Assembly of juxtaparanodes in myelinating DRG culture: Differential clustering of the Kv1/Caspr2 complex and scaffolding protein 4.1B
Autor: | Marilyne Labasque, Catherine Faivre-Sarrailh, Bruno Hivert, Laurence Goutebroze, Nicolas Tricaud, Delphine Pinatel |
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Rok vydání: | 2016 |
Předmět: |
0301 basic medicine
Scaffold protein Node of Ranvier Cell adhesion molecule Fluorescence recovery after photobleaching Biology Potassium channel Cell biology 03 medical and health sciences Cellular and Molecular Neuroscience 030104 developmental biology medicine.anatomical_structure nervous system Neurology Membrane protein medicine Cell adhesion Neuroscience Ion channel |
Zdroj: | Glia. 64:840-852 |
ISSN: | 0894-1491 |
DOI: | 10.1002/glia.22968 |
Popis: | The precise distribution of ion channels at the nodes of Ranvier is essential for the efficient propagation of action potentials along myelinated axons. The voltage-gated potassium channels Kv1.1/1.2 are clustered at the juxtaparanodes in association with the cell adhesion molecules, Caspr2 and TAG-1 and the scaffolding protein 4.1B. In the present study, we set up myelinating cultures of DRG neurons and Schwann cells to look through the formation of juxtaparanodes in vitro. We showed that the Kv1.1/Kv1.2 channels were first enriched at paranodes before being restricted to distal paranodes and juxtaparanodes. In addition, the Kv1 channels displayed an asymmetric expression enriched at the distal juxtaparanodes. Caspr2 was strongly co-localized with Kv1.2 whereas the scaffolding protein 4.1B was preferentially recruited at paranodes while being present at juxtaparanodes too. Kv1.2/Caspr2 but not 4.1B, also transiently accumulated within the nodal region both in myelinated cultures and developing sciatic nerves. Studying cultures and sciatic nerves from 4.1B KO mice, we further showed that 4.1B is required for the proper targeting of Caspr2 early during myelination. Moreover, using adenoviral-mediated expression of Caspr-GFP and photobleaching experiments, we analyzed the stability of paranodal junctions and showed that the lateral stability of paranodal Caspr was not altered in 4.1B KO mice indicating that 4.1B is not required for the assembly and stability of the paranodal junctions. Thus, developing an adapted culture paradigm, we provide new insights into the dynamic and differential distribution of Kv1 channels and associated proteins during myelination. |
Databáze: | OpenAIRE |
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