Abstract

Ultimately, we want to understand how the myelin sheath acquires its extraordinary morphology, and so provide the groundwork for understanding a wide variety of de- and dysmyelinating disease states, such as Multiple Sclerosis, Guillain-Barre Syndrome and the Charcot-Marie-Tooth Diseases. The mechanisms by which the myelin sheath is generated remain elusive. We will test during the next grant period the validity of a new model we have developed for the generation of the myelin spiral. This model anticipates that the first step in the myelination program occurs when a protein scaffold is laid down adhesively linking the myelinating cell with the axon, and forming a guide for new membrane addition. In order to test this model we must first accurately define the positions of certain key marker proteins, (some of which are newly discovered) when these molecules are expressed naturally (in terms of temporal and spatial distribution) in the myelin-axon protein scaffold. We also propose to uncover the actual pattern of new membrane addition to forming myelin, and observe the dynamical movements of protein, lipid and cytoplasmic compartments, using selected fluorescently-labeled myelin protein or axonal moieties as """"""""reference markers."""""""" Our approach is to study living, actively myelinating cells directly observed by high resolution confocal and two photon microscopy, and we will define how initially completely segregated intracellular pathways ultimately converge to yield the myelin sheath. Accordingly, (I) we will engineer mice using bacterial artificial chromosomes (BAC cloning) to express, as naturally as possible, certain key neural cell proteins labeled in tandem with innocuous fluorescent moieties. The protein products of these artificial genes will be fluorescent, obviating the need for antibodies visualized by indirect methods. Furthermore, BAC methodologies yield protein products whose expression (temporal and spatial) is identical to the natural gene. These mice will be used as source material for in vitro myelination studies. (II) We will study fluorescent lipid incorporation into surface membranes of myelinating cells, and compare these data to the assembly parameters of the protein scaffold formed at the internodal ends, as ascertained in Aim I. Finally, (III) we will directly observe dynamical movements of the cytoplasmic channels that enclose non-compact myelin through the injection of fluorescent beads directly into pre-myelinating Schwann cells in culture, and examine the movement of these beads over time as myelination progresses. The studies we propose will allow a comprehensive analysis of the short and long term (several hours to weeks) continuous, relative contributions of proteins, membrane lipid and fluid cytoplasmic components to myelin formation.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS020147-20
Application #
6640525
Study Section
Special Emphasis Panel (ZRG1-MDCN-2 (01))
Program Officer
Utz, Ursula
Project Start
1987-09-30
Project End
2007-07-31
Budget Start
2003-08-01
Budget End
2004-07-31
Support Year
20
Fiscal Year
2003
Total Cost
$256,500
Indirect Cost

  Institution

Name
Mcgill University
Department
Type
DUNS #
205667090
City
Montreal
State
PQ
Country
Canada
Zip Code
H3 0-G4

  Publications

Maret, Deborah; Gruzglin, Eugenia; Sadr, Mohamad Seyed et al. (2010) Surface expression of precursor N-cadherin promotes tumor cell invasion. Neoplasia 12:1066-80
Corell, Mikael; Wicher, Grzegorz; Limbach, Christoph et al. (2010) Spatiotemporal distribution and function of N-cadherin in postnatal Schwann cells: A matter of adhesion? J Neurosci Res 88:2338-49
Yagita, Yoshiki; Sakurai, Takeshi; Tanaka, Hidekazu et al. (2009) N-cadherin mediates interaction between precursor cells in the subventricular zone and regulates further differentiation. J Neurosci Res 87:3331-42
Pedraza, Liliana; Huang, Jeffrey K; Colman, David (2009) Disposition of axonal caspr with respect to glial cell membranes: Implications for the process of myelination. J Neurosci Res 87:3480-91
Zalc, B; Goujet, D; Colman, D (2008) The origin of the myelination program in vertebrates. Curr Biol 18:R511-2
Yasuda, Shin; Tanaka, Hidekazu; Sugiura, Hiroko et al. (2007) Activity-induced protocadherin arcadlin regulates dendritic spine number by triggering N-cadherin endocytosis via TAO2beta and p38 MAP kinases. Neuron 56:456-71
Roth, Alejandro D; Ivanova, Anna; Colman, David R (2006) New observations on the compact myelin proteome. Neuron Glia Biol 2:15-21
Frank, Marcus; Ebert, Matthias; Shan, Weisong et al. (2005) Differential expression of individual gamma-protocadherins during mouse brain development. Mol Cell Neurosci 29:603-16
Yagita, Yoshiki; Barjis, Isaac; Hecht, Michael et al. (2005) Partial nucleotide sequences and expression patterns of frog (Rana pipiens) ephrin-A2 and ephrin-A5 mRNA. Brain Res Dev Brain Res 159:72-7
Huang, Jeffrey K; Phillips, Greg R; Roth, Alejandro D et al. (2005) Glial membranes at the node of Ranvier prevent neurite outgrowth. Science 310:1813-7

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