Your search keyword '"Paul De Koninck"' showing total 10 results

1. New Phosphospecific Antibody Reveals Isoform-Specific Phosphorylation of CPEB3 Protein.

Author

Lech Kaczmarczyk, Étienne Labrie-Dion, Kapil Sehgal, Marc Sylvester, Magdalena Skubal, Michele Josten, Christian Steinhäuser, Paul De Koninck, and Martin Theis

Subjects

Medicine, Science

Abstract

Cytoplasmic Polyadenylation Element Binding proteins (CPEBs) are a family of polyadenylation factors interacting with 3'UTRs of mRNA and thereby regulating gene expression. Various functions of CPEBs in development, synaptic plasticity, and cellular senescence have been reported. Four CPEB family members of partially overlapping functions have been described to date, each containing a distinct alternatively spliced region. This region is highly conserved between CPEBs-2-4 and contains a putative phosphorylation consensus, overlapping with the exon seven of CPEB3. We previously found CPEBs-2-4 splice isoforms containing exon seven to be predominantly present in neurons, and the isoform expression pattern to be cell type-specific. Here, focusing on the alternatively spliced region of CPEB3, we determined that putative neuronal isoforms of CPEB3 are phosphorylated. Using a new phosphospecific antibody directed to the phosphorylation consensus we found Protein Kinase A and Calcium/Calmodulin-dependent Protein Kinase II to robustly phosphorylate CPEB3 in vitro and in primary hippocampal neurons. Interestingly, status epilepticus induced by systemic kainate injection in mice led to specific upregulation of the CPEB3 isoforms containing exon seven. Extensive analysis of CPEB3 phosphorylation in vitro revealed two other phosphorylation sites. In addition, we found plethora of potential kinases that might be targeting the alternatively spliced kinase consensus site of CPEB3. As this site is highly conserved between the CPEB family members, we suggest the existence of a splicing-based regulatory mechanism of CPEB function, and describe a robust phosphospecific antibody to study it in future.

Published

2016

2. FRET-FLIM investigation of PSD95-NMDA receptor interaction in dendritic spines; control by calpain, CaMKII and Src family kinase.

Author

Kim Doré, Simon Labrecque, Christian Tardif, and Paul De Koninck

Subjects

Medicine, Science

Abstract

Little is known about the changes in protein interactions inside synapses during synaptic remodeling, as their live monitoring in spines has been limited. We used a FRET-FLIM approach in developing cultured rat hippocampal neurons expressing fluorescently tagged NMDA receptor (NMDAR) and PSD95, two essential proteins in synaptic plasticity, to examine the regulation of their interaction. NMDAR stimulation caused a transient decrease in FRET between the NMDAR and PSD95 in spines of young and mature neurons. The activity of both CaMKII and calpain were essential for this effect in both developmental stages. Meanwhile, inhibition of Src family kinase (SFK) had opposing impacts on this decrease in FRET in young versus mature neurons. Our data suggest concerted roles for CaMKII, SFK and calpain activity in regulating activity-dependent separation of PSD95 from GluN2A or GluN2B. Finally, we found that calpain inhibition reduced spine growth that was caused by NMDAR activity, supporting the hypothesis that PSD95-NMDAR separation is implicated in synaptic remodeling.

Published

2014

3. Fragile X mental retardation protein interacts with the RNA-binding protein Caprin1 in neuronal RiboNucleoProtein complexes [corrected].

Author

Rachid El Fatimy, Sandra Tremblay, Alain Y Dury, Samuel Solomon, Paul De Koninck, John W Schrader, and Edouard W Khandjian

Subjects

Medicine, Science

Abstract

Fragile X syndrome is caused by the absence of the Fragile X Mental Retardation Protein (FMRP), an RNA-binding protein. FMRP is associated with messenger RiboNucleoParticles (mRNPs) present in polyribosomes and its absence in neurons leads to alteration in synaptic plasticity as a result of translation regulation defects. The molecular mechanisms by which FMRP plays a role in translation regulation remain elusive. Using immunoprecipitation approaches with monoclonal Ab7G1-1 and a new generation of chicken antibodies, we identified Caprin1 as a novel FMRP-cellular partner. In vivo and in vitro evidence show that Caprin1 interacts with FMRP at the level of the translation machinery as well as in trafficking neuronal granules. As an RNA-binding protein, Caprin1 has in common with FMRP at least two RNA targets that have been identified as CaMKIIα and Map1b mRNAs. In view of the new concept that FMRP species bind to RNA regardless of known structural motifs, we propose that protein interactors might modulate FMRP functions.

Published

2012

4. Correction: Fragile Mental Retardation Protein Interacts with the RNA-Binding Protein Caprin1 in Neuronal RiboNucleoProtein Complexes.

Author

Rachid El Fatimy, Sandra Tremblay, Alain Y. Dury, Samuel Solomon, Paul De Koninck, John W. Schrader, and Edouard W. Khandjian

Subjects

Medicine, Science

Published

2012

5. Activity-dependent subcellular cotrafficking of the small GTPase Rem2 and Ca2+/CaM-dependent protein kinase IIα.

Author

Robyn Flynn, Etienne Labrie-Dion, Nikolas Bernier, Michael A Colicos, Paul De Koninck, and Gerald W Zamponi

Subjects

Medicine, Science

Abstract

Rem2 is a small monomeric GTP-binding protein of the RGK family, whose known functions are modulation of calcium channel currents and alterations of cytoskeletal architecture. Rem2 is the only RGK protein found predominantly in the brain, where it has been linked to synaptic development. We wished to determine the effect of neuronal activity on the subcellular distribution of Rem2 and its interacting partners.We show that Rem2 undergoes activity-and N-Methyl-D-Aspartate Receptor (NMDAR)-dependent translocation in rat hippocampal neurons. This redistribution of Rem2, from a diffuse pattern to one that is highly punctate, is dependent on Ca(2+) influx, on binding to calmodulin (CaM), and also involves an auto-inhibitory domain within the Rem2 distal C-terminus region. We found that Rem2 can bind to Ca(2+)/CaM-dependent protein kinase IIα (CaMKII) a in Ca(2+)/CaM-dependent manner. Furthermore, our data reveal a spatial and temporal correlation between NMDAR-dependent clustering of Rem2 and CaMKII in neurons, indicating co-assembly and co-trafficking in neurons. Finally, we show that inhibiting CaMKII aggregation in neurons and HEK cells reduces Rem2 clustering, and that Rem2 affects the baseline distribution of CaMKII in HEK cells.Our data suggest a novel function for Rem2 in co-trafficking with CaMKII, and thus potentially expose a role in neuronal plasticity.

Published

2012

6. Adaptive movement compensation for in vivo imaging of fast cellular dynamics within a moving tissue.

Author

Sophie Laffray, Stéphane Pagès, Hugues Dufour, Paul De Koninck, Yves De Koninck, and Daniel Côté

Subjects

Medicine, Science

Abstract

In vivo non-linear optical microscopy has been essential to advance our knowledge of how intact biological systems work. It has been particularly enabling to decipher fast spatiotemporal cellular dynamics in neural networks. The power of the technique stems from its optical sectioning capability that in turn also limits its application to essentially immobile tissue. Only tissue not affected by movement or in which movement can be physically constrained can be imaged fast enough to conduct functional studies at high temporal resolution. Here, we show dynamic two-photon Ca(2+) imaging in the spinal cord of a living rat at millisecond time scale, free of motion artifacts using an optical stabilization system. We describe a fast, non-contact adaptive movement compensation approach, applicable to rough and weakly reflective surfaces, allowing real-time functional imaging from intrinsically moving tissue in live animals. The strategy involves enslaving the position of the microscope objective to that of the tissue surface in real-time through optical monitoring and a closed feedback loop. The performance of the system allows for efficient image locking even in conditions of random or irregular movements.

Published

2011

7. New Phosphospecific Antibody Reveals Isoform-Specific Phosphorylation of CPEB3 Protein

Author

Michele Josten, Kapil Sehgal, Marc Sylvester, Étienne Labrie-Dion, Magdalena Skubal, Paul De Koninck, Martin Theis, Lech Kaczmarczyk, and Christian Steinhäuser

Subjects

0301 basic medicine, Consensus site, Physiology, Cytoplasmic polyadenylation element, lcsh:Medicine, metabolism [Hippocampus], RNA-binding protein, Biochemistry, Hippocampus, Mice, 0302 clinical medicine, Animal Cells, Immune Physiology, Medicine and Health Sciences, Serine, Protein Isoforms, Post-Translational Modification, Phosphorylation, Amino Acids, lcsh:Science, Neurons, Multidisciplinary, Immune System Proteins, Organic Compounds, RNA-Binding Proteins, Precipitation Techniques, Enzymes, metabolism [Antibodies, Phospho-Specific], Nucleic acids, Chemistry, metabolism [Neurons], CPEB3 protein, human, Physical Sciences, Cellular Types, Research Article, Gene isoform, Immunology, Biology, metabolism [RNA-Binding Proteins], Research and Analysis Methods, CPEB, Antibodies, 03 medical and health sciences, Hydroxyl Amino Acids, Genetics, Immunoprecipitation, Animals, Humans, ddc:610, Protein kinase A, metabolism [Protein Isoforms], Alternative splicing, lcsh:R, Organic Chemistry, Chemical Compounds, metabolism [Calcium-Calmodulin-Dependent Protein Kinase Type 2], Biology and Life Sciences, Proteins, Cell Biology, Molecular biology, Mice, Inbred C57BL, Alternative Splicing, 030104 developmental biology, HEK293 Cells, RNA processing, biology.protein, Enzymology, RNA, lcsh:Q, Gene expression, Peptides, Calcium-Calmodulin-Dependent Protein Kinase Type 2, Protein Kinases, Antibodies, Phospho-Specific, 030217 neurology & neurosurgery

Abstract

Cytoplasmic Polyadenylation Element Binding proteins (CPEBs) are a family of polyadenylation factors interacting with 3'UTRs of mRNA and thereby regulating gene expression. Various functions of CPEBs in development, synaptic plasticity, and cellular senescence have been reported. Four CPEB family members of partially overlapping functions have been described to date, each containing a distinct alternatively spliced region. This region is highly conserved between CPEBs-2-4 and contains a putative phosphorylation consensus, overlapping with the exon seven of CPEB3. We previously found CPEBs-2-4 splice isoforms containing exon seven to be predominantly present in neurons, and the isoform expression pattern to be cell type-specific. Here, focusing on the alternatively spliced region of CPEB3, we determined that putative neuronal isoforms of CPEB3 are phosphorylated. Using a new phosphospecific antibody directed to the phosphorylation consensus we found Protein Kinase A and Calcium/Calmodulin-dependent Protein Kinase II to robustly phosphorylate CPEB3 in vitro and in primary hippocampal neurons. Interestingly, status epilepticus induced by systemic kainate injection in mice led to specific upregulation of the CPEB3 isoforms containing exon seven. Extensive analysis of CPEB3 phosphorylation in vitro revealed two other phosphorylation sites. In addition, we found plethora of potential kinases that might be targeting the alternatively spliced kinase consensus site of CPEB3. As this site is highly conserved between the CPEB family members, we suggest the existence of a splicing-based regulatory mechanism of CPEB function, and describe a robust phosphospecific antibody to study it in future.

Published

2016

8. Fragile Mental Retardation Protein Interacts with the RNA-Binding Protein Caprin1 in Neuronal RiboNucleoProtein Complexes

Author

Rachid El Fatimy, John W. Schrader, Sandra Tremblay, Alain Y. Dury, Samuel G. Solomon, Edouard W. Khandjian, and Paul De Koninck

Subjects

Fragile x, Multidisciplinary, Chemistry, Science, lcsh:R, lcsh:Medicine, Correction, RNA-binding protein, Bioinformatics, Cell biology, Medicine, lcsh:Q, lcsh:Science, Ribonucleoprotein

Abstract

There was a typographical error in the title and citation. The correct title is, "Fragile X Mental Retardation Protein Interacts with the RNA-Binding Protein Caprin1 in Neuronal RiboNucleoProtein Complexes" and the correct citation is: El Fatimy R, Tremblay S, Dury AY, Solomon S, De Koninck P, et al. (2012) Fragile X Mental Retardation Protein Interacts with the RNA-Binding Protein Caprin1 in Neuronal RiboNucleoProtein Complexes. PLoS ONE 7(6): e39338. doi:10.1371/journal.pone.0039338

Published

2012

9. Fragile X mental retardation protein interacts with the RNA-binding protein Caprin1 in neuronal RiboNucleoProtein complexes [corrected]

Author

Sandra Tremblay, John W. Schrader, Edouard W. Khandjian, Samuel Solomon, Paul De Koninck, Rachid El Fatimy, and Alain Y. Dury

Subjects

Proteomics, Amino Acid Motifs, lcsh:Medicine, RNA-binding protein, Cell Cycle Proteins, Biochemistry, Fragile X Mental Retardation Protein, Mice, 0302 clinical medicine, Translational regulation, Protein biosynthesis, lcsh:Science, Ribonucleoprotein, Genetics, Mice, Knockout, Neurons, 0303 health sciences, Multidisciplinary, Physics, Antibodies, Monoclonal, Brain, RNA-Binding Proteins, Translation (biology), Cell biology, Nucleic acids, Ribonucleoproteins, Microtubule-Associated Proteins, Protein Binding, Research Article, congenital, hereditary, and neonatal diseases and abnormalities, Immunoprecipitation, Molecular Sequence Data, Biophysics, Biology, Protein Chemistry, 03 medical and health sciences, Animals, Humans, Protein Interactions, 030304 developmental biology, DNA Primers, Messenger RNA, Base Sequence, lcsh:R, RNA, Proteins, nervous system diseases, Mice, Inbred C57BL, Polyribosomes, Protein Biosynthesis, NIH 3T3 Cells, lcsh:Q, Calcium-Calmodulin-Dependent Protein Kinase Type 2, RNA transport, 030217 neurology & neurosurgery, HeLa Cells

Abstract

Fragile X syndrome is caused by the absence of the Fragile X Mental Retardation Protein (FMRP), an RNA-binding protein. FMRP is associated with messenger RiboNucleoParticles (mRNPs) present in polyribosomes and its absence in neurons leads to alteration in synaptic plasticity as a result of translation regulation defects. The molecular mechanisms by which FMRP plays a role in translation regulation remain elusive. Using immunoprecipitation approaches with monoclonal Ab7G1-1 and a new generation of chicken antibodies, we identified Caprin1 as a novel FMRP-cellular partner. In vivo and in vitro evidence show that Caprin1 interacts with FMRP at the level of the translation machinery as well as in trafficking neuronal granules. As an RNA-binding protein, Caprin1 has in common with FMRP at least two RNA targets that have been identified as CaMKIIα and Map1b mRNAs. In view of the new concept that FMRP species bind to RNA regardless of known structural motifs, we propose that protein interactors might modulate FMRP functions.

Published

2011

10. Adaptive movement compensation for in vivo imaging of fast cellular dynamics within a moving tissue

Author

Daniel Côté, Stéphane Pagès, Hugues Dufour, Yves De Koninck, Paul De Koninck, and Sophie Laffray

Subjects

Diagnostic Imaging, Male, Microscope, Optical sectioning, Neural Networks, Biomedical Engineering, lcsh:Medicine, Bioengineering, Neuroimaging, Bioinformatics, Signaling Pathways, law.invention, Compensation (engineering), 03 medical and health sciences, 0302 clinical medicine, Engineering, law, Medical imaging, Animals, Rats, Wistar, lcsh:Science, Biology, 030304 developmental biology, Physics, 0303 health sciences, Millisecond, Multidisciplinary, Artificial neural network, lcsh:R, Feedback loop, Calcium Imaging, Rats, Spinal Cord, lcsh:Q, Calcium, Molecular Neuroscience, Biological system, 030217 neurology & neurosurgery, Preclinical imaging, Research Article, Biotechnology, Neuroscience

Abstract

In vivo non-linear optical microscopy has been essential to advance our knowledge of how intact biological systems work. It has been particularly enabling to decipher fast spatiotemporal cellular dynamics in neural networks. The power of the technique stems from its optical sectioning capability that in turn also limits its application to essentially immobile tissue. Only tissue not affected by movement or in which movement can be physically constrained can be imaged fast enough to conduct functional studies at high temporal resolution. Here, we show dynamic two-photon Ca(2+) imaging in the spinal cord of a living rat at millisecond time scale, free of motion artifacts using an optical stabilization system. We describe a fast, non-contact adaptive movement compensation approach, applicable to rough and weakly reflective surfaces, allowing real-time functional imaging from intrinsically moving tissue in live animals. The strategy involves enslaving the position of the microscope objective to that of the tissue surface in real-time through optical monitoring and a closed feedback loop. The performance of the system allows for efficient image locking even in conditions of random or irregular movements.

Published

2010