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1. DOP40 Inflammatory Bowel Disease single cell atlas construction to enable cell type-specific target identification

Author

De Baets, G, primary, D'Rozario, J, additional, Gehrman, U, additional, Mattsson, J, additional, Castiblanco, D, additional, Kaymak, I, additional, Moldoveanu, A L, additional, Giorgio, C, additional, Prandi, F, additional, Jawale, C, additional, Honsa, P, additional, Ruppova, K, additional, Valny, M, additional, Macuchova, E, additional, Freinkman, E, additional, Sponarova, J, additional, Platt, A, additional, Ort, T, additional, and Corridoni, D, additional

Published
2024
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2. Unbiased Identification of Serum Response Factor as a Central Profibrotic Mechanism in Idiopathic Pulmonary Fibrosis

Author

Olsson, H., primary, Mattsson, J., additional, Overed-Sayer, C., additional, Stellato, M., additional, McElroy, A., additional, Weidner, J., additional, De Baets, G., additional, Monkley, S., additional, Hühn, M., additional, Muthas, D., additional, Bendtsen, C., additional, Escudero-Ibarz, L., additional, Serrano, A., additional, Barrett, I., additional, Kim, C., additional, Ding, M., additional, Johansson, J., additional, Patten, K., additional, Reichert, S., additional, Lang, V., additional, Sanders, P., additional, Catapano, M., additional, Rosser, G., additional, Puvanendran, A., additional, McMahon, S., additional, and Tame, C., additional

Published
2023
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4. Loss of DPP6 in neurodegenerative dementia: a genetic player in the dysfunction of neuronal excitability

Author

Cacace, R., Heeman, B., Mossevelde, S., Roeck, A., Hoogmartens, J., Rijk, P. (Peter) de, Gossye, H., de Vos, K., Coster, W. de, Strazisar, M., De Baets, G., Schymkowitz, J., Rousseau, M.F. (Francois), Geerts, N., Pooter, T. (Tim) de, Peeters, K. (Karin), Sieben, A., Martin, J. (John), Engelborghs, S. (Sebastiaan), Salmon, E. (E.), Santens, P. (Patrick), Vandenberghe, R. (Rik), Cras, P. (Patrick), Deyn, P.P. (Peter) de, Swieten, J.C. (John) van, Duijn, C.M., Zee, J.A. (Johan) van der, Sleegers, K. (Kristel), Broeckhoven, C. (Christine) van, Goeman, J., Crols, R., Nuytten, D., De Bleecker, J.L., Van Langenhove, T, Ivanoiu, A., Deryck, O., Bergmans, B, Versijpt, J., Michotte, A., Delbeck, J., Willems, C., De Klippel, N., Cacace, R., Heeman, B., Mossevelde, S., Roeck, A., Hoogmartens, J., Rijk, P. (Peter) de, Gossye, H., de Vos, K., Coster, W. de, Strazisar, M., De Baets, G., Schymkowitz, J., Rousseau, M.F. (Francois), Geerts, N., Pooter, T. (Tim) de, Peeters, K. (Karin), Sieben, A., Martin, J. (John), Engelborghs, S. (Sebastiaan), Salmon, E. (E.), Santens, P. (Patrick), Vandenberghe, R. (Rik), Cras, P. (Patrick), Deyn, P.P. (Peter) de, Swieten, J.C. (John) van, Duijn, C.M., Zee, J.A. (Johan) van der, Sleegers, K. (Kristel), Broeckhoven, C. (Christine) van, Goeman, J., Crols, R., Nuytten, D., De Bleecker, J.L., Van Langenhove, T, Ivanoiu, A., Deryck, O., Bergmans, B, Versijpt, J., Michotte, A., Delbeck, J., Willems, C., and De Klippel, N.

Abstract

Emerging evidence suggested a converging mechanism in neurodegenerative brain diseases (NBD) involving early neuronal network dysfunctions and alterations in the homeostasis of neuronal fring as culprits of neurodegeneration. In this study, we used paired-end short-read and direct long-read whole genome sequencing to investigate an unresolved autosomal dominant dementia family signifcantly linked to 7q36. We identifed and validated a chromosomal inversion of ca. 4 Mb, segregating on the disease haplotype and disrupting the coding sequence of dipeptidyl-peptidase 6 gene (DPP6). DPP6 resequencing identifed signifcantly more rare variants—nonsense, frameshift, and missense—in early-onset Alzheimer’s disease (EOAD, p value=0.03, OR=2.21 95% CI 1.05–4.82) and frontotemporal dementia (FTD, p=0.006, OR=2.59, 95% CI 1.28–5.49) patient cohorts. DPP6 is a type II transmembrane protein with a highly structured extracellular domain and is mainly expressed in brain, where it binds to the potassium channel Kv4.2 enhancing its expression, regulating its gating properties and controlling the dendritic excitability of hippocampal neurons. Using in vitro modeling, we showed that the missense variants found in patients destabilize DPP6 and reduce its membrane expression (p<0.001 and p<0.0001) leading to a loss of protein. Reduced DPP6 and/or Kv4.2 expression was also detected in brain tissue of missense variant carriers. Loss of DPP6 is known to cause

Published
2019
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5. Loss of DPP6 in neurodegenerative dementia: a genetic player in the dysfunction of neuronal excitability

Author

Cacace, R, Heeman, B, Mossevelde, S, Roeck, A, Hoogmartens, J, De Rijk, P, Gossye, H, Vos, K, De Coster, W, Strazisar, M, De Baets, G, Schymkowitz, J, Rousseau, F, Geerts, N, De Pooter, T, Peeters, K, Sieben, A, Martin, JJ, Engelborghs, S, Salmon, E, Santens, P, Vandenberghe, R, Cras, P, de Deyn, PP, van Swieten, J.C., Duijn, Cornelia, Zee, JA, Sleegers, K, van Broeckhoven, C, Goeman, J, Crols, R, Nuytten, D, De Bleecker, JL, Van Langenhove, T, Ivanoiu, A, Deryck, O, Bergmans, Bas, Versijpt, J, Michotte, A, Delbeck, J, Willems, C, De Klippel, N, Cacace, R, Heeman, B, Mossevelde, S, Roeck, A, Hoogmartens, J, De Rijk, P, Gossye, H, Vos, K, De Coster, W, Strazisar, M, De Baets, G, Schymkowitz, J, Rousseau, F, Geerts, N, De Pooter, T, Peeters, K, Sieben, A, Martin, JJ, Engelborghs, S, Salmon, E, Santens, P, Vandenberghe, R, Cras, P, de Deyn, PP, van Swieten, J.C., Duijn, Cornelia, Zee, JA, Sleegers, K, van Broeckhoven, C, Goeman, J, Crols, R, Nuytten, D, De Bleecker, JL, Van Langenhove, T, Ivanoiu, A, Deryck, O, Bergmans, Bas, Versijpt, J, Michotte, A, Delbeck, J, Willems, C, and De Klippel, N

Published
2019

7. Molecular plasticity regulates oligomerization and cytotoxicity of the multi-peptide length Abeta pool

Author

Vandersteen, A., Masman, M.F., de Baets, G., Jonckheere, W., van der Werf, Kees, Marrink, S.J., Rozenski, J., Benilova, I., De Strooper, B., Subramaniam, Vinod, Schymkowitz, J., Rousseau, F., Broersen, Kerensa, Nanobiophysics, and Faculty of Science and Technology

Subjects
IR-81968, METIS-288675
Abstract

Current therapeutic approaches under development for Alzheimer disease, including γ-secretase modulating therapy, aim at increasing the production of Aβ1–38 and Aβ1–40 at the cost of longer Aβ peptides. Here, we consider the aggregation of Aβ1–38 and Aβ1–43 in addition to Aβ1–40 and Aβ1–42, in particular their behavior in mixtures representing the complex in vivo Aβ pool. We demonstrate that Aβ1–38 and Aβ1–43 aggregate similar to Aβ1–40 and Aβ1–42, respectively, but display a variation in the kinetics of assembly and toxicity due to differences in short timescale conformational plasticity. In biologically relevant mixtures of Aβ, Aβ1–38 and Aβ1–43 significantly affect the behaviors of Aβ1–40 and Aβ1–42. The short timescale conformational flexibility of Aβ1–38 is suggested to be responsible for enhancing toxicity of Aβ1–40 while exerting a cyto-protective effect on Aβ1–42. Our results indicate that the complex in vivo Aβ peptide array and variations thereof is critical in Alzheimer disease, which can influence the selection of current and new therapeutic strategies

Published
2012

9. X-ray crystal structure of aggregation-resistant protective antigen of Bacillus anthracis (mutant S559L T576E)

Author

Ganesan, A., primary, Siekierska, A., additional, Beerten, J., additional, Brams, M., additional, van Durme, J., additional, De Baets, G., additional, van der Kant, R., additional, Gallardo, R., additional, Ramakers, M., additional, Langenberg, T., additional, Wilkinson, H., additional, De Smet, F., additional, Ulens, C., additional, Rousseau, F., additional, and Schymkowitz, J., additional

Published
2016
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10. A comparative analysis of the aggregation behavior of amyloid-beta peptide variants

Author

Vandersteen, A., Hubin, E., Sarroukh, R., De Baets, G., Schymkowitz, J., Rousseau, F., Subramaniam, V., Raussens, V., Wenschuh, H., Wildemann, D., Broersen, K., Vandersteen, A., Hubin, E., Sarroukh, R., De Baets, G., Schymkowitz, J., Rousseau, F., Subramaniam, V., Raussens, V., Wenschuh, H., Wildemann, D., and Broersen, K.

Abstract

Item does not contain fulltext, Aggregated forms of the amyloid-beta peptide are hypothesized to act as the prime toxic agents in Alzheimer disease (AD). The in vivo amyloid-beta peptide pool consists of both C- and N-terminally truncated or mutated peptides, and the composition thereof significantly determines AD risk. Other variations, such as biotinylation, are introduced as molecular tools to aid the understanding of disease mechanisms. Since these modifications have the potential to alter key aggregation properties of the amyloid-beta peptide, we present a comparative study of the aggregation of a substantial set of the most common in vivo identified and in vitro produced amyloid-beta peptides. STRUCTURED SUMMARY OF PROTEIN INTERACTIONS: Amyloid beta and Amyloid betabind by fluorescence technology (View Interaction: 1, 2, 3, 4, 5) Amyloid beta and Amyloid betabind by transmission electron microscopy (View Interaction: 1, 2) Amyloid beta and Amyloid betabind by filter binding (View Interaction: 1, 2, 3).

Published
2012

11. Molecular Plasticity Regulates Oligomerization and Cytotoxicity of the Multipeptide-length Amyloid-beta Peptide Pool

Author

Vandersteen, A., Masman, M.F., De Baets, G., Jonckheere, W., van der Werf, K., Marrink, S.J., Rozenski, J., Benilova, I., De Strooper, B., Subramaniam, V., Schymkowitz, J., Rousseau, F., Broersen, K., Vandersteen, A., Masman, M.F., De Baets, G., Jonckheere, W., van der Werf, K., Marrink, S.J., Rozenski, J., Benilova, I., De Strooper, B., Subramaniam, V., Schymkowitz, J., Rousseau, F., and Broersen, K.

Abstract

Contains fulltext : 108708.pdf (Publisher’s version ) (Open Access), Current therapeutic approaches under development for Alzheimer disease, including gamma-secretase modulating therapy, aim at increasing the production of Abeta(1-38) and Abeta(1-40) at the cost of longer Abeta peptides. Here, we consider the aggregation of Abeta(1-38) and Abeta(1-43) in addition to Abeta(1-40) and Abeta(1-42), in particular their behavior in mixtures representing the complex in vivo Abeta pool. We demonstrate that Abeta(1-38) and Abeta(1-43) aggregate similar to Abeta(1-40) and Abeta(1-42), respectively, but display a variation in the kinetics of assembly and toxicity due to differences in short timescale conformational plasticity. In biologically relevant mixtures of Abeta, Abeta(1-38) and Abeta(1-43) significantly affect the behaviors of Abeta(1-40) and Abeta(1-42). The short timescale conformational flexibility of Abeta(1-38) is suggested to be responsible for enhancing toxicity of Abeta(1-40) while exerting a cyto-protective effect on Abeta(1-42). Our results indicate that the complex in vivo Abeta peptide array and variations thereof is critical in Alzheimer disease, which can influence the selection of current and new therapeutic strategies.

Published
2012

13. Assessing computational predictions of the phenotypic effect of cystathionine-beta-synthase variants

Author

Ayodeji Olatubosun, Dago F Dimster-Denk, Zhiqiang Hu, Pier Luigi Martelli, Mauno Vihinen, Olivier Lichtarge, Frederic Rousseau, Iddo Friedberg, Castrense Savojardo, Sean D. Mooney, Emanuela Leonardi, Greet De Baets, Manuel Giollo, Jouni Väliaho, Yana Bromberg, Rachel Karchin, Chen Cao, Janita Thusberg, Changhua Yu, Susanna Repo, Rita Casadio, David L. Masica, Laura Kasak, Emidio Capriotti, Jasper Rine, Gaurav Pandey, Silvio C. E. Tosatto, John Moult, Lipika R. Pal, Steven E. Brenner, Predrag Radivojac, Panagiotis Katsonis, Joost Schymkowitz, Joost Van Durme, Constantina Bakolitsa, Kasak L., Bakolitsa C., Hu Z., Yu C., Rine J., Dimster-Denk D.F., Pandey G., De Baets G., Bromberg Y., Cao C., Capriotti E., Casadio R., Van Durme J., Giollo M., Karchin R., Katsonis P., Leonardi E., Lichtarge O., Martelli P.L., Masica D., Mooney S.D., Olatubosun A., Radivojac P., Rousseau F., Pal L.R., Savojardo C., Schymkowitz J., Thusberg J., Tosatto S.C.E., Vihinen M., Valiaho J., Repo S., Moult J., Brenner S.E., and Friedberg I.

Subjects
Homocysteine, IMPACT, ved/biology.organism_classification_rank.species, Transsulfuration pathway, chemistry.chemical_compound, 2.1 Biological and endogenous factors, Single amino acid, Aetiology, Precision Medicine, Genetics (clinical), Genetics & Heredity, PROTEIN FUNCTION, 0303 health sciences, biology, 030305 genetics & heredity, CAGI challenge, SNAP, Phenotype, machine learning, Networking and Information Technology R&D (NITRD), phenotype prediction, critical assessment, Life Sciences & Biomedicine, cystathionine-beta-synthase, ENZYME, Clinical Sciences, Cystathionine beta-Synthase, Homocystinuria, Computational biology, single amino acid substitution, CLASSIFICATION, Article, 03 medical and health sciences, Cystathionine, Genetics, medicine, Humans, Model organism, 030304 developmental biology, SERVER, TOOLS, Science & Technology, MUTATIONS, business.industry, ved/biology, Computational Biology, medicine.disease, Cystathionine beta synthase, Good Health and Well Being, chemistry, Amino Acid Substitution, biology.protein, Generic health relevance, Personalized medicine, business, PATHOGENICITY
Abstract

Accurate prediction of the impact of genomic variation on phenotype is a major goal of computational biology and an important contributor to personalized medicine. Computational predictions can lead to a better understanding of the mechanisms underlying genetic diseases, including cancer, but their adoption requires thorough and unbiased assessment. Cystathionine-beta-synthase (CBS) is an enzyme that catalyzes the first step of the transsulfuration pathway, from homocysteine to cystathionine, and in which variations are associated with human hyperhomocysteinemia and homocystinuria. We have created a computational challenge under the CAGI framework to evaluate how well different methods can predict the phenotypic effect(s) of CBS single amino acid substitutions using a blinded experimental data set. CAGI participants were asked to predict yeast growth based on the identity of the mutations. The performance of the methods was evaluated using several metrics. The CBS challenge highlighted the difficulty of predicting the phenotype of an ex vivo system in a model organism when classification models were trained on human disease data. We also discuss the variations in difficulty of prediction for known benign and deleterious variants, as well as identify methodological and experimental constraints with lessons to be learned for future challenges. ispartof: HUMAN MUTATION vol:40 issue:9 pages:1530-1545 ispartof: location:United States status: published

Published
2019

14. Reduced Levels of Misfolded and Aggregated Mutant p53 by Proteostatic Activation.

Author

Naus E, Derweduwe M, Lampi Y, Claeys A, Pauwels J, Langenberg T, Claes F, Xu J, Haemels V, Atak ZK, van der Kant R, Van Durme J, De Baets G, Ligon KL, Fiers M, Gevaert K, Aerts S, Rousseau F, Schymkowitz J, and De Smet F

Subjects
Proteasome Inhibitors pharmacology, Heat-Shock Response, Bortezomib pharmacology, Tumor Suppressor Protein p53 genetics, Tumor Suppressor Protein p53 metabolism, Protein Folding
Abstract

In malignant cancer, excessive amounts of mutant p53 often lead to its aggregation, a feature that was recently identified as druggable. Here, we describe that induction of a heat shock-related stress response mediated by Foldlin, a small-molecule tool compound, reduces the protein levels of misfolded/aggregated mutant p53, while contact mutants or wild-type p53 remain largely unaffected. Foldlin also prevented the formation of stress-induced p53 nuclear inclusion bodies. Despite our inability to identify a specific molecular target, Foldlin also reduced protein levels of aggregating SOD1 variants. Finally, by screening a library of 778 FDA-approved compounds for their ability to reduce misfolded mutant p53, we identified the proteasome inhibitor Bortezomib with similar cellular effects as Foldlin. Overall, the induction of a cellular heat shock response seems to be an effective strategy to deal with pathological protein aggregation. It remains to be seen however, how this strategy can be translated to a clinical setting.

Published
2023
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15. Exposure of a cryptic Hsp70 binding site determines the cytotoxicity of the ALS-associated SOD1-mutant A4V.

Author

Claes F, Rudyak S, Laird AS, Louros N, Beerten J, Debulpaep M, Michiels E, van der Kant R, Van Durme J, De Baets G, Houben B, Ramakers M, Yuan K, Gwee SSL, Hernandez S, Broersen K, Oliveberg M, Moahamed B, Kirstein J, Robberecht W, Rousseau F, and Schymkowitz J

Subjects
Binding Sites, Humans, Models, Molecular, Protein Binding, Protein Conformation, Superoxide Dismutase-1 chemistry, Amyotrophic Lateral Sclerosis genetics, HSP70 Heat-Shock Proteins metabolism, Mutation, Protein Engineering, Superoxide Dismutase-1 genetics, Superoxide Dismutase-1 metabolism
Abstract

The accumulation of toxic protein aggregates is thought to play a key role in a range of degenerative pathologies, but it remains unclear why aggregation of polypeptides into non-native assemblies is toxic and why cellular clearance pathways offer ineffective protection. We here study the A4V mutant of SOD1, which forms toxic aggregates in motor neurons of patients with familial amyotrophic lateral sclerosis (ALS). A comparison of the location of aggregation prone regions (APRs) and Hsp70 binding sites in the denatured state of SOD1 reveals that ALS-associated mutations promote exposure of the APRs more than the strongest Hsc/Hsp70 binding site that we could detect. Mutations designed to increase the exposure of this Hsp70 interaction site in the denatured state promote aggregation but also display an increased interaction with Hsp70 chaperones. Depending on the cell type, in vitro this resulted in cellular inclusion body formation or increased clearance, accompanied with a suppression of cytotoxicity. The latter was also observed in a zebrafish model in vivo. Our results suggest that the uncontrolled accumulation of toxic SOD1A4V aggregates results from insufficient detection by the cellular surveillance network., (© The Author(s) 2020. Published by Oxford University Press. All rights reserved. For Permissions, please e-mail: journals.permissions@oup.com.)

Published
2019
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16. Assessing computational predictions of the phenotypic effect of cystathionine-beta-synthase variants.

Author

Kasak L, Bakolitsa C, Hu Z, Yu C, Rine J, Dimster-Denk DF, Pandey G, De Baets G, Bromberg Y, Cao C, Capriotti E, Casadio R, Van Durme J, Giollo M, Karchin R, Katsonis P, Leonardi E, Lichtarge O, Martelli PL, Masica D, Mooney SD, Olatubosun A, Radivojac P, Rousseau F, Pal LR, Savojardo C, Schymkowitz J, Thusberg J, Tosatto SCE, Vihinen M, Väliaho J, Repo S, Moult J, Brenner SE, and Friedberg I

Subjects
Cystathionine metabolism, Cystathionine beta-Synthase metabolism, Homocysteine metabolism, Humans, Phenotype, Precision Medicine, Amino Acid Substitution, Computational Biology methods, Cystathionine beta-Synthase genetics
Abstract

Accurate prediction of the impact of genomic variation on phenotype is a major goal of computational biology and an important contributor to personalized medicine. Computational predictions can lead to a better understanding of the mechanisms underlying genetic diseases, including cancer, but their adoption requires thorough and unbiased assessment. Cystathionine-beta-synthase (CBS) is an enzyme that catalyzes the first step of the transsulfuration pathway, from homocysteine to cystathionine, and in which variations are associated with human hyperhomocysteinemia and homocystinuria. We have created a computational challenge under the CAGI framework to evaluate how well different methods can predict the phenotypic effect(s) of CBS single amino acid substitutions using a blinded experimental data set. CAGI participants were asked to predict yeast growth based on the identity of the mutations. The performance of the methods was evaluated using several metrics. The CBS challenge highlighted the difficulty of predicting the phenotype of an ex vivo system in a model organism when classification models were trained on human disease data. We also discuss the variations in difficulty of prediction for known benign and deleterious variants, as well as identify methodological and experimental constraints with lessons to be learned for future challenges., (© 2019 Wiley Periodicals, Inc.)

Published
2019
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17. Loss of DPP6 in neurodegenerative dementia: a genetic player in the dysfunction of neuronal excitability.

Author

Cacace R, Heeman B, Van Mossevelde S, De Roeck A, Hoogmartens J, De Rijk P, Gossye H, De Vos K, De Coster W, Strazisar M, De Baets G, Schymkowitz J, Rousseau F, Geerts N, De Pooter T, Peeters K, Sieben A, Martin JJ, Engelborghs S, Salmon E, Santens P, Vandenberghe R, Cras P, P De Deyn P, C van Swieten J, M van Duijn C, van der Zee J, Sleegers K, and Van Broeckhoven C

Subjects
Action Potentials physiology, Adult, Aged, Chromosomes, Human, Pair 7 genetics, Dementia physiopathology, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases genetics, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases physiology, Female, Genes, Dominant, Homeostasis, Humans, Male, Middle Aged, Nerve Tissue Proteins genetics, Nerve Tissue Proteins physiology, Neurodegenerative Diseases physiopathology, Pedigree, Penetrance, Polymorphism, Single Nucleotide, Potassium Channels genetics, Potassium Channels physiology, Protein Stability, Protein Transport, Synaptic Transmission, Whole Genome Sequencing, Chromosome Inversion, Dementia genetics, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases deficiency, Mutation, Nerve Tissue Proteins deficiency, Neurodegenerative Diseases genetics, Neurons physiology, Potassium Channels deficiency
Abstract

Emerging evidence suggested a converging mechanism in neurodegenerative brain diseases (NBD) involving early neuronal network dysfunctions and alterations in the homeostasis of neuronal firing as culprits of neurodegeneration. In this study, we used paired-end short-read and direct long-read whole genome sequencing to investigate an unresolved autosomal dominant dementia family significantly linked to 7q36. We identified and validated a chromosomal inversion of ca. 4 Mb, segregating on the disease haplotype and disrupting the coding sequence of dipeptidyl-peptidase 6 gene (DPP6). DPP6 resequencing identified significantly more rare variants-nonsense, frameshift, and missense-in early-onset Alzheimer's disease (EOAD, p value = 0.03, OR = 2.21 95% CI 1.05-4.82) and frontotemporal dementia (FTD, p = 0.006, OR = 2.59, 95% CI 1.28-5.49) patient cohorts. DPP6 is a type II transmembrane protein with a highly structured extracellular domain and is mainly expressed in brain, where it binds to the potassium channel K v 4.2 enhancing its expression, regulating its gating properties and controlling the dendritic excitability of hippocampal neurons. Using in vitro modeling, we showed that the missense variants found in patients destabilize DPP6 and reduce its membrane expression (p < 0.001 and p < 0.0001) leading to a loss of protein. Reduced DPP6 and/or K v 4.2 expression was also detected in brain tissue of missense variant carriers. Loss of DPP6 is known to cause neuronal hyperexcitability and behavioral alterations in Dpp6-KO mice. Taken together, the results of our genomic, genetic, expression and modeling analyses, provided direct evidence supporting the involvement of DPP6 loss in dementia. We propose that loss of function variants have a higher penetrance and disease impact, whereas the missense variants have a variable risk contribution to disease that can vary from high to low penetrance. Our findings of DPP6, as novel gene in dementia, strengthen the involvement of neuronal hyperexcitability and alteration in the homeostasis of neuronal firing as a disease mechanism to further investigate.

Published
2019
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18. High-throughput discovery of functional disordered regions: investigation of transactivation domains.

Author

Ravarani CN, Erkina TY, De Baets G, Dudman DC, Erkine AM, and Babu MM

Subjects
Cloning, Molecular, Gene Library, High-Throughput Nucleotide Sequencing, Machine Learning, Proteome genetics, Sequence Analysis, DNA, DNA-Binding Proteins genetics, Heat-Shock Proteins genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins genetics, Transcription Factors genetics, Transcriptional Activation
Abstract

Over 40% of proteins in any eukaryotic genome encode intrinsically disordered regions (IDRs) that do not adopt defined tertiary structures. Certain IDRs perform critical functions, but discovering them is non-trivial as the biological context determines their function. We present IDR-Screen, a framework to discover functional IDRs in a high-throughput manner by simultaneously assaying large numbers of DNA sequences that code for short disordered sequences. Functionality-conferring patterns in their protein sequence are inferred through statistical learning. Using yeast HSF1 transcription factor-based assay, we discovered IDRs that function as transactivation domains (TADs) by screening a random sequence library and a designed library consisting of variants of 13 diverse TADs. Using machine learning, we find that segments devoid of positively charged residues but with redundant short sequence patterns of negatively charged and aromatic residues are a generic feature for TAD functionality. We anticipate that investigating defined sequence libraries using IDR-Screen for specific functions can facilitate discovering novel and functional regions of the disordered proteome as well as understand the impact of natural and disease variants in disordered segments., (© 2018 MRC Laboratory of Molecular Biology. Published under the terms of the CC BY 4.0 license.)

Published
2018
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19. AmyPro: a database of proteins with validated amyloidogenic regions.

Author

Varadi M, De Baets G, Vranken WF, Tompa P, and Pancsa R

Subjects
User-Computer Interface, Amyloidogenic Proteins chemistry, Databases, Protein
Abstract

Soluble functional proteins may transform into insoluble amyloid fibrils that deposit in a variety of tissues. Amyloid formation is a hallmark of age-related degenerative disorders. Perhaps surprisingly, amyloid fibrils can also be beneficial and are frequently exploited for diverse functional roles in organisms. Here we introduce AmyPro, an open-access database providing a comprehensive, carefully curated collection of validated amyloid fibril-forming proteins from all kingdoms of life classified into broad functional categories (http://amypro.net). In particular, AmyPro provides the boundaries of experimentally validated amyloidogenic sequence regions, short descriptions of the functional relevance of the proteins and their amyloid state, a list of the experimental techniques applied to study the amyloid state, important structural/functional/variation/mutation data transferred from UniProt, a list of relevant PDB structures categorized according to protein states, database cross-references and literature references. AmyPro greatly improves on similar currently available resources by incorporating both prions and functional amyloids in addition to pathogenic amyloids, and allows users to screen their sequences against the entire collection of validated amyloidogenic sequence fragments. By enabling further elucidation of the sequential determinants of amyloid fibril formation, we hope AmyPro will enhance the development of new methods for the precise prediction of amyloidogenic regions within proteins., (© The Author(s) 2017. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published
2018
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20. Nuclear inclusion bodies of mutant and wild-type p53 in cancer: a hallmark of p53 inactivation and proteostasis remodelling by p53 aggregation.

Author

De Smet F, Saiz Rubio M, Hompes D, Naus E, De Baets G, Langenberg T, Hipp MS, Houben B, Claes F, Charbonneau S, Delgado Blanco J, Plaisance S, Ramkissoon S, Ramkissoon L, Simons C, van den Brandt P, Weijenberg M, Van England M, Lambrechts S, Amant F, D'Hoore A, Ligon KL, Sagaert X, Schymkowitz J, and Rousseau F

Subjects
Biopsy, Cell Line, Tumor, Colonic Neoplasms complications, Colonic Neoplasms metabolism, Colonic Neoplasms pathology, Cytoplasm metabolism, Glioblastoma complications, Glioblastoma metabolism, Glioblastoma pathology, Heat-Shock Response genetics, Heat-Shock Response physiology, Humans, Kaplan-Meier Estimate, Mutation, Protein Aggregation, Pathological etiology, Protein Aggregation, Pathological metabolism, Proteostasis Deficiencies etiology, Proteostasis Deficiencies metabolism, Receptors, sigma metabolism, Tumor Suppressor Protein p53 metabolism, Colonic Neoplasms genetics, Glioblastoma genetics, Intranuclear Inclusion Bodies metabolism, Protein Aggregation, Pathological genetics, Proteostasis Deficiencies genetics, Tumor Suppressor Protein p53 genetics
Abstract

Although p53 protein aggregates have been observed in cancer cell lines and tumour tissue, their impact in cancer remains largely unknown. Here, we extensively screened for p53 aggregation phenotypes in tumour biopsies, and identified nuclear inclusion bodies (nIBs) of transcriptionally inactive mutant or wild-type p53 as the most frequent aggregation-like phenotype across six different cancer types. p53-positive nIBs co-stained with nuclear aggregation markers, and shared molecular hallmarks of nIBs commonly found in neurodegenerative disorders. In cell culture, tumour-associated stress was a strong inducer of p53 aggregation and nIB formation. This was most prominent for mutant p53, but could also be observed in wild-type p53 cell lines, for which nIB formation correlated with the loss of p53's transcriptional activity. Importantly, protein aggregation also fuelled the dysregulation of the proteostasis network in the tumour cell by inducing a hyperactivated, oncogenic heat-shock response, to which tumours are commonly addicted, and by overloading the proteasomal degradation system, an observation that was most pronounced for structurally destabilized mutant p53. Patients showing tumours with p53-positive nIBs suffered from a poor clinical outcome, similar to those with loss of p53 expression, and tumour biopsies showed a differential proteostatic expression profile associated with p53-positive nIBs. p53-positive nIBs therefore highlight a malignant state of the tumour that results from the interplay between (1) the functional inactivation of p53 through mutation and/or aggregation, and (2) microenvironmental stress, a combination that catalyses proteostatic dysregulation. This study highlights several unexpected clinical, biological and therapeutically unexplored parallels between cancer and neurodegeneration. Copyright © 2017 Pathological Society of Great Britain and Ireland. Published by John Wiley & Sons, Ltd., (Copyright © 2016 Pathological Society of Great Britain and Ireland. Published by John Wiley & Sons, Ltd.)

Published
2017
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21. Solubis: a webserver to reduce protein aggregation through mutation.

Author

Van Durme J, De Baets G, Van Der Kant R, Ramakers M, Ganesan A, Wilkinson H, Gallardo R, Rousseau F, and Schymkowitz J

Subjects
Algorithms, Databases, Protein, Models, Molecular, Protein Conformation, Protein Stability, Thermodynamics, User-Computer Interface, Computational Biology methods, Internet, Mutation, Protein Aggregates genetics, Proteins chemistry, Proteins genetics, Software
Abstract

Protein aggregation is a major factor limiting the biotechnological and therapeutic application of many proteins, including enzymes and monoclonal antibodies. The molecular principles underlying aggregation are by now sufficiently understood to allow rational redesign of natural polypeptide sequences for decreased aggregation tendency, and hence potentially increased expression and solubility. Given that aggregation-prone regions (APRs) tend to contribute to the stability of the hydrophobic core or to functional sites of the protein, mutations in these regions have to be carefully selected in order not to disrupt protein structure or function. Therefore, we here provide access to an automated pipeline to identify mutations that reduce protein aggregation by reducing the intrinsic aggregation propensity of the sequence (using the TANGO algorithm), while taking care not to disrupt the thermodynamic stability of the native structure (using the empirical force-field FoldX). Moreover, by providing a plot of the intrinsic aggregation propensity score of APRs corrected by the local stability of that region in the folded structure, we allow users to prioritize those regions in the protein that are most in need of improvement through protein engineering. The method can be accessed at http://solubis.switchlab.org/., (© The Author 2016. Published by Oxford University Press. All rights reserved. For Permissions, please e-mail: journals.permissions@oup.com.)

Published
2016
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22. Restricted Location of PSEN2/γ-Secretase Determines Substrate Specificity and Generates an Intracellular Aβ Pool.

Author

Sannerud R, Esselens C, Ejsmont P, Mattera R, Rochin L, Tharkeshwar AK, De Baets G, De Wever V, Habets R, Baert V, Vermeire W, Michiels C, Groot AJ, Wouters R, Dillen K, Vints K, Baatsen P, Munck S, Derua R, Waelkens E, Basi GS, Mercken M, Vooijs M, Bollen M, Schymkowitz J, Rousseau F, Bonifacino JS, Van Niel G, De Strooper B, and Annaert W

Subjects
Adaptor Protein Complex 1 metabolism, Alzheimer Disease genetics, Alzheimer Disease metabolism, Amino Acid Motifs, Amyloid Precursor Protein Secretases metabolism, Animals, Cell Line, Tumor, Endosomes chemistry, Humans, Lysosomes chemistry, Mice, Presenilin-1 analysis, Presenilin-1 chemistry, Presenilin-1 genetics, Presenilin-1 metabolism, Presenilin-2 chemistry, Presenilin-2 genetics, Presenilin-2 metabolism, Rats, Substrate Specificity, Alzheimer Disease pathology, Amyloid Precursor Protein Secretases analysis, Amyloid beta-Peptides metabolism, Peptide Fragments metabolism, Presenilin-2 analysis
Abstract

γ-Secretases are a family of intramembrane-cleaving proteases involved in various signaling pathways and diseases, including Alzheimer's disease (AD). Cells co-express differing γ-secretase complexes, including two homologous presenilins (PSENs). We examined the significance of this heterogeneity and identified a unique motif in PSEN2 that directs this γ-secretase to late endosomes/lysosomes via a phosphorylation-dependent interaction with the AP-1 adaptor complex. Accordingly, PSEN2 selectively cleaves late endosomal/lysosomal localized substrates and generates the prominent pool of intracellular Aβ that contains longer Aβ; familial AD (FAD)-associated mutations in PSEN2 increased the levels of longer Aβ further. Moreover, a subset of FAD mutants in PSEN1, normally more broadly distributed in the cell, phenocopies PSEN2 and shifts its localization to late endosomes/lysosomes. Thus, localization of γ-secretases determines substrate specificity, while FAD-causing mutations strongly enhance accumulation of aggregation-prone Aβ42 in intracellular acidic compartments. The findings reveal potentially important roles for specific intracellular, localized reactions contributing to AD pathogenesis., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published
2016
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23. Structural hot spots for the solubility of globular proteins.

Author

Ganesan A, Siekierska A, Beerten J, Brams M, Van Durme J, De Baets G, Van der Kant R, Gallardo R, Ramakers M, Langenberg T, Wilkinson H, De Smet F, Ulens C, Rousseau F, and Schymkowitz J

Subjects
Amino Acid Sequence, Antigens, Bacterial chemistry, Antigens, Bacterial genetics, Bacterial Toxins chemistry, Bacterial Toxins genetics, Blotting, Western, Cell Line, Tumor, Chromatography, Gel, Crystallography, X-Ray, Electrophoresis, Polyacrylamide Gel, HeLa Cells, Humans, Mutation, Protein Stability, Solubility, alpha-Galactosidase chemistry, alpha-Galactosidase genetics, Antigens, Bacterial metabolism, Bacterial Toxins metabolism, alpha-Galactosidase metabolism
Abstract

Natural selection shapes protein solubility to physiological requirements and recombinant applications that require higher protein concentrations are often problematic. This raises the question whether the solubility of natural protein sequences can be improved. We here show an anti-correlation between the number of aggregation prone regions (APRs) in a protein sequence and its solubility, suggesting that mutational suppression of APRs provides a simple strategy to increase protein solubility. We show that mutations at specific positions within a protein structure can act as APR suppressors without affecting protein stability. These hot spots for protein solubility are both structure and sequence dependent but can be computationally predicted. We demonstrate this by reducing the aggregation of human α-galactosidase and protective antigen of Bacillus anthracis through mutation. Our results indicate that many proteins possess hot spots allowing to adapt protein solubility independently of structure and function.

Published
2016
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24. Drosophila screen connects nuclear transport genes to DPR pathology in c9ALS/FTD.

Author

Boeynaems S, Bogaert E, Michiels E, Gijselinck I, Sieben A, Jovičić A, De Baets G, Scheveneels W, Steyaert J, Cuijt I, Verstrepen KJ, Callaerts P, Rousseau F, Schymkowitz J, Cruts M, Van Broeckhoven C, Van Damme P, Gitler AD, Robberecht W, and Van Den Bosch L

Subjects
Active Transport, Cell Nucleus genetics, Animals, Arginine metabolism, Disease Models, Animal, Eye pathology, HeLa Cells, Humans, Methylation, RNA Interference, Amyotrophic Lateral Sclerosis genetics, Cell Nucleus metabolism, Dipeptides chemistry, Drosophila melanogaster genetics, Frontotemporal Dementia genetics, Genes, Insect, Genetic Testing, Repetitive Sequences, Amino Acid
Abstract

Hexanucleotide repeat expansions in C9orf72 are the most common cause of amyotrophic lateral sclerosis (ALS) and frontotemporal degeneration (FTD) (c9ALS/FTD). Unconventional translation of these repeats produces dipeptide repeat proteins (DPRs) that may cause neurodegeneration. We performed a modifier screen in Drosophila and discovered a critical role for importins and exportins, Ran-GTP cycle regulators, nuclear pore components, and arginine methylases in mediating DPR toxicity. These findings provide evidence for an important role for nucleocytoplasmic transport in the pathogenic mechanism of c9ALS/FTD.

Published
2016
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25. Loss of TBK1 is a frequent cause of frontotemporal dementia in a Belgian cohort.

Author

Gijselinck I, Van Mossevelde S, van der Zee J, Sieben A, Philtjens S, Heeman B, Engelborghs S, Vandenbulcke M, De Baets G, Bäumer V, Cuijt I, Van den Broeck M, Peeters K, Mattheijssens M, Rousseau F, Vandenberghe R, De Jonghe P, Cras P, De Deyn PP, Martin JJ, Cruts M, and Van Broeckhoven C

Subjects
Adult, Aged, Aged, 80 and over, Belgium epidemiology, Cohort Studies, Female, Frontotemporal Dementia epidemiology, Humans, Male, Middle Aged, Pedigree, Frontotemporal Dementia diagnosis, Frontotemporal Dementia genetics, Mutation genetics, Protein Serine-Threonine Kinases deficiency, Protein Serine-Threonine Kinases genetics
Abstract

Objective: To assess the genetic contribution of TBK1, a gene implicated in amyotrophic lateral sclerosis (ALS), frontotemporal dementia (FTD), and FTD-ALS, in Belgian FTD and ALS patient cohorts containing a significant part of genetically unresolved patients., Methods: We sequenced TBK1 in a hospital-based cohort of 482 unrelated patients with FTD and FTD-ALS and 147 patients with ALS and an extended Belgian FTD-ALS family DR158. We followed up mutation carriers by segregation studies, transcript and protein expression analysis, and immunohistochemistry., Results: We identified 11 patients carrying a loss-of-function (LOF) mutation resulting in an overall mutation frequency of 1.7% (11/629), 1.1% in patients with FTD (5/460), 3.4% in patients with ALS (5/147), and 4.5% in patients with FTD-ALS (1/22). We found 1 LOF mutation, p.Glu643del, in 6 unrelated patients segregating with disease in family DR158. Of 2 mutation carriers, brain and spinal cord was characterized by TDP-43-positive pathology. The LOF mutations including the p.Glu643del mutation led to loss of transcript or protein in blood and brain., Conclusions: TBK1 LOF mutations are the third most frequent cause of clinical FTD in the Belgian clinically based patient cohort, after C9orf72 and GRN, and the second most common cause of clinical ALS after C9orf72. These findings reinforce that FTD and ALS belong to the same disease continuum., (© 2015 American Academy of Neurology.)

Published
2015
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26. Increased Aggregation Is More Frequently Associated to Human Disease-Associated Mutations Than to Neutral Polymorphisms.

Author

De Baets G, Van Doorn L, Rousseau F, and Schymkowitz J

Subjects
Computational Biology, Databases, Factual, Humans, Protein Stability, Genetic Predisposition to Disease genetics, Mutation genetics, Polymorphism, Genetic genetics, Protein Aggregation, Pathological genetics
Abstract

Protein aggregation is a hallmark of over 30 human pathologies. In these diseases, the aggregation of one or a few specific proteins is often toxic, leading to cellular degeneration and/or organ disruption in addition to the loss-of-function resulting from protein misfolding. Although the pathophysiological consequences of these diseases are overt, the molecular dysregulations leading to aggregate toxicity are still unclear and appear to be diverse and multifactorial. The molecular mechanisms of protein aggregation and therefore the biophysical parameters favoring protein aggregation are better understood. Here we perform an in silico survey of the impact of human sequence variation on the aggregation propensity of human proteins. We find that disease-associated variations are statistically significantly enriched in mutations that increase the aggregation potential of human proteins when compared to neutral sequence variations. These findings suggest that protein aggregation might have a broader impact on human disease than generally assumed and that beyond loss-of-function, the aggregation of mutant proteins involved in cancer, immune disorders or inflammation could potentially further contribute to disease by additional burden on cellular protein homeostasis.

Published
2015
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27. Solubis: optimize your protein.

Author

De Baets G, Van Durme J, van der Kant R, Schymkowitz J, and Rousseau F

Subjects
Databases, Protein, Humans, Protein Conformation, Protein Multimerization, Protein Stability, Proteins metabolism, Thermodynamics, Mutation genetics, Protein Folding, Proteins chemistry, Proteins genetics, Sequence Analysis, Protein methods, Software
Abstract

Motivation: Protein aggregation is associated with a number of protein misfolding diseases and is a major concern for therapeutic proteins. Aggregation is caused by the presence of aggregation-prone regions (APRs) in the amino acid sequence of the protein. The lower the aggregation propensity of APRs and the better they are protected by native interactions within the folded structure of the protein, the more aggregation is prevented. Therefore, both the local thermodynamic stability of APRs in the native structure and their intrinsic aggregation propensity are a key parameter that needs to be optimized to prevent protein aggregation., Results: The Solubis method presented here automates the process of carefully selecting point mutations that minimize the intrinsic aggregation propensity while improving local protein stability., (© The Author 2015. Published by Oxford University Press. All rights reserved. For Permissions, please e-mail: journals.permissions@oup.com.)

Published
2015
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28. Selectivity of aggregation-determining interactions.

Author

Ganesan A, Debulpaep M, Wilkinson H, Van Durme J, De Baets G, Jonckheere W, Ramakers M, Ivarsson Y, Zimmermann P, Van Eldere J, Schymkowitz J, and Rousseau F

Subjects
Bacterial Proteins metabolism, C-Reactive Protein genetics, C-Reactive Protein metabolism, Escherichia coli genetics, Escherichia coli metabolism, Humans, Male, Molecular Chaperones genetics, Molecular Chaperones metabolism, Peptides metabolism, Prostate-Specific Antigen blood, Prostate-Specific Antigen genetics, Protein Binding genetics, Proteome genetics, Proteome metabolism, Proteomics methods, Spectroscopy, Fourier Transform Infrared, beta-Galactosidase metabolism, Bacterial Proteins genetics, Protein Aggregates, Protein Interaction Maps, beta-Galactosidase genetics
Abstract

Protein aggregation is sequence specific, favoring self-assembly over cross-seeding with non-homologous sequences. Still, as the majority of proteins in a proteome are aggregation prone, the high level of homogeneity of protein inclusions in vivo both during recombinant overexpression and in disease remains surprising. To investigate the selectivity of protein aggregation in a proteomic context, we here compared the selectivity of aggregation-determined interactions with antibody binding. To that purpose, we synthesized biotin-labeled peptides, corresponding to aggregation-determining sequences of the bacterial protein β-galactosidase and two human disease biomarkers: C-reactive protein and prostate-specific antigen. We analyzed the selectivity of their interactions in Escherichia coli lysate, human serum and human seminal plasma, respectively, using a Western blot-like approach in which the aggregating peptides replace the conventional antibody. We observed specific peptide accumulation in the same bands detected by antibody staining. Combined spectroscopic and mutagenic studies confirmed accumulation resulted from binding of the peptide on the identical sequence of the immobilized target protein. Further, we analyzed the sequence redundancy of aggregating sequences and found that about 90% of them are unique within their proteome. As a result, the combined specificity and low sequence redundancy of aggregating sequences therefore contribute to the observed homogeneity of protein aggregation in vivo. This suggests that these intrinsic proteomic properties naturally compartmentalize aggregation events in sequence space. In the event of physiological stress, this might benefit the ability of cells to respond to proteostatic stress by allowing chaperones to focus on specific aggregation events rather than having to face systemic proteostatic failure., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published
2015
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29. Sequence-dependent internalization of aggregating peptides.

Author

Couceiro JR, Gallardo R, De Smet F, De Baets G, Baatsen P, Annaert W, Roose K, Saelens X, Schymkowitz J, and Rousseau F

Subjects
Actin Cytoskeleton chemistry, Actin Cytoskeleton drug effects, Actin Cytoskeleton metabolism, Amiloride analogs & derivatives, Amiloride pharmacology, Amino Acid Sequence, Cytochalasin D pharmacology, DNA-Binding Proteins metabolism, Endocytosis drug effects, Endosomes drug effects, HEK293 Cells, HSP70 Heat-Shock Proteins metabolism, Heat Shock Transcription Factors, Humans, Hydrazones pharmacology, Hydrogen-Ion Concentration, Kinetics, Lovastatin pharmacology, Lysosomes drug effects, Molecular Sequence Data, Peptides chemical synthesis, Peptides chemistry, Protein Binding, Protein Folding, Protein Transport drug effects, Protein Transport physiology, Proteolysis, Structure-Activity Relationship, Transcription Factors metabolism, Endocytosis physiology, Endosomes metabolism, Lysosomes metabolism, Peptides metabolism, Protein Aggregates
Abstract

Recently, a number of aggregation disease polypeptides have been shown to spread from cell to cell, thereby displaying prionoid behavior. Studying aggregate internalization, however, is often hampered by the complex kinetics of the aggregation process, resulting in the concomitant uptake of aggregates of different sizes by competing mechanisms, which makes it difficult to isolate pathway-specific responses to aggregates. We designed synthetic aggregating peptides bearing different aggregation propensities with the aim of producing modes of uptake that are sufficiently distinct to differentially analyze the cellular response to internalization. We found that small acidic aggregates (≤500 nm in diameter) were taken up by nonspecific endocytosis as part of the fluid phase and traveled through the endosomal compartment to lysosomes. By contrast, bigger basic aggregates (>1 μm) were taken up through a mechanism dependent on cytoskeletal reorganization and membrane remodeling with the morphological hallmarks of phagocytosis. Importantly, the properties of these aggregates determined not only the mechanism of internalization but also the involvement of the proteostatic machinery (the assembly of interconnected networks that control the biogenesis, folding, trafficking, and degradation of proteins) in the process; whereas the internalization of small acidic aggregates is HSF1-independent, the uptake of larger basic aggregates was HSF1-dependent, requiring Hsp70. Our results show that the biophysical properties of aggregates determine both their mechanism of internalization and proteostatic response. It remains to be seen whether these differences in cellular response contribute to the particular role of specific aggregated proteins in disease., (© 2015 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published
2015
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30. A genome-wide sequence-structure analysis suggests aggregation gatekeepers constitute an evolutionary constrained functional class.

Author

De Baets G, Van Durme J, Rousseau F, and Schymkowitz J

Subjects
Conserved Sequence, Escherichia coli genetics, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Protein Binding, Protein Conformation, Thermodynamics, Escherichia coli chemistry, Escherichia coli Proteins chemistry, Protein Denaturation, Protein Multimerization, Protein Stability
Abstract

Protein aggregation is geared by aggregation-prone regions that self-associate by β-strand interactions. Charged residues and prolines are enriched at the flanks of aggregation-prone regions resulting in decreased aggregation. It is still unclear what drives the overrepresentation of these "aggregation gatekeepers", that is, whether their presence results from structural constraints determining protein stability or whether they constitute a bona fide functional class selectively maintained to control protein aggregation. As functional residues are typically conserved regardless of their cost to protein stability, we compared sequence conservation and thermodynamic cost of these residues in 2659 protein families in Escherichia coli. Across protein families, we find gatekeepers to be under strong selective conservation while at the same time representing a significant thermodynamic cost to protein structure. This finding supports the notion that aggregation gatekeepers are not structurally determined but evolutionary selected to control protein aggregation., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published
2014
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31. Horizontal gene transfer from human host to HIV-1 reverse transcriptase confers drug resistance and partly compensates for replication deficits.

Author

Megens S, Vaira D, De Baets G, Dekeersmaeker N, Schrooten Y, Li G, Schymkowitz J, Rousseau F, Vandamme AM, Moutschen M, and Van Laethem K

Subjects
Chromosomes, Human, HIV Infections virology, HIV-1 drug effects, HIV-1 isolation & purification, HIV-1 physiology, Humans, Models, Molecular, Molecular Sequence Data, Mutagenesis, Insertional, Phylogeny, Protein Conformation, RNA, Viral genetics, Sequence Analysis, DNA, Sequence Homology, Drug Resistance, Viral, Gene Transfer, Horizontal, HIV Reverse Transcriptase genetics, HIV-1 enzymology, HIV-1 genetics, Virus Replication
Abstract

We investigated the origin and the effect of insertion D67D-THGERDLGPA within HIV-1 RT from a patient failing antiviral therapy. The insertion developed within the context of pre-existing NRTI and NNRTI mutations (M41L, L210W, T215Y and N348I). Concurrently, the NRTI mutations T69I and V118I and the NNRTI mutations K103N and Y181C were detected for the first time. High-level drug resistance (fold-changes≥50) and a good replication capacity (87% of wild-type) were observed, significantly higher than for the previous virus without insertion. The insertion was very similar to a region within human chromosome 17 (31/34 nucleotide identity), and had already been detected independently in a Japanese HIV-1 isolate. These results suggest that a particular sequence within human chromosome 17 is prone to horizontal gene transfer into the HIV-1 RT finger subdomain. This insertion confers selective advantage to HIV-1 by its contribution to multi-drug resistance and restoration of impaired replication capacity., (Copyright © 2014 Elsevier Inc. All rights reserved.)

Published
2014
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32. Predicting aggregation-prone sequences in proteins.

Author

De Baets G, Schymkowitz J, and Rousseau F

Subjects
Amino Acid Sequence, Animals, Humans, Molecular Sequence Data, Protein Aggregation, Pathological metabolism, Protein Conformation, Protein Folding, Sequence Analysis, Protein, Amyloid chemistry, Computer Simulation, Models, Molecular
Abstract

Owing to its association with a diverse range of human diseases, the determinants of protein aggregation are studied intensively. It is generally accepted that the effective aggregation tendency of a protein depends on many factors such as folding efficiency towards the native state, thermodynamic stability of that conformation, intrinsic aggregation propensity of the polypeptide sequence and its ability to be recognized by the protein quality control system. The intrinsic aggregation propensity of a polypeptide sequence is related to the presence of short APRs (aggregation-prone regions) that self-associate to form intermolecular β-structured assemblies. These are typically short sequence segments (5-15 amino acids) that display high hydrophobicity, low net charge and a high tendency to form β-structures. As the presence of such APRs is a prerequisite for aggregation, a plethora of methods have been developed to identify APRs in amino acid sequences. In the present chapter, the methodological basis of these approaches is discussed, as well as some practical applications.

Published
2014
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33. A comparative analysis of the aggregation behavior of amyloid-β peptide variants.

Author

Vandersteen A, Hubin E, Sarroukh R, De Baets G, Schymkowitz J, Rousseau F, Subramaniam V, Raussens V, Wenschuh H, Wildemann D, and Broersen K

Subjects
Amyloid beta-Peptides ultrastructure, Biotinylation, Microscopy, Electron, Transmission, Spectroscopy, Fourier Transform Infrared, Amyloid beta-Peptides chemistry
Abstract

Aggregated forms of the amyloid-β peptide are hypothesized to act as the prime toxic agents in Alzheimer disease (AD). The in vivo amyloid-β peptide pool consists of both C- and N-terminally truncated or mutated peptides, and the composition thereof significantly determines AD risk. Other variations, such as biotinylation, are introduced as molecular tools to aid the understanding of disease mechanisms. Since these modifications have the potential to alter key aggregation properties of the amyloid-β peptide, we present a comparative study of the aggregation of a substantial set of the most common in vivo identified and in vitro produced amyloid-β peptides., (Copyright © 2012 Federation of European Biochemical Societies. Published by Elsevier B.V. All rights reserved.)

Published
2012
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34. Molecular plasticity regulates oligomerization and cytotoxicity of the multipeptide-length amyloid-β peptide pool.

Author

Vandersteen A, Masman MF, De Baets G, Jonckheere W, van der Werf K, Marrink SJ, Rozenski J, Benilova I, De Strooper B, Subramaniam V, Schymkowitz J, Rousseau F, and Broersen K

Subjects
Alzheimer Disease metabolism, Amino Acid Motifs, Amyloid pharmacology, Amyloid ultrastructure, Amyloid beta-Peptides pharmacology, Amyloid beta-Peptides physiology, Benzothiazoles, Cell Line, Cell Survival drug effects, Fluorescent Dyes chemistry, Humans, Kinetics, Microscopy, Atomic Force, Peptide Fragments pharmacology, Peptide Fragments physiology, Protein Structure, Quaternary, Thiazoles chemistry, Amyloid physiology, Amyloid beta-Peptides chemistry, Peptide Fragments chemistry, Protein Multimerization
Abstract

Current therapeutic approaches under development for Alzheimer disease, including γ-secretase modulating therapy, aim at increasing the production of Aβ(1-38) and Aβ(1-40) at the cost of longer Aβ peptides. Here, we consider the aggregation of Aβ(1-38) and Aβ(1-43) in addition to Aβ(1-40) and Aβ(1-42), in particular their behavior in mixtures representing the complex in vivo Aβ pool. We demonstrate that Aβ(1-38) and Aβ(1-43) aggregate similar to Aβ(1-40) and Aβ(1-42), respectively, but display a variation in the kinetics of assembly and toxicity due to differences in short timescale conformational plasticity. In biologically relevant mixtures of Aβ, Aβ(1-38) and Aβ(1-43) significantly affect the behaviors of Aβ(1-40) and Aβ(1-42). The short timescale conformational flexibility of Aβ(1-38) is suggested to be responsible for enhancing toxicity of Aβ(1-40) while exerting a cyto-protective effect on Aβ(1-42). Our results indicate that the complex in vivo Aβ peptide array and variations thereof is critical in Alzheimer disease, which can influence the selection of current and new therapeutic strategies.

Published
2012
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35. α-Galactosidase aggregation is a determinant of pharmacological chaperone efficacy on Fabry disease mutants.

Author

Siekierska A, De Baets G, Reumers J, Gallardo R, Rudyak S, Broersen K, Couceiro J, Van Durme J, Schymkowitz J, and Rousseau F

Subjects
1-Deoxynojirimycin pharmacology, Enzyme Activation drug effects, Fabry Disease drug therapy, Fabry Disease genetics, Fibroblasts metabolism, Fibroblasts pathology, Gene Expression Regulation genetics, HeLa Cells, Humans, Molecular Chaperones genetics, alpha-Galactosidase genetics, 1-Deoxynojirimycin analogs & derivatives, Fabry Disease metabolism, Gene Expression Regulation drug effects, Molecular Chaperones biosynthesis, Mutation, Missense, alpha-Galactosidase metabolism
Abstract

Fabry disease is a lysosomal storage disorder caused by loss of α-galactosidase function. More than 500 Fabry disease mutants have been identified, the majority of which are structurally destabilized. A therapeutic strategy under development for lysosomal storage diseases consists of using pharmacological chaperones to stabilize the structure of the mutant protein, thereby promoting lysosomal delivery over retrograde degradation. The substrate analog 1-deoxygalactonojirimycin (DGJ) has been shown to restore activity of mutant α-galactosidase and is currently in clinical trial for treatment of Fabry disease. However, only ∼65% of tested mutants respond to treatment in cultured patient fibroblasts, and the structural underpinnings of DGJ response remain poorly explained. Using computational modeling and cell culture experiments, we show that the DGJ response is negatively affected by protein aggregation of α-galactosidase mutants, revealing a qualitative difference between misfolding-associated and aggregation-associated loss of function. A scoring function combining predicted thermodynamic stability and intrinsic aggregation propensity of mutants captures well their aggregation behavior under overexpression in HeLa cells. Interestingly, the same classifier performs well on DGJ response data of patient-derived cultured lymphoblasts, showing that protein aggregation is an important determinant of chemical chaperone efficiency under endogenous expression levels as well. Our observations reinforce the idea that treatment of aggregation-associated loss of function observed for the more severe α-galactosidase mutants could be enhanced by combining pharmacological chaperone treatment with the suppression of mutant aggregation, e.g. via proteostatic regulator compounds that increase cellular chaperone expression.

Published
2012
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36. SNPeffect 4.0: on-line prediction of molecular and structural effects of protein-coding variants.

Author

De Baets G, Van Durme J, Reumers J, Maurer-Stroh S, Vanhee P, Dopazo J, Schymkowitz J, and Rousseau F

Subjects
Humans, Internet, Meta-Analysis as Topic, Phenotype, Databases, Protein, Polymorphism, Single Nucleotide, Protein Conformation, Proteins genetics
Abstract

Single nucleotide variants (SNVs) are, together with copy number variation, the primary source of variation in the human genome and are associated with phenotypic variation such as altered response to drug treatment and susceptibility to disease. Linking structural effects of non-synonymous SNVs to functional outcomes is a major issue in structural bioinformatics. The SNPeffect database (http://snpeffect.switchlab.org) uses sequence- and structure-based bioinformatics tools to predict the effect of protein-coding SNVs on the structural phenotype of proteins. It integrates aggregation prediction (TANGO), amyloid prediction (WALTZ), chaperone-binding prediction (LIMBO) and protein stability analysis (FoldX) for structural phenotyping. Additionally, SNPeffect holds information on affected catalytic sites and a number of post-translational modifications. The database contains all known human protein variants from UniProt, but users can now also submit custom protein variants for a SNPeffect analysis, including automated structure modeling. The new meta-analysis application allows plotting correlations between phenotypic features for a user-selected set of variants.

Published
2012
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37. An evolutionary trade-off between protein turnover rate and protein aggregation favors a higher aggregation propensity in fast degrading proteins.

Author

De Baets G, Reumers J, Delgado Blanco J, Dopazo J, Schymkowitz J, and Rousseau F

Subjects
Databases, Protein, Disease Susceptibility, Evolution, Molecular, Gene Expression Profiling, Humans, Membrane Proteins, Protein Array Analysis, Protein Stability, Proteins genetics, Statistics, Nonparametric, Thermodynamics, Time Factors, Computational Biology methods, Proteins chemistry, Proteins metabolism
Abstract

We previously showed the existence of selective pressure against protein aggregation by the enrichment of aggregation-opposing 'gatekeeper' residues at strategic places along the sequence of proteins. Here we analyzed the relationship between protein lifetime and protein aggregation by combining experimentally determined turnover rates, expression data, structural data and chaperone interaction data on a set of more than 500 proteins. We find that selective pressure on protein sequences against aggregation is not homogeneous but that short-living proteins on average have a higher aggregation propensity and fewer chaperone interactions than long-living proteins. We also find that short-living proteins are more often associated to deposition diseases. These findings suggest that the efficient degradation of high-turnover proteins is sufficient to preclude aggregation, but also that factors that inhibit proteasomal activity, such as physiological ageing, will primarily affect the aggregation of short-living proteins.

Published
2011
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