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The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair

In vitro cell-based assays have been fundamental in modern drug discovery and have led to the identification of novel therapeutics. We have developed complex mixed central nervous system (CNS) cultures, which recapitulate the normal process of myelination over time and allow the study of several par...

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Autores principales: McCanney, George A., Lindsay, Susan L., McGrath, Michael A., Willison, Hugh J., Moss, Claire, Bavington, Charles, Barnett, Susan C.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6784161/
https://www.ncbi.nlm.nih.gov/pubmed/31261710
http://dx.doi.org/10.3390/biology8030052
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author McCanney, George A.
Lindsay, Susan L.
McGrath, Michael A.
Willison, Hugh J.
Moss, Claire
Bavington, Charles
Barnett, Susan C.
author_facet McCanney, George A.
Lindsay, Susan L.
McGrath, Michael A.
Willison, Hugh J.
Moss, Claire
Bavington, Charles
Barnett, Susan C.
author_sort McCanney, George A.
collection PubMed
description In vitro cell-based assays have been fundamental in modern drug discovery and have led to the identification of novel therapeutics. We have developed complex mixed central nervous system (CNS) cultures, which recapitulate the normal process of myelination over time and allow the study of several parameters associated with CNS damage, both during development and after injury or disease. In particular, they have been used as a reliable screen to identify drug candidates that may promote (re)myelination and/or neurite outgrowth. Previously, using these cultures, we demonstrated that a panel of low sulphated heparin mimetics, with structures similar to heparan sulphates (HSs), can reduce astrogliosis, and promote myelination and neurite outgrowth. HSs reside in either the extracellular matrix or on the surface of cells and are thought to modulate cell signaling by both sequestering ligands, and acting as co-factors in the formation of ligand-receptor complexes. In this study, we have used these cultures as a screen to address the repair potential of numerous other commercially available sulphated glycomolecules, namely heparosans, ulvans, and fucoidans. These compounds are all known to have certain characteristics that mimic cellular glycosaminoglycans, similar to heparin mimetics. We show that the N-sulphated heparosans promoted myelination. However, O-sulphated heparosans did not affect myelination but promoted neurite outgrowth, indicating the importance of structure in HS function. Moreover, neither highly sulphated ulvans nor fucoidans had any effect on remyelination but CX-01, a low sulphated porcine intestinal heparin, promoted remyelination in vitro. These data illustrate the use of myelinating cultures as a screen and demonstrate the potential of heparin mimetics as CNS therapeutics.
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spelling pubmed-67841612019-10-16 The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair McCanney, George A. Lindsay, Susan L. McGrath, Michael A. Willison, Hugh J. Moss, Claire Bavington, Charles Barnett, Susan C. Biology (Basel) Article In vitro cell-based assays have been fundamental in modern drug discovery and have led to the identification of novel therapeutics. We have developed complex mixed central nervous system (CNS) cultures, which recapitulate the normal process of myelination over time and allow the study of several parameters associated with CNS damage, both during development and after injury or disease. In particular, they have been used as a reliable screen to identify drug candidates that may promote (re)myelination and/or neurite outgrowth. Previously, using these cultures, we demonstrated that a panel of low sulphated heparin mimetics, with structures similar to heparan sulphates (HSs), can reduce astrogliosis, and promote myelination and neurite outgrowth. HSs reside in either the extracellular matrix or on the surface of cells and are thought to modulate cell signaling by both sequestering ligands, and acting as co-factors in the formation of ligand-receptor complexes. In this study, we have used these cultures as a screen to address the repair potential of numerous other commercially available sulphated glycomolecules, namely heparosans, ulvans, and fucoidans. These compounds are all known to have certain characteristics that mimic cellular glycosaminoglycans, similar to heparin mimetics. We show that the N-sulphated heparosans promoted myelination. However, O-sulphated heparosans did not affect myelination but promoted neurite outgrowth, indicating the importance of structure in HS function. Moreover, neither highly sulphated ulvans nor fucoidans had any effect on remyelination but CX-01, a low sulphated porcine intestinal heparin, promoted remyelination in vitro. These data illustrate the use of myelinating cultures as a screen and demonstrate the potential of heparin mimetics as CNS therapeutics. MDPI 2019-06-28 /pmc/articles/PMC6784161/ /pubmed/31261710 http://dx.doi.org/10.3390/biology8030052 Text en © 2019 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
McCanney, George A.
Lindsay, Susan L.
McGrath, Michael A.
Willison, Hugh J.
Moss, Claire
Bavington, Charles
Barnett, Susan C.
The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair
title The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair
title_full The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair
title_fullStr The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair
title_full_unstemmed The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair
title_short The Use of Myelinating Cultures as a Screen of Glycomolecules for CNS Repair
title_sort use of myelinating cultures as a screen of glycomolecules for cns repair
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6784161/
https://www.ncbi.nlm.nih.gov/pubmed/31261710
http://dx.doi.org/10.3390/biology8030052
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