Your search keyword '"Torbeev V"' showing total 19 results

1. Het-Ncap - De novo designed three-helix heterodimer with Cysteine at the Ncap position of the alpha-helix

Author

McEwen, A.G., primary, Poussin-Courmontagne, P., additional, Naudin, E.A., additional, DeGrado, W.F., additional, and Torbeev, V., additional

Published

2021

2. Het-N2-SO3- - De novo designed three-helix heterodimer with Cysteine S-sulfate at the N2 position of the alpha-helix

Author

McEwen, A.G., primary, Poussin-Courmontagne, P., additional, Naudin, E.A., additional, DeGrado, W.F., additional, and Torbeev, V., additional

Published

2021

3. Crystal structure of complex between nuclear coactivator binding domain of CBP and [1040-1086]ACTR containing alpha-methylated Leu1055 and Leu1076

Author

Bauer, V., primary, Schmidtgall, B., additional, Gogl, G., additional, Dolenc, j., additional, Osz, J., additional, Kostmann, C., additional, Mitschler, A., additional, Cousido-Siah, A., additional, Rochel, N., additional, Trave, G., additional, Kieffer, B., additional, and Torbeev, V., additional

Published

2020

4. Molecular mechanism of IKK catalytic dimer docking to NF-κB substrates.

Author

Li C, Moro S, Shostak K, O'Reilly FJ, Donzeau M, Graziadei A, McEwen AG, Desplancq D, Poussin-Courmontagne P, Bachelart T, Fiskin M, Berrodier N, Pichard S, Brillet K, Orfanoudakis G, Poterszman A, Torbeev V, Rappsilber J, Davey NE, Chariot A, and Zanier K

Subjects

Humans, Phosphorylation, Protein Binding, Signal Transduction, NF-KappaB Inhibitor alpha metabolism, NF-KappaB Inhibitor alpha genetics, Molecular Docking Simulation, HEK293 Cells, Substrate Specificity, I-kappa B Kinase metabolism, I-kappa B Kinase chemistry, I-kappa B Kinase genetics, NF-kappa B metabolism, Protein Multimerization, Amino Acid Motifs

Abstract

The inhibitor of κB (IκB) kinase (IKK) is a central regulator of NF-κB signaling. All IKK complexes contain hetero- or homodimers of the catalytic IKKβ and/or IKKα subunits. Here, we identify a YDDΦxΦ motif, which is conserved in substrates of canonical (IκBα, IκBβ) and alternative (p100) NF-κB pathways, and which mediates docking to catalytic IKK dimers. We demonstrate a quantitative correlation between docking affinity and IKK activity related to IκBα phosphorylation/degradation. Furthermore, we show that phosphorylation of the motif's conserved tyrosine, an event previously reported to promote IκBα accumulation and inhibition of NF-κB gene expression, suppresses the docking interaction. Results from integrated structural analyzes indicate that the motif binds to a groove at the IKK dimer interface. Consistently, suppression of IKK dimerization also abolishes IκBα substrate binding. Finally, we show that an optimized bivalent motif peptide inhibits NF-κB signaling. This work unveils a function for IKKα/β dimerization in substrate motif recognition., (© 2024. The Author(s).)

Published

2024

5. Design, Synthesis and Catalytic Activity of Protein Containing Thiotyrosine as an Active Site Residue.

Author

Bachelart T, Kumar S, Jouin A, Yousef M, Kieffer B, and Torbeev V

Subjects

Catalysis, Biocatalysis, Sulfhydryl Compounds chemistry, Peptides, Cyclic chemistry, Peptides, Cyclic chemical synthesis, Molecular Structure, Proteins chemistry, Proteins chemical synthesis, Tyrosine chemistry, Tyrosine analogs & derivatives, Catalytic Domain

Abstract

Native chemical ligation is a key reaction in the toolbox of chemical methods for the synthesis of native and modified proteins. The catalysis of ligation is commonly performed by using small aryl-thiol molecules added at high concentrations. In this work, we incorporated thiotyrosine, a non-canonical amino acid containing an aryl-thiol moiety, into a designed cyclic protein « sans queue ni tête ». Importantly, the protein environment reduced the pK a of the thiol group to 5.8-5.9, which is significantly lower than the previously reported value for thiotyrosine in a short peptide (pK a 6.4). Furthermore, we demonstrated the catalytic activity of this protein both as hydrolase and in native chemical ligation of peptides. These results will be useful for the development of efficient protein catalysts (enzymes) for protein synthesis and modification., (© 2024 The Authors. ChemBioChem published by Wiley-VCH GmbH.)

Published

2024

6. Amyloid engineering - how terminal capping modifies morphology and secondary structure of supramolecular peptide aggregates.

Author

Grelich-Mucha M, Bachelart T, Torbeev V, Ożga K, Berlicki Ł, and Olesiak-Bańska J

Subjects

Peptide Fragments chemistry, Protein Structure, Secondary, Peptides chemistry, Amyloid chemistry

Abstract

The effects of peptide N- and C-termini on aggregation behavior have been scarcely studied. Herein, we examine (105-115) peptide fragments of transthyretin (TTR) containing various functional groups at both termini and study their impact on the morphology and the secondary structure. We synthesized TTR(105-115) peptides functionalized with α-amino (H-), N -acetyl-α-amino (Ac-) or N , N -dimethyl-α-amino (DiMe-) groups at the N-terminus, and with amide (-NH 2 ) or carboxyl (-OH) functions at the C-terminus. We also investigated quasi-racemic mixtures by mixing the L-enantiomers with the D-enantiomer capped by H- and -NH 2 groups. We observed that fibril formation is promoted by the sufficient number of hydrogen bonds at peptides' termini. Moreover, the final morphology of the aggregates can be controlled by the functional groups at the N-terminus. Remarkably, all quasi-racemic mixtures resulted in the robust formation of fibrils. Overall, this work illustrates how modifications of peptide termini may help to engineer supramolecular aggregates with a predicted morphology.

Published

2024

7. Fluorine NMR study of proline-rich sequences using fluoroprolines.

Author

Sinnaeve D, Ben Bouzayene A, Ottoy E, Hofman GJ, Erdmann E, Linclau B, Kuprov I, Martins JC, Torbeev V, and Kieffer B

Abstract

Proline homopolymer motifs are found in many proteins; their peculiar conformational and dynamic properties are often directly involved in those proteins' functions. However, the dynamics of proline homopolymers is hard to study by NMR due to a lack of amide protons and small chemical shift dispersion. Exploiting the spectroscopic properties of fluorinated prolines opens interesting perspectives to address these issues. Fluorinated prolines are already widely used in protein structure engineering - they introduce conformational and dynamical biases - but their use as 19 F NMR reporters of proline conformation has not yet been explored. In this work, we look at model peptides where C γ -fluorinated prolines with opposite configurations of the chiral C γ centre have been introduced at two positions in distinct polyproline segments. By looking at the effects of swapping these (4 R )-fluoroproline and (4 S )-fluoroproline within the polyproline segments, we were able to separate the intrinsic conformational properties of the polyproline sequence from the conformational alterations instilled by fluorination. We assess the fluoroproline 19 F relaxation properties, and we exploit the latter in elucidating binding kinetics to the SH3 (Src homology 3) domain., Competing Interests: The contact author has declared that neither they nor their co-authors have any competing interests., (Copyright: © 2021 Davy Sinnaeve et al.)

Published

2021

8. Autofluorescence of Amyloids Determined by Enantiomeric Composition of Peptides.

Author

Grelich-Mucha M, Garcia AM, Torbeev V, Ożga K, Berlicki Ł, and Olesiak-Bańska J

Subjects

Amino Acid Sequence, Protein Conformation, beta-Strand, Stereoisomerism, Amyloid, Peptides

Abstract

Amyloid fibrils are peptide or protein aggregates possessing a cross-β-sheet structure. They possess intrinsic fluorescence property, which is still not fully understood. Herein, we compare structural and optical properties of fibrils formed from L- and D-enantiomers of the (105-115) fragment of transthyretin (TTR) and from their racemic mixture. Our results show that autofluorescence of fibrils obtained from enantiomers differs from that of fibrils from the racemic mixture. In order to elucidate the origin of observed differences, we analyzed the structure and morphology of fibrils and showed how variations in β-sheet organization influence optical properties of fibrils. We clarified the contribution of aromatic rings and the amyloid backbone to the final blue-green emission of fibrils. This work demonstrates how enantiomeric composition of amino acids allows us to modulate the self-assembly and final morphology of well-defined fibrillar bionanostructures with optical properties controlled by supramolecular organization.

Published

2021

9. Acyl Transfer Catalytic Activity in De Novo Designed Protein with N-Terminus of α-Helix As Oxyanion-Binding Site.

Author

Naudin EA, McEwen AG, Tan SK, Poussin-Courmontagne P, Schmitt JL, Birck C, DeGrado WF, and Torbeev V

Subjects

Acyltransferases chemical synthesis, Acyltransferases chemistry, Amino Acid Sequence, Biocatalysis, Cysteine chemistry, Hydrolysis, Kinetics, Peptide Synthases chemical synthesis, Peptides chemical synthesis, Protein Conformation, alpha-Helical, Protein Engineering, Substrate Specificity, Catalytic Domain, Peptide Synthases chemistry

Abstract

The design of catalytic proteins with functional sites capable of specific chemistry is gaining momentum and a number of artificial enzymes have recently been reported, including hydrolases, oxidoreductases, retro-aldolases, and others. Our goal is to develop a peptide ligase for robust catalysis of amide bond formation that possesses no stringent restrictions to the amino acid composition at the ligation junction. We report here the successful completion of the first step in this long-term project by building a completely de novo protein with predefined acyl transfer catalytic activity. We applied a minimalist approach to rationally design an oxyanion hole within a small cavity that contains an adjacent thiol nucleophile. The N-terminus of the α-helix with unpaired hydrogen-bond donors was exploited as a structural motif to stabilize negatively charged tetrahedral intermediates in nucleophilic addition-elimination reactions at the acyl group. Cysteine acting as a principal catalytic residue was introduced at the second residue position of the α-helix N-terminus in a designed three-α-helix protein based on structural informatics prediction. We showed that this minimal set of functional elements is sufficient for the emergence of catalytic activity in a de novo protein. Using peptide- α thioesters as acyl-donors, we demonstrated their catalyzed amidation concomitant with hydrolysis and proved that the environment at the catalytic site critically influences the reaction outcome. These results represent a promising starting point for the development of efficient catalysts for protein labeling, conjugation, and peptide ligation.

Published

2021

10. Conformational editing of intrinsically disordered protein by α-methylation.

Author

Bauer V, Schmidtgall B, Gógl G, Dolenc J, Osz J, Nominé Y, Kostmann C, Cousido-Siah A, Mitschler A, Rochel N, Travé G, Kieffer B, and Torbeev V

Abstract

Intrinsically disordered proteins (IDPs) constitute a large portion of "Dark Proteome" - difficult to characterize or yet to be discovered protein structures. Here we used conformationally constrained α-methylated amino acids to bias the conformational ensemble in the free unstructured activation domain of transcriptional coactivator ACTR. Different sites and patterns of substitutions were enabled by chemical protein synthesis and led to distinct populations of α-helices. A specific substitution pattern resulted in a substantially higher binding affinity to nuclear coactivator binding domain (NCBD) of CREB-binding protein, a natural binding partner of ACTR. The first X-ray structure of the modified ACTR domain - NCBD complex visualized a unique conformation of ACTR and confirmed that the key α-methylated amino acids are localized within α-helices in the bound state. This study demonstrates a strategy for characterization of individual conformational states of IDPs., Competing Interests: There are no conflicts to declare., (This journal is © The Royal Society of Chemistry.)

Published

2020

11. Aggregation and Amyloidogenicity of the Nuclear Coactivator Binding Domain of CREB-Binding Protein.

Author

Garcia AM, Giorgiutti C, El Khoury Y, Bauer V, Spiegelhalter C, Leize-Wagner E, Hellwig P, Potier N, and Torbeev V

Subjects

Models, Molecular, Protein Binding, Protein Domains, Amyloid chemistry, Amyloid metabolism, CREB-Binding Protein chemistry, CREB-Binding Protein metabolism, Protein Aggregates, Protein Aggregation, Pathological, Protein Folding

Abstract

The nuclear coactivator binding domain (NCBD) of transcriptional co-regulator CREB-binding protein (CBP) is an example of conformationally malleable proteins that can bind to structurally unrelated protein targets and adopt distinct folds in the respective protein complexes. Here, we show that the folding landscape of NCBD contains an alternative pathway that results in protein aggregation and self-assembly into amyloid fibers. The initial steps of such protein misfolding are driven by intermolecular interactions of its N-terminal α-helix bringing multiple NCBD molecules into contact. These oligomers then undergo slow but progressive interconversion into β-sheet-containing aggregates. To reveal the concealed aggregation potential of NCBD we used a chemically synthesized mirror-image d-NCBD form. The addition of d-NCBD promoted self-assembly into amyloid precipitates presumably due to formation of thermodynamically more stable racemic β-sheet structures. The unexpected aggregation of NCBD needs to be taken into consideration given the multitude of protein-protein interactions and resulting biological functions mediated by CBP., (© 2020 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2020

12. Illuminating Voltage Sensor Paddling in Different Membrane Milieu.

Author

Torbeev V

Subjects

Biomechanical Phenomena, Cell Membrane, Voltage-Dependent Anion Channels

Published

2020

13. Modification of Enzyme Activity by Vibrational Strong Coupling of Water.

Author

Vergauwe RMA, Thomas A, Nagarajan K, Shalabney A, George J, Chervy T, Seidel M, Devaux E, Torbeev V, and Ebbesen TW

Abstract

Vibrational strong coupling (VSC) has recently emerged as a completely new tool for influencing chemical reactivity. It harnesses electromagnetic vacuum fluctuations through the creation of hybrid states of light and matter, called polaritonic states, in an optical cavity resonant to a molecular absorption band. Here, we investigate the effect of vibrational strong coupling of water on the enzymatic activity of pepsin, where a water molecule is directly involved in the enzyme's chemical mechanism. We observe an approximately 4.5-fold decrease of the apparent second-order rate constant k cat /K m when coupling the water stretching vibration, whereas no effect was detected for the strong coupling of the bending vibration. The possibility of modifying enzymatic activity by coupling water demonstrates the potential of VSC as a new tool to study biochemical reactivity., (© 2019 The Authors. Published by Wiley-VCH Verlag GmbH & Co. KGaA.)

Published

2019

14. Total chemical synthesis and biophysical properties of a designed soluble 24 kDa amyloid analogue.

Author

Boehringer R, Kieffer B, and Torbeev V

Abstract

Discovering molecular probes that specifically recognize distinct amyloid structures is highly important for physiological studies of protein-misfolding diseases as well as for the development of diagnostic reagents and inhibitors of amyloid self-assembly. Here, we demonstrate an approach that allows for identification of N -methylated peptides that are specific binders for a particular amyloid fiber subtype (or polymorph). Protein design and chemical synthesis were used to produce covalently tethered amyloid analogues with molecular masses approaching 24 kDa and containing nine copies of an amyloidogenic peptide. Such engineered constructs served as a molecular testing platform to evaluate the aggregation properties and solubility as a function of N -methylation pattern. An advantage of the method is the possibility of biophysical characterization of amyloid constructs in solution.

Published

2018

15. Dissecting mechanism of coupled folding and binding of an intrinsically disordered protein by chemical synthesis of conformationally constrained analogues.

Author

Schmidtgall B, Chaloin O, Bauer V, Sumyk M, Birck C, and Torbeev V

Subjects

Amino Acids chemistry, Kinetics, Protein Binding, Protein Conformation, Thermodynamics, Transcription Factors chemistry, Intrinsically Disordered Proteins chemical synthesis, Intrinsically Disordered Proteins chemistry, Protein Folding

Abstract

Non-canonical α-methyl amino acids were incorporated at various sites in the sequence of intrinsically disordered activation domain from the p160 transcriptional co-activator (ACTR) to facilitate the formation of α-helical structures. Kinetic and thermodynamic data confirm the induced fit mechanism of complex formation between the synthesized ACTR variants and the nuclear co-activator binding domain (NCBD).

Published

2017

16. Covalent Tethering and Residues with Bulky Hydrophobic Side Chains Enable Self-Assembly of Distinct Amyloid Structures.

Author

Ruiz J, Boehringer R, Grogg M, Raya J, Schirer A, Crucifix C, Hellwig P, Schultz P, and Torbeev V

Subjects

Humans, Hydrophobic and Hydrophilic Interactions, Models, Molecular, Protein Conformation, Amyloid chemical synthesis, Amyloid chemistry

Abstract

Polymorphism is a common property of amyloid fibers that complicates their detailed structural and functional studies. Here we report experiments illustrating the chemical principles that enable the formation of amyloid polymorphs with distinct stoichiometric composition. Using appropriate covalent tethering we programmed self-assembly of a model peptide corresponding to the [20-41] fragment of human β2-microglobulin into fibers with either trimeric or dimeric amyloid cores. Using a set of biophysical and biochemical methods we demonstrated their distinct structural, morphological, and templating properties. Furthermore, we showed that supramolecular approaches in which the peptide is modified with bulky substituents can also be applied to modulate the formation of different fiber polymorphs. Such strategies, when applied to disease-related peptides and proteins, will greatly help in the evaluation of the biological properties of structurally distinct amyloids., (© 2016 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2016

17. Chiral recognition in amyloid fiber growth.

Author

Torbeev V, Grogg M, Ruiz J, Boehringer R, Schirer A, Hellwig P, Jeschke G, and Hilvert D

Subjects

Humans, Models, Molecular, Peptides chemistry, Protein Structure, Secondary, Spectroscopy, Fourier Transform Infrared, Stereoisomerism, Amyloid chemistry, Peptides chemical synthesis, beta 2-Microglobulin chemistry

Abstract

Insoluble amyloid fibers represent a pathological signature of many human diseases. To treat such diseases, inhibition of amyloid formation has been proposed as a possible therapeutic strategy. d-Peptides, which possess high proteolytic stability and lessened immunogenicity, are attractive candidates in this context. However, a molecular understanding of chiral recognition phenomena for d-peptides and l-amyloids is currently incomplete. Here we report experiments on amyloid growth of individual enantiomers and their mixtures for two distinct polypeptide systems of different length and structural organization: a 44-residue covalently-linked dimer derived from a peptide corresponding to the [20-41]-fragment of human β2-microglobulin (β2m) and the 99-residue full-length protein. For the dimeric [20-41]β2m construct, a combination of electron paramagnetic resonance of nitroxide-labeled constructs and (13) C-isotope edited FT-IR spectroscopy of (13) C-labeled preparations was used to show that racemic mixtures precipitate as intact homochiral fibers, i.e. undergo spontaneous Pasteur-like resolution into a mixture of left- and right-handed amyloids. In the case of full-length β2m, the presence of the mirror-image d-protein affords morphologically distinct amyloids that are composed largely of enantiopure domains. Removal of the l-component from hybrid amyloids by proteolytic digestion results in their rapid transformation into characteristic long straight d-β2m amyloids. Furthermore, the full-length d-enantiomer of β2m was found to be an efficient inhibitor of l-β2m amyloid growth. This observation highlights the potential of longer d-polypeptides for future development into inhibitors of amyloid propagation. Copyright © 2016 European Peptide Society and John Wiley & Sons, Ltd., (Copyright © 2016 European Peptide Society and John Wiley & Sons, Ltd.)

Published

2016

18. Towards Prebiotic Catalytic Amyloids Using High Throughput Screening.

Author

Friedmann MP, Torbeev V, Zelenay V, Sobol A, Greenwald J, and Riek R

Subjects

Catalysis, Circular Dichroism, Humans, Hydrolysis, Microscopy, Electron, Transmission, Spectroscopy, Fourier Transform Infrared, Amyloid chemistry, High-Throughput Screening Assays methods, Peptide Fragments chemistry, Prebiotics

Abstract

Enzymes are capable of directing complex stereospecific transformations and of accelerating reaction rates many orders of magnitude. As even the simplest known enzymes comprise thousands of atoms, the question arises as to how such exquisite catalysts evolved. A logical predecessor would be shorter peptides, but they lack the defined structure and size that are apparently necessary for enzyme functions. However, some very short peptides are able to assemble into amyloids, thereby forming a well-defined tertiary structure called the cross-β-sheet, which bestows unique properties upon the peptides. We have hypothesized that amyloids could have been the catalytically active precursor to modern enzymes. To test this hypothesis, we designed an amyloid peptide library that could be screened for catalytic activity. Our approach, amenable to high-throughput methodologies, allowed us to find several peptides and peptide mixtures that form amyloids with esterase activity. These results indicate that amyloids, with their stability in a wide range of conditions and their potential as catalysts with low sequence specificity, would indeed be fitting precursors to modern enzymes. Furthermore, our approach can be efficiently expanded upon in library size, screening conditions, and target activity to yield novel amyloid catalysts with potential applications in aqueous-organic mixtures, at high temperature and in other extreme conditions that could be advantageous for industrial applications.

Published

2015

19. Substitution of proline32 by α-methylproline preorganizes β2-microglobulin for oligomerization but not for aggregation into amyloids.

Author

Torbeev V, Ebert MO, Dolenc J, and Hilvert D

Subjects

Humans, Hydrogen-Ion Concentration, Molecular Dynamics Simulation, Proline chemistry, Protein Stability, Protein Structure, Secondary, Rifamycins pharmacology, Stereoisomerism, beta 2-Microglobulin genetics, Amino Acid Substitution, Amyloid chemistry, Proline analogs & derivatives, Protein Multimerization drug effects, beta 2-Microglobulin chemistry

Abstract

Conversion of soluble folded proteins into insoluble amyloids generally proceeds in three distinct mechanistic stages: (1) initial protein misfolding into aggregation-competent conformers, (2) subsequent formation of oligomeric species and, finally, (3) self-assembly into extended amyloid fibrils. In the work reported herein, we interrogated the amyloidogenesis mechanism of human β2-microglobulin (β2m), which is thought to be triggered by a pivotal cis-trans isomerization of a proline residue at position 32 in the polypeptide, with nonstandard amino acids. Using chemical protein synthesis we prepared a β2m analogue in which Pro32 was replaced by the conformationally constrained amino acid α-methylproline (MePro). The strong propensity of MePro to adopt a trans prolyl bond led to enhanced population of a non-native [trans-MePro32]β2m protein conformer, which readily formed oligomers at neutral pH. In the presence of the antibiotic rifamycin SV, which inhibits amyloid growth of wild-type β2m, [MePro32]β2m was nearly quantitatively converted into different spherical oligomeric species. Self-assembly into amyloid fibrils was not observed in the absence of seeding, however, even at low pH (<3), where wild-type β2m spontaneously forms amyloids. Nevertheless, we found that aggregation-preorganized [MePro32]β2m can act in a prion-like fashion, templating misfolded conformations in a natively folded protein. Overall, these results provide detailed insight into the role of cis-trans isomerization of Pro32 and ensuing structural rearrangements that lead to initial β2m misfolding and aggregation. They corroborate the view that conformational protein dynamics enabled by reversible Pro32 cis-trans interconversion rather than simple population of the trans conformer is critical for both nucleation and subsequent growth of β2m amyloid structures.

Published

2015