Two genetically different MU-NANA neuraminidases in human leucocytes

Two genetically different MU-NANA neuraminidases in human leucocytes

Human leucocytes contain two different MU-NANA neuraminidases, which can be distinguished by Concanavalin A binding. The Con A binding form is predominant in lymphocytes (more than 80%) and the non-binding form predominates in granulocytes. The pH optima of both these neuraminidases as well as their...

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Bibliographic Details
Published in:Biochemical and biophysical research communications Vol. 117; no. 2; p. 470
Main Authors: Verheijen, F W, Janse, H C, van Diggelen, O P, Bakker, H D, Loonen, M C, Durand, P, Galjaard, H
Format: Journal Article
Language:English
Published: United States 16-12-1983
Subjects:
beta-Galactosidase - blood
Chromatography, Affinity
Concanavalin A - metabolism
Granulocytes - enzymology
Humans
Hydrogen-Ion Concentration
Hymecromone - analogs & derivatives
Hymecromone - metabolism
Isoenzymes - deficiency
Isoenzymes - genetics
Leukocytes - enzymology
Neuraminidase - deficiency
Neuraminidase - genetics
Umbelliferones - metabolism
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Summary:Human leucocytes contain two different MU-NANA neuraminidases, which can be distinguished by Concanavalin A binding. The Con A binding form is predominant in lymphocytes (more than 80%) and the non-binding form predominates in granulocytes. The pH optima of both these neuraminidases as well as their subcellular localization as determined by Percoll gradient centrifugation suggest that they are both lysosomal. Immunological studies indicate that the Con A binding form is present in a complex with beta-galactosidase whereas the non-binding form is not. Leucocytes from patients with sialidosis or galactosialidosis are deficient in the Con A binding neuraminidase, whereas the non-binding form is normal. In sialolipidosis both forms are normal. These results demonstrate that leucocytes contain at least two genetically different MU-NANA neuraminidases. Thus, the use of leucocytes should be avoided for the diagnosis of sialidosis and galactosialidosis, and isolated lymphocytes should be used to obtain reliable results.
ISSN:0006-291X
DOI:10.1016/0006-291X(83)91224-X