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2. Selective PDE4 subtype inhibition provides new opportunities to intervene in neuroinflammatory versus myelin damaging hallmarks of multiple sclerosis.

Author

Schepers, Melissa, Paes, Dean, Tiane, Assia, Rombaut, Ben, Piccart, Elisabeth, van Veggel, Lieve, Gervois, Pascal, Wolfs, Esther, Lambrichts, Ivo, Brullo, Chiara, Bruno, Olga, Fedele, Ernesto, Ricciarelli, Roberta, Ffrench-Constant, Charles, Bechler, Marie E., van Schaik, Pauline, Baron, Wia, Lefevere, Evy, Wasner, Kobi, Grünewald, Anne, Verfaillie, Catherine, Baeten, Paulien, Broux, Bieke, Wieringa, Paul, Hellings, Niels, Prickaerts, Jos, Vanmierlo, Tim, Schepers, Melissa, Paes, Dean, Tiane, Assia, Rombaut, Ben, Piccart, Elisabeth, van Veggel, Lieve, Gervois, Pascal, Wolfs, Esther, Lambrichts, Ivo, Brullo, Chiara, Bruno, Olga, Fedele, Ernesto, Ricciarelli, Roberta, Ffrench-Constant, Charles, Bechler, Marie E., van Schaik, Pauline, Baron, Wia, Lefevere, Evy, Wasner, Kobi, Grünewald, Anne, Verfaillie, Catherine, Baeten, Paulien, Broux, Bieke, Wieringa, Paul, Hellings, Niels, Prickaerts, Jos, and Vanmierlo, Tim

Abstract

Multiple sclerosis (MS) is a chronic autoimmune disease of the central nervous system (CNS) characterized by focal inflammatory lesions and prominent demyelination. Even though the currently available therapies are effective in treating the initial stages of disease, they are unable to halt or reverse disease progression into the chronic progressive stage. Thus far, no repair-inducing treatments are available for progressive MS patients. Hence, there is an urgent need for the development of new therapeutic strategies either targeting the destructive immunological demyelination or boosting endogenous repair mechanisms. Using in vitro, ex vivo, and in vivo models, we demonstrate that selective inhibition of phosphodiesterase 4 (PDE4), a family of enzymes that hydrolyzes and inactivates cyclic adenosine monophosphate (cAMP), reduces inflammation and promotes myelin repair. More specifically, we segregated the myelination-promoting and anti-inflammatory effects into a PDE4D- and PDE4B-dependent process respectively. We show that inhibition of PDE4D boosts oligodendrocyte progenitor cells (OPC) differentiation and enhances (re)myelination of both murine OPCs and human iPSC-derived OPCs. In addition, PDE4D inhibition promotes in vivo remyelination in the cuprizone model, which is accompanied by improved spatial memory and reduced visual evoked potential latency times. We further identified that PDE4B-specific inhibition exerts anti-inflammatory effects since it lowers in vitro monocytic nitric oxide (NO) production and improves in vivo neurological scores during the early phase of experimental autoimmune encephalomyelitis (EAE). In contrast to the pan PDE4 inhibitor roflumilast, the therapeutic dose of both the PDE4B-specific inhibitor A33 and the PDE4D-specific inhibitor Gebr32a did not trigger emesis-like side effects in rodents. Finally, we report distinct PDE4D isoform expression patterns in human area postrema neurons and human oligodendroglia lineage cells. Using th

Published
2023

4. The phospholipase complex PAFAH lb regulates the functional organization of the Golgi complex

Author

Bechler, Marie E., Doody, Anne M., Racoosin, Esther, Lin, Lin, Lee, Kelvin H., and Brown, William J.

Subjects
Phospholipases -- Physiological aspects, Phospholipases -- Chemical properties, Dynein -- Chemical properties, Dynein -- Physiological aspects, Golgi apparatus -- Chemical properties, Biological sciences
Abstract

We report that platelet-activating factor acetyl-hydrolase (PAFAH) lb, comprised of two phospholipase [A.sub.2] ([PLA.sub.2]) subunits, [alpha]1 and [alpha]2, and a third subunit, the dynein regulator lissen-cephaly 1 (LIS1), mediates the structure and function of the Golgi complex. Both [alpha]1 and [alpha]2 partially localize on Golgi membranes, and purified catalytically active, but not inactive [alpha]1 and [alpha]2 induce Golgi membrane tubule formation in a reconstitution system. Overexpression of wild-type or mutant [alpha]1 or [alpha]2 revealed that both [PLA.sub.2] activity and LIS1 are important for maintaining Golgi structure. Knockdown of PAFAH Ib subunits fragments the Golgi complex, inhibits tubule-mediated reassembly of intact Golgi ribbons, and slows secretion of cargo. Our results demonstrate a cooperative interplay between the [PLA.sub.2] activity of [alpha]1 and [alpha]2 with LIS1 to facilitate the functional organization of the Golgi complex, thereby suggesting a model that links phospholipid remodeling and membrane tubulation to dyne-independent transport. doi/ 10.1083/jcb.200908105

Published
2010

6. CNS Myelin Sheath Lengths Are an Intrinsic Property of Oligodendrocytes

Author

Bechler, Marie E., Byrne, Lauren, and ffrench-Constant, Charles

Subjects
Rats, Sprague-Dawley, Agricultural and Biological Sciences(all), integumentary system, nervous system, Spinal Cord, Biochemistry, Genetics and Molecular Biology(all), Report, Animals, Axons, Myelin Sheath, Rats, Signal Transduction
Abstract

Summary Since Río-Hortega’s description of oligodendrocyte morphologies nearly a century ago, many studies have observed myelin sheath-length diversity between CNS regions [1–3]. Myelin sheath length directly impacts axonal conduction velocity by influencing the spacing between nodes of Ranvier. Such differences likely affect neural signal coordination and synchronization [4]. What accounts for regional differences in myelin sheath lengths is unknown; are myelin sheath lengths determined solely by axons or do intrinsic properties of different oligodendrocyte precursor cell populations affect length? The prevailing view is that axons provide molecular cues necessary for oligodendrocyte myelination and appropriate sheath lengths. This view is based upon the observation that axon diameters correlate with myelin sheath length [1, 5, 6], as well as reports that PNS axonal neuregulin-1 type III regulates the initiation and properties of Schwann cell myelin sheaths [7, 8]. However, in the CNS, no such instructive molecules have been shown to be required, and increasing in vitro evidence supports an oligodendrocyte-driven, neuron-independent ability to differentiate and form initial sheaths [9–12]. We test this alternative signal-independent hypothesis—that variation in internode lengths reflects regional oligodendrocyte-intrinsic properties. Using microfibers, we find that oligodendrocytes have a remarkable ability to self-regulate the formation of compact, multilamellar myelin and generate sheaths of physiological length. Our results show that oligodendrocytes respond to fiber diameters and that spinal cord oligodendrocytes generate longer sheaths than cortical oligodendrocytes on fibers, co-cultures, and explants, revealing that oligodendrocytes have regional identity and generate different sheath lengths that mirror internodes in vivo., Graphical Abstract, Highlights • Oligodendrocytes, not Schwann cells, form myelin sheaths without axonal signals • Oligodendrocytes sense diameter, increasing sheath length with larger fibers • Oligodendrocytes from cortex and spinal cord form sheaths of different lengths • Regional differences in sheath lengths may initially be hard-wired, Much of the mammalian brain comprises axons wrapped by myelin sheaths, whose length determines conduction velocity. Bechler et al. overturn the long-held view that sheath-forming oligodendrocytes are all the same. Oligodendrocytes from different regions generate sheath lengths on microfibers and neurons that reflect their in vivo origin.

Published
2015
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7. Intrinsic and adaptive myelination - a sequential mechanism for smart wiring in the brain

Author

Bechler, Marie E, Swire, Matthew, and Ffrench-Constant, Charles

Subjects
nervous system, Journal Article, Review
Abstract

The concept of adaptive myelination - myelin plasticity regulated by activity - is an important advance for the field. What signals set up the adaptable pattern in the first place? Here we review work that demonstrates an intrinsic pathway within oligodendrocytes requiring only an axon-shaped substrate to generate multilayered and compacted myelin sheaths of a physiological length. Based on this, we discuss a model we proposed in 2015 which argues that myelination has two phases -intrinsic and then adaptive - which together generate "smart wiring" in which active axons become more myelinated. This model explains why prior studies have failed to identify a signal necessary for central nervous system myelination and argues that myelination, like synapses, might contribute to learning by the activity-dependent modification of an initially hard-wired pattern. This article is protected by copyright. All rights reserved.

Published
2017
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8. Scaffold-Mediated Sustained, Non-viral Delivery of miR-219/miR-338 Promotes CNS Remyelination

Author

Milbreta, Ulla, Lin, Junquan, Pinese, Coline, Ong, William, Chin, Jiah Shin, Shirahama, Hitomi, Mi, Ruifa, Williams, Anna, Bechler, Marie E., Wang, Jun, ffrench-Constant, Charles, Hoke, Ahmet, and Chew, Sing Yian

Abstract

The loss of oligodendrocytes (OLs) and subsequently myelin sheaths following injuries or pathologies in the CNS leads to debilitating functional deficits. Unfortunately, effective methods of remyelination remain limited. Here, we present a scaffolding system that enables sustained non-viral delivery of microRNAs (miRs) to direct OL differentiation, maturation, and myelination. We show that miR-219/miR-338 promoted primary rat OL differentiation and myelination in vitro. Using spinal cord injury as a proof-of-concept, we further demonstrate that miR-219/miR-338 could also be delivered non-virally in vivousing an aligned fiber-hydrogel scaffold to enhance remyelination after a hemi-incision injury at C5 level of Sprague-Dawley rats. Specifically, miR-219/miR-338 mimics were incorporated as complexes with the carrier, TransIT-TKO (TKO), together with neurotrophin-3 (NT-3) within hybrid scaffolds that comprised poly(caprolactone-co-ethyl ethylene phosphate) (PCLEEP)-aligned fibers and collagen hydrogel. After 1, 2, and 4 weeks post-treatment, animals that received NT-3 and miR-219/miR-338 treatment preserved a higher number of Olig2+oligodendroglial lineage cells as compared with those treated with NT-3 and negative scrambled miRs (Neg miRs; p < 0.001). Additionally, miR-219/miR-338 increased the rate and extent of differentiation of OLs. At the host-implant interface, more compact myelin sheaths were observed when animals received miR-219/miR-338. Similarly within the scaffolds, miR-219/miR-338 samples contained significantly more myelin basic protein (MBP) signals (p < 0.01) and higher myelination index (p < 0.05) than Neg miR samples. These findings highlight the potential of this platform to promote remyelination within the CNS.

Published
2024
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9. The phospholipase A₂ enzyme complex PAFAH Ib mediates endosomal membrane tubule formation and trafficking

Author

Bechler, Marie E, Doody, Anne M, Ha, Kevin D, Judson, Bret L, Chen, Ina, and Brown, William J

Subjects
Cytoplasm, Cell Membrane, Transferrin, Dyneins, Membrane Transport Proteins, Endosomes, Intracellular Membranes, Microtubules, Endocytosis, Phospholipases A2, Protein Subunits, Protein Transport, 1-Alkyl-2-acetylglycerophosphocholine Esterase, Humans, Microtubule-Associated Proteins, HeLa Cells
Abstract

Previous studies have shown that membrane tubule-mediated export from endosomal compartments requires a cytoplasmic phospholipase A(2) (PLA(2)) activity. Here we report that the cytoplasmic PLA(2) enzyme complex platelet-activating factor acetylhydrolase (PAFAH) Ib, which consists of α1, α2, and LIS1 subunits, regulates the distribution and function of endosomes. The catalytic subunits α1 and α2 are located on early-sorting endosomes and the central endocytic recycling compartment (ERC) and their overexpression, but not overexpression of their catalytically inactive counterparts, induced endosome membrane tubules. In addition, overexpression α1 and α2 altered normal endocytic trafficking; transferrin was recycled back to the plasma membrane directly from peripheral early-sorting endosomes instead of making an intermediate stop in the ERC. Consistent with these results, small interfering RNA-mediated knockdown of α1 and α2 significantly inhibited the formation of endosome membrane tubules and delayed the recycling of transferrin. In addition, the results agree with previous reports that PAFAH Ib α1 and α2 expression levels affect the distribution of endosomes within the cell through interactions with the dynein regulator LIS1. These studies show that PAFAH Ib regulates endocytic membrane trafficking through novel mechanisms involving both PLA(2) activity and LIS1-dependent dynein function.

Published
2011
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12. Selective PDE4 subtype inhibition provides new opportunities to intervene in neuroinflammatory versus myelin damaging hallmarks of multiple sclerosis

Author

Melissa Schepers, Dean Paes, Assia Tiane, Ben Rombaut, Elisabeth Piccart, Lieve van Veggel, Pascal Gervois, Esther Wolfs, Ivo Lambrichts, Chiara Brullo, Olga Bruno, Ernesto Fedele, Roberta Ricciarelli, Charles ffrench-Constant, Marie E. Bechler, Pauline van Schaik, Wia Baron, Evy Lefevere, Kobi Wasner, Anne Grünewald, Catherine Verfaillie, Paulien Baeten, Bieke Broux, Paul Wieringa, Niels Hellings, Jos Prickaerts, Tim Vanmierlo, Grunewald, Anne/0000-0002-4179-2994, SCHEPERS, Melissa, PAES, Dean, TIANE, Assia, ROMBAUT, Ben, PICCART, Elisabeth, VAN VEGGEL, Lieve, GERVOIS, Pascal, Brullo, Chiara, Bruno, Olga, Fedele, Ernesto, Ricciarelli, Roberta, Ffrench-Constant, Charles, Bechler, Marie E., Schaik, Pauline van, WOLFS, Esther, LAMBRICHTS, Ivo, Baron, Wia, LEFEVERE, Evy, Wasner, Kobi, Gruenewald, Anne, Verfaillie, Catherine, Wieringa, Paul, Prickaerts, Jos, BROUX, Bieke, BAETEN, Paulien, HELLINGS, Niels, VANMIERLO, Tim, RS: MHeNs - R3 - Neuroscience, Basic Neuroscience 2, Basic Neuroscience 1, CTR, RS: MERLN - Complex Tissue Regeneration (CTR), and Psychiatrie & Neuropsychologie

Subjects
Multiple sclerosis, Behavioral Neuroscience, Neuroinflammation, Remyelination, Endocrine and Autonomic Systems, Phosphodiesterases, Immunology, Biochemistry, biophysics & molecular biology [F05] [Life sciences], Biochimie, biophysique & biologie moléculaire [F05] [Sciences du vivant]
Abstract

Multiple sclerosis (MS) is a chronic autoimmune disease of the central nervous system (CNS) characterized by focal inflammatory lesions and prominent demyelination. Even though the currently available therapies are effective in treating the initial stages of disease, they are unable to halt or reverse disease progression into the chronic progressive stage. Thus far, no repair-inducing treatments are available for progressive MS patients. Hence, there is an urgent need for the development of new therapeutic strategies either targeting the destructive immunological demyelination or boosting endogenous repair mechanisms. Using in vitro, ex vivo, and in vivo models, we demonstrate that selective inhibition of phosphodiesterase 4 (PDE4), a family of enzymes that hydrolyzes and inactivates cyclic adenosine monophosphate (cAMP), reduces inflammation and promotes myelin repair. More specifically, we segregated the myelination-promoting and anti-inflammatory effects into a PDE4Dand PDE4B-dependent process respectively. We show that inhibition of PDE4D boosts oligodendrocyte progenitor cells (OPC) differentiation and enhances (re)myelination of both murine OPCs and human iPSC-derived OPCs. In addition, PDE4D inhibition promotes in vivo remyelination in the cuprizone model, which is accompanied by improved spatial memory and reduced visual evoked potential latency times. We further identified that PDE4B-specific inhibition exerts anti-inflammatory effects since it lowers in vitro monocytic nitric oxide (NO) production and improves in vivo neurological scores during the early phase of experimental autoimmune encephalomyelitis (EAE). In contrast to the pan PDE4 inhibitor roflumilast, the therapeutic dose of both the PDE4B-specific inhibitor A33 and the PDE4D-specific inhibitor Gebr32a did not trigger emesis-like side effects in rodents. Finally, we report distinct PDE4D isoform expression patterns in human area postrema neurons and human oligodendroglia lineage cells. Using the CRISPR-Cas9 system, we confirmed that pde4d1/2 and pde4d6 are the key targets to induce OPC differentiation. Collectively, these data demonstrate that gene specific PDE4 inhibitors have potential as novel therapeutic agents for targeting the distinct disease processes of MS. This work has been supported by FWO (12G0817N, 1S57521N, G041421N, and 12G0817N), Fondation Charctot Stichting (ID2020- 0019), Nationale Belgische Multiple Sclerose Liga (Charco18VT), MS Liga Vlaanderen and Stichting MS Research (18-1016 MS). MS, EP, JP and TV have a proprietary interest in selective PDE4D inhibitors for the treatment of demyelinating disorders and neurodegenerative disorders. JP has a proprietary interest in the PDE4 inhibitor roflumilast for the treatment of cognitive impairment as well as PDE4D inhibitors for the treatment of Alzheimer’s disease. We thank Prof. Dr. O.N. Viacheslav (University Medical Center Hamburg-Eppendorf, German Center for Cardiovascular Research) and Prof. Dr. M. Conti (University of California), for providing the PDE4B KO animals. Furthermore, we thank Rewind Therapeutics for providing the visual evoked potential equipment.

Published
2023

13. Gβ1γ2 activates phospholipase A 2 -dependent Golgi membrane tubule formation.

Author

Bechler ME and Brown WJ

Abstract

Heterotrimeric G proteins transduce the ligand binding of transmembrane G protein coupled receptors into a variety of intracellular signaling pathways. Recently, heterotrimeric Gβγ subunit signaling at the Golgi complex has been shown to regulate the formation of vesicular transport carriers that deliver cargo from the Golgi to the plasma membrane. In addition to vesicles, membrane tubules have also been shown to mediate export from the Golgi complex, which requires the activity of cytoplasmic phospholipase A 2 (PLA 2 ) enzyme activity. Through the use of an in vitro reconstitution assay with isolated Golgi complexes, we provide evidence that Gβ1γ2 signaling also stimulates Golgi membrane tubule formation. In addition, we show that an inhibitor of Gβγ activation of PLA 2 enzymes inhibits in vitro Golgi membrane tubule formation. Additionally, purified Gβγ protein stimulates membrane tubules in the presence of low (sub-threshold) cytosol concentrations. Importantly, this Gβγ stimulation of Golgi membrane tubule formation was inhibited by treatment with the PLA 2 antagonist ONO-RS-082. These studies indicate that Gβ1γ2 signaling activates PLA 2 enzymes required for Golgi membrane tubule formation, thus establishing a new layer of regulation for this process.

Published
2014
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