Relationship between the acid phosphatases of the Kurloff body and the major 30-35 kDa glycoproteins of the Kurloff cell

Relationship between the acid phosphatases of the Kurloff body and the major 30-35 kDa glycoproteins of the Kurloff cell

This study deals with the acid phosphatase (AcPase) of the Kurloff body (KB), a large (10 microns diameter) periodic acid-Schiff-positive lysosomal inclusion body present in Kurloff cells (KC). KC AcPase were extracted, with similar yields, either with non-ionic detergent solution or after Dounce ho...

Full description

Saved in:
Bibliographic Details
Published in:Biology of the cell Vol. 83; no. 2-3; p. 141
Main Authors: Oulhaj, N, Taouji, S, Izard, J, Landemore, G
Format: Journal Article
Language:English
Published: England 1995
Subjects:
Acid Phosphatase - chemistry
Acid Phosphatase - metabolism
Animals
Chromatography, Affinity
Female
Glycoproteins - chemistry
Guinea Pigs
Lymphoid Tissue - cytology
Lymphoid Tissue - enzymology
Male
Molecular Weight
Sialic Acids - metabolism
Subcellular Fractions - enzymology
Online Access:Get more information
Tags: Add Tag
No Tags, Be the first to tag this record!
Description
Summary:This study deals with the acid phosphatase (AcPase) of the Kurloff body (KB), a large (10 microns diameter) periodic acid-Schiff-positive lysosomal inclusion body present in Kurloff cells (KC). KC AcPase were extracted, with similar yields, either with non-ionic detergent solution or after Dounce homogenization in low ionic strength buffer suggesting that they mainly correspond to hydrosoluble AcPase. After DEAE-cellulose chromatography of such crude Dounce-extracts, 97% of KC AcPase activity was recovered in the unbound glycoprotein fraction (peak I)1). The main protein content consisted of, as testified by SDS-PAGE analysis, major KC glycoproteins of 30-35 kDa. Thus, KC AcPase, and particularly sialoAcPase, may be assumed to correspond to these N-glycosylproteins among which the presence of alpha (2,6) sialoglycoproteins was previously established. Following electrophoresis on a 4-15% gradient native polyacrylamide gel or isoelectric focusing, the two size populations (200 kDa and 500 kDa) and up to 20 isoforms of KC AcPase were respectively detected by zymography in peak I. After Clostridium-derived sialidase digestion of peak I, the highly active bands observed at pH 3.5-5.2 disappeared. These zymographic patterns were similar to those obtained with crude extracts. After Concanavalin A (ConA)-Sepharose chromatography of peak I, the single ConA-bound glucosamine-labelled peak, eluted at 200 methyl-alpha-D-mannopyranose, contained the AcPase activity while the ConA-unbound peak was devoid of any acid phosphatase activity. After SDS-PAGE analysis, the ConA-bound fraction appeared to correspond only to a single broad protein band in the 30-35 kDa zone.
ISSN:0248-4900
DOI:10.1016/0248-4900(96)81302-5