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2. RETRACTED ARTICLE: Secretome of endothelial progenitor cells from stroke patients promotes endothelial barrier tightness and protects against hypoxia-induced vascular leakage

Author

Loiola, Rodrigo Azevedo, García-Gabilondo, Miguel, Grayston, Alba, Bugno, Paulina, Kowalska, Agnieszka, Duban-Deweer, Sophie, Rizzi, Eleonora, Hachani, Johan, Sano, Yasuteru, Shimizu, Fumitaka, Kanda, Takashi, Mysiorek, Caroline, Mazurek, Maciej Piotr, Rosell, Anna, and Gosselet, Fabien

Published
2021
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4. Gel electrophoresis of human sperm: a simple method for evaluating sperm protein quality

Author

Jumeau Fanny, Sigala Julien, Fernandez-Gomez Francisco-Jose, Eddarkaoui Sabiha, Duban-Deweer Sophie, Buée Luc, Béhal Hélène, Sergeant Nicolas, and Mitchell Valérie

Subjects
Fibrous sheath, One-dimensional PAGE, Sperm, Medicine (General), R5-920
Abstract

Résumé Contexte Les limites des analyses conventionnelles du sperme ont mis en évidence la nécessité de moyens supplémentaires d’évaluation de la qualité du sperme. Matériel et Méthodes La méthode d’électrophorèse unidimensionnelle a été utilisée pour évaluer la teneur et la qualité protéique dans des échantillons d’éjaculats individuels de 245 hommes avec des paramètres spermatiques connus. Résultats La teneur en protéines du sperme variait d’un échantillon à l’autre, en particulier dans la gamme des poids moléculaires élevés. L’intensité des bandes de 80–110 kDa était corrélée à la mobilité progressive (r = 0,15, p = 0,015) et était significativement plus élevée (p = 0,0367) dans le groupe des hommes avec des paramètres conventionnels spermatiques supérieurs aux valeurs de référence (OMS, 2010) comparé au groupe d’hommes dont l’éjaculat présentait au moins un paramètre spermatique (volume de sperme, concentration de spermatozoïdes, numération des spermatozoïdes, motilité progressive, formes normales et indice d’anomalies multiples) en deça de la valeur de référence. Les bandes dans la gamme de 80–110 kDa ont été identifiées en spectrométrie de masse et se sont révélées être des protéines de la gaine fibreuse du flagelle: la protéine d’ancrage A-kinase 4, la protéine d’ancrage A-kinase 3 et l’hexokinase de type 1. Conclusion La méthode d’électrophorèse unidimensionnelle constitue une méthode simple, rapide, fiable et peu coûteuse pour analyser la qualité des protéines du sperme dans les éjaculats humains individuels.

Published
2018
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6. Highlighting In Vitro the Role of Brain-like Endothelial Cells on the Maturation and Metabolism of Brain Pericytes by SWATH Proteomics.

Author

Menaceur, Camille, Hachani, Johan, Dib, Shiraz, Duban-Deweer, Sophie, Karamanos, Yannis, Shimizu, Fumitaka, Kanda, Takashi, Gosselet, Fabien, Fenart, Laurence, and Saint-Pol, Julien

Subjects
BLOOD-brain barrier, ENDOTHELIAL cells, CELL metabolism, BRAIN metabolism, PROTEOMICS, PERICYTES, MASS spectrometry
Abstract

Within the neurovascular unit, brain pericytes (BPs) are of major importance for the induction and maintenance of the properties of the blood-brain barrier (BBB) carried by the brain microvessel endothelial cells (ECs). Throughout barriergenesis, ECs take advantage of soluble elements or contact with BPs to maintain BBB integrity and the regulation of their cellular homeostasis. However, very few studies have focused on the role of ECs in the maturation of BPs. The aim of this study is to shed light on the proteome of BPs solocultured (hBP-solo) or cocultured with ECs (hBP-coc) to model the human BBB in a non-contact manner. We first generated protein libraries for each condition and identified 2233 proteins in hBP-solo versus 2492 in hBP-coc and 2035 common proteins. We performed a quantification of the enriched proteins in each condition by sequential window acquisition of all theoretical mass spectra (SWATH) analysis. We found 51 proteins enriched in hBP-solo related to cell proliferation, contractility, adhesion and extracellular matrix element production, a protein pattern related to an immature cell. In contrast, 90 proteins are enriched in hBP-coc associated with a reduction in contractile activities as observed in vivo in 'mature' BPs, and a significant gain in different metabolic functions, particularly related to mitochondrial activities and sterol metabolism. This study highlights that BPs take advantage of ECs during barriergenesis to make a metabolic switch in favor of BBB homeostasis in vitro. [ABSTRACT FROM AUTHOR]

Published
2023
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8. Secretome of endothelial progenitor cells from stroke patients promotes endothelial barrier tightness and protects against hypoxia-induced vascular leakage.

Author

Loiola, Rodrigo Azevedo, García-Gabilondo, Miguel, Grayston, Alba, Bugno, Paulina, Kowalska, Agnieszka, Duban-Deweer, Sophie, Rizzi, Eleonora, Hachani, Johan, Sano, Yasuteru, Shimizu, Fumitaka, Kanda, Takashi, Mysiorek, Caroline, Mazurek, Maciej Piotr, Rosell, Anna, and Gosselet, Fabien

Subjects
PROGENITOR cells, ENDOTHELIAL cells, BLOOD-brain barrier, STROKE patients, LEAKAGE, RETRIEVAL practice, OCCLUDINS
Abstract

Background: Cell-based therapeutic strategies have been proposed as an alternative for brain repair after stroke, but their clinical application has been hampered by potential adverse effects in the long term. The present study was designed to test the effect of the secretome of endothelial progenitor cells (EPCs) from stroke patients (scCM) on in vitro human models of angiogenesis and vascular barrier. Methods: Two different scCM batches were analysed by mass spectrometry and a proteome profiler. Human primary CD34+-derived endothelial cells (CD34+-ECs) were used for designing angiogenesis studies (proliferation, migration, and tubulogenesis) or in vitro models of EC monolayer (confluent monolayer ECs—CMECs) and blood–brain barrier (BBB; brain-like ECs—BLECs). Cells were treated with scCM (5 μg/mL) or protein-free endothelial basal medium (scEBM—control). CMECs or BLECs were exposed (6 h) to oxygen–glucose deprivation (OGD) conditions (1% oxygen and glucose-free medium) or normoxia (control—5% oxygen, 1 g/L of glucose) and treated with scCM or scEBM during reoxygenation (24 h). Results: The analysis of different scCM batches showed a good reproducibility in terms of protein yield and composition. scCM increased CD34+-EC proliferation, tubulogenesis, and migration compared to the control (scEBM). The proteomic analysis of scCM revealed the presence of growth factors and molecules modulating cell metabolism and inflammatory pathways. Further, scCM decreased the permeability of CMECs and upregulated the expression of the junctional proteins such as occludin, VE-cadherin, and ZO-1. Such effects were possibly mediated through the activation of the interferon pathway and a moderate downregulation of Wnt signalling. Furthermore, OGD increased the permeability of both CMECs and BLECs, while scCM prevented the OGD-induced vascular leakage in both models. These effects were possibly mediated through the upregulation of junctional proteins and the regulation of MAPK/VEGFR2 activity. Conclusion: Our results suggest that scCM promotes angiogenesis and the maturation of newly formed vessels while restoring the BBB function in ischemic conditions. In conclusion, our results highlight the possibility of using EPC-secretome as a therapeutic alternative to promote brain angiogenesis and protect from ischemia-induced vascular leakage. [ABSTRACT FROM AUTHOR]

Published
2021
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9. A large-scale electrophoresis- and chromatography-based determination of gene expression profiles in bovine brain capillary endothelial cells after the re-induction of blood-brain barrier properties

Author

Duban-Deweer Sophie, Deracinois Barbara, Pottiez Gwënaël, Cecchelli Roméo, Fenart Laurence, Karamanos Yannis, and Flahaut Christophe

Subjects
Cytology, QH573-671
Abstract

Abstract Background Brain capillary endothelial cells (BCECs) form the physiological basis of the blood-brain barrier (BBB). The barrier function is (at least in part) due to well-known proteins such as transporters, tight junctions and metabolic barrier proteins (e.g. monoamine oxidase, gamma glutamyltranspeptidase and P-glycoprotein). Our previous 2-dimensional gel proteome analysis had identified a large number of proteins and revealed the major role of dynamic cytoskeletal remodelling in the differentiation of bovine BCECs. The aim of the present study was to elaborate a reference proteome of Triton X-100-soluble species from bovine BCECs cultured in the well-established in vitro BBB model developed in our laboratory. Results A total of 215 protein spots (corresponding to 130 distinct proteins) were identified by 2-dimensional gel electrophoresis, whereas over 350 proteins were identified by a shotgun approach. We classified around 430 distinct proteins expressed by bovine BCECs. Our large-scale gene expression analysis enabled the correction of mistakes referenced into protein databases (e.g. bovine vinculin) and constitutes valuable evidence for predictions based on genome annotation. Conclusions Elaboration of a reference proteome constitutes the first step in creating a gene expression database dedicated to capillary endothelial cells displaying BBB characteristics. It improves of our knowledge of the BBB and the key proteins in cell structures, cytoskeleton organization, metabolism, detoxification and drug resistance. Moreover, our results emphasize the need for both appropriate experimental design and correct interpretation of proteome datasets.

Published
2010
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10. Serological proteome analysis reveals new specific biases in the IgM and IgG autoantibody repertoires in autoimmune polyendocrine syndrome type 1.

Author

Dubucquoi, Sylvain, Proust-Lemoine, Emmanuelle, Kemp, E. Helen, Ryndak, Amélie, Lefèvre-Dutoit, Virginie, Bellart, Marine, Saugier-Véber, Pascale, Duban-Deweer, Sophie, Wémeau, Jean-Louis, Prin, Lionel, and Lefranc, Didier

Subjects
IMMUNOGLOBULIN G, IMMUNOGLOBULIN M, GENETICS of autoimmune diseases, AUTOIMMUNE polyendocrinopathies, AUTOANTIBODIES, GENETIC mutation, SERODIAGNOSIS
Abstract

Objective: Autoimmune polyendocrine syndrome type 1 (APS 1) is caused by mutations in theAIREgene that induce intrathymic T-cell tolerance breakdown, which results in tissue-specific autoimmune diseases.Design: To evaluate the effect of a well-defined T-cell repertoire impairment on humoral self-reactive fingerprints, comparative serum self-IgG and self-IgM reactivities were analyzed using both one- and two-dimensional western blotting approaches against a broad spectrum of peripheral tissue antigens.Methods: Autoantibody patterns of APS 1 patients were compared with those of subjects affected by other autoimmune endocrinopathies (OAE) and healthy controls.Results: Using a Chi-square test, significant changes in the Ab repertoire were found when intergroup patterns were compared. A singular distortion of both serum self-IgG and self-IgM repertoires was noted in APS 1 patients. The molecular characterization of these antigenic targets was conducted using a proteomic approach. In this context, autoantibodies recognized more significantly either tissue-specific antigens, such as pancreatic amylase, pancreatic triacylglycerol lipase and pancreatic regenerating protein 1α, or widely distributed antigens, such as peroxiredoxin-2, heat shock cognate 71-kDa protein and aldose reductase. As expected, a well-defined self-reactive T-cell repertoire impairment, as described in APS 1 patients, affected the tissue-specific self-IgG repertoire. Interestingly, discriminant IgM reactivities targeting both tissue-specific and more widely expressed antigens were also specifically observed in APS 1 patients. Using recombinant targets, we observed that post translational modifications of these specific antigens impacted upon their recognition.Conclusions: The data suggest that T-cell-dependent but also T-cell-independent mechanisms are involved in the dynamic evolution of autoimmunity in APS 1. [ABSTRACT FROM PUBLISHER]

Published
2015
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11. An Optimized Fluorescence-Based Bidimensional Immunoproteomic Approach for Accurate Screening of Autoantibodies.

Author

Dutoit-Lefèvre, Virginie, Dubucquoi, Sylvain, Launay, David, Sobanski, Vincent, Dussart, Patricia, Chafey, Philippe, Broussard, Cédric, Duban-Deweer, Sophie, Vermersch, Patrick, Prin, Lionel, and Lefranc, Didier

Subjects
FLUORESCENCE, PROTEOMICS, AUTOANTIBODIES, MEDICAL screening, SEROLOGY, TWO-dimensional models
Abstract

Serological proteome analysis (SERPA) combines classical proteomic technology with effective separation of cellular protein extracts on two-dimensional gel electrophoresis, western blotting, and identification of the antigenic spot of interest by mass spectrometry. A critical point is related to the antigenic target characterization by mass spectrometry, which depends on the accuracy of the matching of antigenic reactivities on the protein spots during the 2D immunoproteomic procedures. The superimposition, based essentially on visual criteria of antigenic and protein spots, remains the major limitation of SERPA. The introduction of fluorescent dyes in proteomic strategies, commonly known as 2D-DIGE (differential in-gel electrophoresis), has boosted the qualitative capabilities of 2D electrophoresis. Based on this 2D-DIGE strategy, we have improved the conventional SERPA by developing a new and entirely fluorescence-based bi-dimensional immunoproteomic (FBIP) analysis, performed with three fluorescent dyes. To optimize the alignment of the different antigenic maps, we introduced a landmark map composed of a combination of specific antibodies. This methodological development allows simultaneous revelation of the antigenic, landmark and proteomic maps on each immunoblot. A computer-assisted process using commercially available software automatically leads to the superimposition of the different maps, ensuring accurate localization of antigenic spots of interest. [ABSTRACT FROM AUTHOR]

Published
2015
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13. Maternal calorie restriction modulates placental mitochondrial biogenesis and bioenergetic efficiency: putative involvement in fetoplacental growth defects in rats.

Author

Mayeur, Sylvain, Lancel, Steve, Theys, Nicolas, Lukaszewski, Marie-Amélie, Duban-Deweer, Sophie, Bastide, Bruno, Hachani, Johan, Cecchelli, Roméo, Breton, Christophe, Gabory, Anne, Storme, Laurent, Reusens, Brigitte, Junien, Claudine, Vieau, Didier, and Lesage, Jean

Abstract

Low birth weight is associated with an increased risk for developing type 2 diabetes and metabolic diseases. The placental capacity to supply nutrients and oxygen to the fetus represents the main determiner of fetal growth. However, few studies have investigated the effects of maternal diet on the placenta. We explored placental adaptive proteomic processes implicated in response to maternal undernutrition. Rat term placentas from 70% food-restricted (FR30) mothers were used for a proteomic screen. Placental mitochondrial functions were evaluated using molecular and functional approaches, and ATP production was measured. FR30 drastically reduced placental and fetal weights. FR30 placentas displayed 14 proteins that were differentially expressed, including several mitochondrial proteins. FR30 induced a marked increase in placental mtDNA content and changes in mitochondrial functions, including modulation of the expression of genes implicated in biogenesis and bioenergetic pathways. FR30 mitochondria showed higher oxygen consumption but failed to maintain their ATP production. Maternal undernutrition induces placental mitochondrial abnormalities. Although an increase in biogenesis and bioenergetic efficiency was noted, placental ATP level was reduced. Our data suggest that placental mitochondrial defects may be implicated in fetoplacental pathologies. [ABSTRACT FROM AUTHOR]

Published
2013
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14. TNAP and EHD1 Are Over-Expressed in Bovine Brain Capillary Endothelial Cells after the Re-Induction of Blood-Brain Barrier Properties.

Author

Deracinois, Barbara, Duban-Deweer, Sophie, Pottiez, Gwënaël, Cecchelli, Roméo, Karamanos, Yannis, and Flahaut, Christophe

Subjects
*BLOOD-brain barrier, *PHENOTYPES, *ENDOTHELIAL cells, *PROTEOMICS, *CELL differentiation, *ALKALINE phosphatase
Abstract

Although the physiological properties of the blood-brain barrier (BBB) are relatively well known, the phenotype of the component brain capillary endothelial cells (BCECs) has yet to be described in detail. Likewise, the molecular mechanisms that govern the establishment and maintenance of the BBB are largely unknown. Proteomics can be used to assess quantitative changes in protein levels and identify proteins involved in the molecular pathways responsible for cellular differentiation. Using the well-established in vitro BBB model developed in our laboratory, we performed a differential nano- LC MALDI-TOF/TOF-MS study of Triton X-100-soluble protein species from bovine BCECs displaying either limited BBB functions or BBB functions re-induced by glial cells. Due to the heterogeneity of the crude extract, we increased identification yields by applying a repeatable, reproducible fractionation process based on the proteins' relative hydrophobicity. We present proteomic and biochemical evidence to show that tissue non-specific alkaline phosphatase (TNAP) and Eps15 homology domain-containing protein 1(EDH1) are over-expressed by bovine BCECs after the re-induction of BBB properties. We discuss the impact of these findings on current knowledge of endothelial and BBB permeability. [ABSTRACT FROM AUTHOR]

Published
2012
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17. A large-scale electrophoresis-- and chromatography-based determination of gene expression profiles in bovine brain capillary endothelial cells after the re-induction of blood-brain barrier properties.

Author

Pottiez, Gwënaël, Deracinois, Barbara, Duban-Deweer, Sophie, Cecchelli, Roméo, Fenart, Laurence, Karamanos, Yannis, and Flahaut, Christophe

Subjects
BLOOD-brain barrier, GENE expression, BRAIN blood-vessels, ELECTROPHORESIS, CHROMATOGRAPHIC analysis
Abstract

Background: Brain capillary endothelial cells (BCECs) form the physiological basis of the blood-brain barrier (BBB). The barrier function is (at least in part) due to well-known proteins such as transporters, tight junctions and metabolic barrier proteins (e.g. monoamine oxidase, gamma glutamyltranspeptidase and P-glycoprotein). Our previous 2-dimensional gel proteome analysis had identified a large number of proteins and revealed the major role of dynamic cytoskeletal remodelling in the differentiation of bovine BCECs. The aim of the present study was to elaborate a reference proteome of Triton X-100-soluble species from bovine BCECs cultured in the wellestablished in vitro BBB model developed in our laboratory. Results: A total of 215 protein spots (corresponding to 130 distinct proteins) were identified by 2-dimensional gel electrophoresis, whereas over 350 proteins were identified by a shotgun approach. We classified around 430 distinct proteins expressed by bovine BCECs. Our large-scale gene expression analysis enabled the correction of mistakes referenced into protein databases (e.g. bovine vinculin) and constitutes valuable evidence for predictions based on genome annotation. Conclusions: Elaboration of a reference proteome constitutes the first step in creating a gene expression database dedicated to capillary endothelial cells displaying BBB characteristics. It improves of our knowledge of the BBB and the key proteins in cell structures, cytoskeleton organization, metabolism, detoxification and drug resistance. Moreover, our results emphasize the need for both appropriate experimental design and correct interpretation of proteome datasets. [ABSTRACT FROM AUTHOR]

Published
2010
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18. Targeting and Crossing the Blood-Brain Barrier with Extracellular Vesicles.

Author

Saint-Pol, Julien, Gosselet, Fabien, Duban-Deweer, Sophie, Pottiez, Gwënaël, and Karamanos, Yannis

Subjects
EXTRACELLULAR vesicles, EXTRACELLULAR matrix, CENTRAL nervous system, BLOOD-brain barrier, PRODUCT elimination, PHYSIOLOGY, ASTROCYTES, NEURAL stem cells
Abstract

The blood–brain barrier (BBB) is one of the most complex and selective barriers in the human organism. Its role is to protect the brain and preserve the homeostasis of the central nervous system (CNS). The central elements of this physical and physiological barrier are the endothelial cells that form a monolayer of tightly joined cells covering the brain capillaries. However, as endothelial cells regulate nutrient delivery and waste product elimination, they are very sensitive to signals sent by surrounding cells and their environment. Indeed, the neuro-vascular unit (NVU) that corresponds to the assembly of extracellular matrix, pericytes, astrocytes, oligodendrocytes, microglia and neurons have the ability to influence BBB physiology. Extracellular vesicles (EVs) play a central role in terms of communication between cells. The NVU is no exception, as each cell can produce EVs that could help in the communication between cells in short or long distances. Studies have shown that EVs are able to cross the BBB from the brain to the bloodstream as well as from the blood to the CNS. Furthermore, peripheral EVs can interact with the BBB leading to changes in the barrier's properties. This review focuses on current knowledge and potential applications regarding EVs associated with the BBB. [ABSTRACT FROM AUTHOR]

Published
2020
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19. O-GlcNAcylation is a key modulator of skeletal muscle sarcomeric morphometry associated to modulation of protein–protein interactions.

Author

Lambert, Matthias, Richard, Elodie, Duban-Deweer, Sophie, Krzewinski, Frederic, Deracinois, Barbara, Dupont, Erwan, Bastide, Bruno, and Cieniewski-Bernard, Caroline

Subjects
*SKELETAL muscle, *PROTEIN-protein interactions, *SARCOMERES, *CRYSTALLINS, *GLYCOSYLATION
Abstract

Background The sarcomere structure of skeletal muscle is determined through multiple protein–protein interactions within an intricate sarcomeric cytoskeleton network. The molecular mechanisms involved in the regulation of this sarcomeric organization, essential to muscle function, remain unclear. O -GlcNAcylation, a post-translational modification modifying several key structural proteins and previously described as a modulator of the contractile activity, was never considered to date in the sarcomeric organization. Methods C2C12 skeletal myotubes were treated with Thiamet-G (OGA inhibitor) in order to increase the global O -GlcNAcylation level. Results Our data clearly showed a modulation of the O -GlcNAc level more sensitive and dynamic in the myofilament-enriched fraction than total proteome. This fine O -GlcNAc level modulation was closely related to changes of the sarcomeric morphometry. Indeed, the dark-band and M -line widths increased, while the I-band width and the sarcomere length decreased according to the myofilament O -GlcNAc level. Some structural proteins of the sarcomere such as desmin, αB-crystallin, α-actinin, moesin and filamin-C have been identified within modulated protein complexes through O -GlcNAc level variations. Their interactions seemed to be changed, especially for desmin and αB-crystallin. Conclusions For the first time, our findings clearly demonstrate that O -GlcNAcylation, through dynamic regulations of the structural interactome, could be an important modulator of the sarcomeric structure and may provide new insights in the understanding of molecular mechanisms of neuromuscular diseases characterized by a disorganization of the sarcomeric structure. General significance In the present study, we demonstrated a role of O -GlcNAcylation in the sarcomeric structure modulation. [ABSTRACT FROM AUTHOR]

Published
2016
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20. Amine coupling versus biotin capture for the assessment of sulfonamide as ligands of hCA isoforms.

Author

Rogez-Florent, Tiphaine, Goossens, Laurence, Drucbert, Anne-Sophie, Duban-Deweer, Sophie, Six, Perrine, Depreux, Patrick, Danzé, Pierre-Marie, Goossens, Jean-François, and Foulon, Catherine

Subjects
*SULFONAMIDES, *COUPLING reactions (Chemistry), *SURFACE plasmon resonance, *STREPTAVIDIN, *THERAPEUTIC immobilization
Abstract

This work was dedicated to the development of a reliable SPR method allowing the simultaneous and quick determination of the affinity and selectivity of designed sulfonamide derivatives for hCAIX and hCAXII versus hCAII, in order to provide an efficient tool to discover drugs for anticancer therapy of solid tumors. We performed for the first time a comparison of two immobilization approaches of hCA isoforms. First one relies on the use of an amine coupling strategy, using a CM7 chip to obtain higher immobilization levels than with a CM5 chip and consequently the affinity with an higher precision (CV% < 10%). The second corresponds to a capture of proteins on a streptavidin chip, named CAP chip, after optimization of biotinylation conditions (amine versus carboxyl coupling, biotin to protein ratio). Thanks to the amine coupling approach, only hCAII and hCAXII isoforms were efficiently biotinylated to reach relevant immobilization (3000 RU and 2700 RU, respectively) to perform affinity studies. For hCAIX, despite a successful biotinylation, capture on the CAP chip was a failure. Finally, concordance between affinities obtained for the three derivatives to CAs isozymes on both chips has allowed to valid the approaches for a further screening of new derivatives. [ABSTRACT FROM AUTHOR]

Published
2016
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21. Optimization of 2-DE and multiplexed detection of O-GlcNAcome, phosphoproteome and whole proteome protocol of synapse-associated proteins within the rat sensorimotor cortex.

Author

Fourneau, Julie, Cieniewski-Bernard, Caroline, Canu, Marie-Hélène, Duban-Deweer, Sophie, Hachani, Johann, Bastide, Bruno, and Dupont, Erwan

Subjects
*SENSORIMOTOR cortex, *CEREBRAL cortex, *PROTEINS, *MOIETIES (Chemistry), *CLICK chemistry
Abstract

• Optimization of separating conditions for 2D-gel electrophoresis of synapse associated proteins within the cerebral cortex. • Optimization of a multiplexed proteomic strategy to detect O-GlcNAc proteins, phosphoproteins, and the whole proteome within the same 2-D gel. • Applicable on low amounts of sample material of rat brain tissue. Several studies have shown the importance of phosphorylation, O-GlcNAcylation and their interplay in neuronal processes. To get understanding about molecular mechanisms of synaptic plasticity, we performed a preparation of synaptic protein-enriched fraction on a small sample of rat sensorimotor cortex. We then optimized a multiplexed proteomic strategy to detect O-GlcNAcylated proteins, phosphoproteins, and the whole proteome within the same bidimensional gel. We compared different protocols (solubilisation buffer, reticulation and composition of the gel, migration buffer) to optimize separating conditions for 2D-gel electrophoresis of synaptic proteins. The O-GlcNAcome was revealed using Click chemistry and the azide–alkyne cycloaddition of a fluorophore on O-GlcNAc moieties. The phosphoproteome was detected by Phospho-Tag staining, while the whole proteome was visualized through SYPRORuby staining. This method permitted, after sequential image acquisition, the direct in-gel detection of O-GlcNAcome, phosphoproteome, and whole proteome of synapse-associated proteins. This original method of differential proteomic analysis will permit to identify key markers of synaptic plasticity that are O-GlcNAcylated and/or phosphorylated, and their molecular regulations in neuronal processes. [ABSTRACT FROM AUTHOR]

Published
2020
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