Abstract

The long term objective of this research is to characterize axolemmnal and myelin molecules which cause Schwann cells (SC) to proliferate and to understand the mechanism by which these signals are transduced across the Schwann cell plasma membrane. Axolemma- enriched fractions (AEF) from myelinated, non-myelinated and unmyelinated sources will be incubated with cultured SC. After stimulation of SC with AEF, fluorescent dyes will be used to study calcium mobilization and activation of the Na+/H+ antiporter; the pattern of cytoplasmic and membrane phosphorylation by 32P will also be examined. Using fluorescent labelled AEF, we will quantitate the amount of AEF per SC to test the hypothesis that a threshold amount of AEF-SC interaction is required to """"""""trigger"""""""" mitosis. The myelin-related mitogens will be solubilized and purified by high performance liquid chromatography (HPLC) followed by biochemical characterization. The role of macrophage versus SC processing of exogenous myelin membrane to produce a SC mitogen will be evaluated via the development of macrophage-free cultures. A transformed SC line will be produced utilizing a new DNA construct containing a metallothionein promoter linked to the large T antigen of SV-40 virus in the absence of divalent cation the SC line should undergo normal differentiation when presented with a myelin-competent neurite. Soluble neuronrelated SC mitogen will be produced from cultured neurons by severing them from their neurites and inhibiting the synthesis of a class of molecules to which they are normally bound. The nature of axonal molecules responsible for three molecular manifestations of SC differentiation will be examined; secretion of Type IV procollogen, aggregation of SC surface laminin into linear arrays and possible increase of SC laminin receptors and increase of myelin specific lipids (galactocerebroside) as visualized immunologically and protein (Po, the major myelin glycoprotein) as determined by increased levels of Po mRNA or increased translation of Po mRNA. It is anticipated that these studies will profice a baseline from which to evaluate how glial cells normally respond to neuronal signals os that we can assess how such signalling may be compromised in cases of uncontrolled SC proliferation as in neurofibromatosis. In addition, this research will clarify the relative roles of macrophages verus SC in the proliferative response which follows the Wallerian degeneration characteristic of peripheral nerve injury.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS015408-11
Application #
3396214
Study Section
Neurological Sciences Subcommittee 1 (NLS)
Project Start
1979-07-01
Project End
1991-08-31
Budget Start
1989-09-01
Budget End
1990-08-31
Support Year
11
Fiscal Year
1989
Total Cost
Indirect Cost

  Institution

Name
Virginia Commonwealth University
Department
Type
Overall Medical
DUNS #
City
Richmond
State
VA
Country
United States
Zip Code
23298

  Publications

South, S A; Deibler, G E; Tzeng, S F et al. (2000) Myelin basic protein (MBP) and MBP peptides are mitogens for cultured astrocytes. Glia 29:81-90
Tzeng, S F; Deibler, G E; DeVries, G H (1999) Myelin basic protein and myelin basic protein peptides induce the proliferation of Schwann cells via ganglioside GM1 and the FGF receptor. Neurochem Res 24:255-60
DeVries, G H; Campbell, B; Saunders, R (1999) Isolation and characterization of unmyelinated axolemma from bovine splenic nerve. J Neurosci Res 57:670-9
Calderon, R O; DeVries, G H (1997) Lipid composition and phospholipid asymmetry of membranes from a Schwann cell line. J Neurosci Res 49:372-80
Chakrabarti, A K; Neuberger, T; Russell, T et al. (1997) Immunolocalization of cytoplasmic and myelin mcalpain in transfected Schwann cells: II. Effect of withdrawal of growth factors. J Neurosci Res 47:609-16
Neuberger, T; Chakrabarti, A K; Russell, T et al. (1997) Immunolocalization of cytoplasmic and myelin mcalpain in transfected Schwann cells: I. Effect of treatment with growth factors. J Neurosci Res 47:521-30
Raabe, T D; Clive, D R; Neuberger, T J et al. (1996) Cultured neonatal Schwann cells contain and secrete neuregulins. J Neurosci Res 46:263-70
Starr, R; Attema, B; DeVries, G H et al. (1996) Neurofilament phosphorylation is modulated by myelination. J Neurosci Res 44:328-37
Eichberg, J; Sheldon, R; Kuruvilla, R et al. (1996) Receptor-mediated phosphoinositide metabolism in peripheral nerve and cultured Schwann cells. J Lipid Mediat Cell Signal 14:187-95
Lee, M M; Sato-Bigbee, C; De Vries, G H (1996) Schwann cells stimulated by axolemma-enriched fractions express cyclic AMP responsive element binding protein. J Neurosci Res 46:204-10

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