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JBC, Vol. 251, Issue 1, 153-158, Jan, 1976
J. F. Poduslo, R. H. Quarles and R. O. Brady
The molecular organization of surface galactose residues in glycoproteins
of the intact myelin sheath was investigated using the enzymatic membrane
probe, galactose oxidase. Rat spinal cords treated under physiological
conditions with this nonpermanent probe were labeled specifically in
galactose residues by reduction with tritiated sodium borohydride. The
enzymatically modified proteins from isolated myelin were analyzed
electrophoretically and their specific radioactivities determined. Results
indicated tritium label associated with a surprising variety of high
molecular weight proteins. The most extensively labeled peak corresponded
to the major myelin glycoprotein as indicated by the coincidence of tritium
label with that of [14C]fucose used as an internal marker for the
glycoproteins. The radioactivity associated with this protein was 1.1 to
2.7 times higher after treatment with galactose oxidase when compared to
reduction in the absence of the enzyme and 1.4 to 4.8 times higher when
oxidized and reduced after prior treatment with neuraminidase. The results
suggest a complex heterogeneity of minor glycoproteins associated with
isolated myelin. It is concluded that from this complexity of
glycoproteins, a major glycoprotein is at least partially localized on the
external surface of either the intact myelin sheath or the closely
associated oligodendroglial plasma membrane. Such a localization of this
glycoprotein and the probable localization of the other glycoproteins
enhances their potential role in specific interactions in the process of
mpyelination or myelin maintenance.
External labeling of galactose in surface membrane glycoproteins of the intact myelin sheath
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