein Stabilization

et al. 2023

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Misfolding and self-assembly of several intrinsically disordered proteins into ordered β-sheet-rich amyloid aggregates emerged as hallmarks of several neurodegenerative disorders such as Alzheimer’s and Parkinson’s diseases. Here we show how the naringenin-embedded nanostructure effectively retards aggregation and fibril formation of α-synuclein, which is strongly associated with the pathology of Parkinson’s-like diseases. Naringenin is a polyphenolic compound from a plant source, and in our current investigation, we reported the one-pot synthesis of naringenin-coated spherical and monophasic gold nanoparticles (NAR-AuNPs) under optimized conditions. The average hydrodynamic diameter of the produced nanoparticle was ∼24 nm and showed a distinct absorption band at 533 nm. The zeta potential of the nanocomposite was ∼−22 mV and indicated the presence of naringenin on the surface of nanoparticles. Core-level XPS spectrum analysis showed prominent peaks at 84.02 and 87.68 eV, suggesting the zero oxidation state of metal in the nanostructure. Additionally, the peaks at 86.14 and 89.76 eV were due to the Au–O bond, induced by the hydroxyl groups of the naringenin molecule. The FT-IR analysis further confirmed strong interactions of the molecule with the gold nanosurface via the phenolic oxygen group. The composite surface was found to interact with monomeric α-synuclein and caused a red shift in the nanoparticle absorption band by ∼5 nm. The binding affinity of the composite nanostructure toward α-synuclein was in the micromolar range (K a∼ 5.02 × 106 M–1) and may produce a protein corona over the gold nanosurface. A circular dichroism study showed that the nanocomposite can arrest the conformational fluctuation of the protein and hindered its transformation into a compact cross-β-sheet conformation, a prerequisite for amyloid fibril formation. Furthermore, it was found that naringenin and its nanocomplex did not perturb the viability of neuronal cells. It thus appeared that engineering of the nanosurface with naringenin could be an alternative strategy in developing treatment approaches for Parkinson’s and other diseases linked to protein conformation.

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Section: ■ Introductionsupporting

confidence: 64%

Naringenin-Functionalized Gold Nanoparticles and Their Role in α-Synuclein Stabilization

et al. 2023

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“…3 Alternatively, incubation of αSyn under limited hydration conditions (either PBS with moderate concentrations of alcohols or high concentrations of salts, or upon protein lyophilization in water) promoted αSyn aggregation into structures with an antiparallel intermolecular βsheet structure and particularly slow conversion to fibrils. 28,29 These oligomeric forms, particularly those generated upon αSyn lyophilization and resuspension at high protein concentrations (typically 12 mg•mL −1 ), were morphologically and biologically analogous to the type B oligomers, and were thus named type B* oligomers. 28 Importantly, similar oligomeric species are formed inside neuronal cells, 30 and analogous levels of stress and dysfunction were observed in PD-related cellular models of αSyn aggregation.…”

Section: αSyn Oligomersmentioning

confidence: 99%

Characterization of Pairs of Toxic and Nontoxic Misfolded Protein Oligomers Elucidates the Structural Determinants of Oligomer Toxicity in Protein Misfolding Diseases

et al. 2023

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Conspectus The aberrant misfolding and aggregation of peptides and proteins into amyloid aggregates occurs in over 50 largely incurable protein misfolding diseases. These pathologies include Alzheimer’s and Parkinson’s diseases, which are global medical emergencies owing to their prevalence in increasingly aging populations worldwide. Although the presence of mature amyloid aggregates is a hallmark of such neurodegenerative diseases, misfolded protein oligomers are increasingly recognized as of central importance in the pathogenesis of many of these maladies. These oligomers are small, diffusible species that can form as intermediates in the amyloid fibril formation process or be released by mature fibrils after they are formed. They have been closely associated with the induction of neuronal dysfunction and cell death. It has proven rather challenging to study these oligomeric species because of their short lifetimes, low concentrations, extensive structural heterogeneity, and challenges associated with producing stable, homogeneous, and reproducible populations. Despite these difficulties, investigators have developed protocols to produce kinetically, chemically, or structurally stabilized homogeneous populations of protein misfolded oligomers from several amyloidogenic peptides and proteins at experimentally ameneable concentrations. Furthermore, procedures have been established to produce morphologically similar but structurally distinct oligomers from the same protein sequence that are either toxic or nontoxic to cells. These tools offer unique opportunities to identify and investigate the structural determinants of oligomer toxicity by a close comparative inspection of their structures and the mechanisms of action through which they cause cell dysfunction. This Account reviews multidisciplinary results, including from our own groups, obtained by combining chemistry, physics, biochemistry, cell biology, and animal models for pairs of toxic and nontoxic oligomers. We describe oligomers comprised of the amyloid-β peptide, which underlie Alzheimer’s disease, and α-synuclein, which are associated with Parkinson’s disease and other related neurodegenerative pathologies, collectively known as synucleinopathies. Furthermore, we also discuss oligomers formed by the 91-residue N-terminal domain of [NiFe]-hydrogenase maturation factor from E. coli, which we use as a model non-disease-related protein, and by an amyloid stretch of Sup35 prion protein from yeast. These oligomeric pairs have become highly useful experimental tools for studying the molecular determinants of toxicity characteristic of protein misfolding diseases. Key properties have been identified that differentiate toxic from nontoxic oligomers in their ability to induce cellular dysfunction. These characteristics include solvent-exposed hydrophobic regions, interactions with membranes, insertion into lipid bilayers, and disruption of plasma membrane integrity. By using these properties, it has been possible to rationalize in model systems the responses...

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“…Recently, Aβ40-WT fibrils with mixed anti-parallel and parallel structures have been observed in the presence of the ganglioside GM1 (41). Moreover, studies on -synuclein have indicated that more hydrophobic environments favor anti-parallel fibril structure over parallel structure (42).…”

Section: Anti-parallel and Parallel Structure In Aβ Fibrils In Sporadic Caamentioning

confidence: 99%

Human cerebral vascular amyloid contains both antiparallel and parallel in-register Aβ40 fibrils

Irizarry

Davis

Zhu

et al. 2021

Journal of Biological Chemistry

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This is a PDF file of an article that has undergone enhancements after acceptance, such as the addition of a cover page and metadata, and formatting for readability, but it is not yet the definitive version of record. This version will undergo additional copyediting, typesetting and review before it is published in its final form, but we are providing this version to give early visibility of the article. Please note that, during the production process, errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.

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The extent of protein hydration dictates the preference for heterogeneous or homogeneous nucleation generating either parallel or antiparallel β-sheet α-synuclein aggregates

Cited by 6 publications

References 83 publications

Naringenin-Functionalized Gold Nanoparticles and Their Role in α-Synuclein Stabilization

Naringenin-Functionalized Gold Nanoparticles and Their Role in α-Synuclein Stabilization

Characterization of Pairs of Toxic and Nontoxic Misfolded Protein Oligomers Elucidates the Structural Determinants of Oligomer Toxicity in Protein Misfolding Diseases

Human cerebral vascular amyloid contains both antiparallel and parallel in-register Aβ40 fibrils

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