MICROSOMAL CASEIN KINASE-II IN ENDOPLASMIC-RETICULUM-RICH AND GOLGI-APPARATUS-RICH FRACTIONS OF ROS-17/2.8 OSTEOBLAST-LIKE CELLS - AN ENZYME THAT MODIFIES OSTEOPONTIN

被引：14

作者：

WU, CB

PAN, YM

SHIMIZU, Y

机构：

[1] Department of Clinical Dental Sciences, Faculty of Dentistry, University of British Columbia, Vancouver, V6T 1Z3, B.C.

来源：

CALCIFIED TISSUE INTERNATIONAL | 1995年 / 57卷 / 04期

关键词：

CASEIN KINASE II; OSTEOBLASTS; OSTEOPONTIN; PHOSPHORYLATION;

D O I：

10.1007/BF00298884

中图分类号：

R5 [内科学];

学科分类号：

1002 ; 100201 ;

摘要：

Osteopontin is an acidic phosphoprotein containing casein kinase II (CKII) phosphorylatable sites and an acidic amino acid cluster. The metabolically P-32-labelings of both serines and threonines in vitro in osteopontin immunoprecipitated from rat osteoblast-like ROS 17/2.8 cells may suggest that casein kinase II catalyzes this modification, The enzyme occurs in microsomal fractions of rat osteoblast-like ROS 17/2.8 cells. Subcellular fractions containing endoplasmic reticulum and Golgi apparatus were isolated by differential centrifugation and were identified according to their ultrastructures and the presence of marker enzymes such as glucose-6-phosphatase and thiamine pyrophosphatase, respectively. Both fractions phosphorylated the partially dephosphorylated osteopontin and the specific substrate peptide RRREEETEEE. Endoplasmic reticulum-catalyzed peptide phosphorylation was 2.7 times lower than that of Golgi although both endoplasmic reticulum- and Golgi-catalyzed peptide reactions were 50% inhibited by 20 and 100 ng/ml heparin, respectively. Western blot analysis revealed that both fractions contained osteopontin and microsomal CKII. Furthermore, microsomal CKII was immunogold-labeled in endoplasmic reticulum and Golgi apparatus. Heparin inhibition and utilization of [gamma-P-32]GTP as a phosphate donor by both fractions confirmed their capacity to phosphorylate osteopontin. The results suggest that microsomal CKII modifies the acidic matrix proteins during transportation. These matrix phosphoproteins may participate in the mineralization process of hard tissues.

引用

页码：285 / 292

页数：8

共 46 条

[21] MULTIPLE FORMS OF SPPI (SECRETED PHOSPHOPROTEIN, OSTEOPONTIN) SYNTHESIZED BY NORMAL AND TRANSFORMED RAT BONE CELL-POPULATIONS - REGULATION BY TGF-BETA [J].

KUBOTA, T ;

ZHANG, Q ;

WRANA, JL ;

BER, R ;

AUBIN, JE ;

BUTLER, WT ;

SODEK, J .

BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS, 1989, 162 (03) :1453-1459

[22] A SYNTHETIC PEPTIDE SUBSTRATE SPECIFIC FOR CASEIN KINASE-II [J].

KUENZEL, EA ;

KREBS, EG .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1985, 82 (03) :737-741

[23] DENTIN PHOSPHOPROTEIN - EXTRACELLULAR CALCIUM-BINDING PROTEIN [J].

LEE, SL ;

VEIS, A ;

GLONEK, T .

BIOCHEMISTRY, 1977, 16 (13) :2971-2979

[24] P-31 NUCLEAR MAGNETIC-RESONANCE SPECTROSCOPIC EVIDENCE FOR TERNARY COMPLEX-FORMATION OF FETAL DENTIN PHOSPHOPROTEIN WITH CALCIUM AND INORGANIC ORTHO-PHOSPHATE IONS [J].

LEE, SL ;

GLONEK, T ;

GLIMCHER, MJ .

CALCIFIED TISSUE INTERNATIONAL, 1983, 35 (06) :815-818

[25]

LOWRY OH, 1951, J BIOL CHEM, V193, P265

[26] IMPROVEMENTS IN EPOXY RESIN EMBEDDING METHODS [J].

LUFT, JH .

JOURNAL OF BIOPHYSICAL AND BIOCHEMICAL CYTOLOGY, 1961, 9 (02) :409-&

[27] INDUCTION AND INHIBITION OF HYDROXYAPATITE FORMATION BY RAT DENTIN PHOSPHOPROTEIN INVITRO [J].

LUSSI, A ;

CRENSHAW, MA ;

LINDE, A .

ARCHIVES OF ORAL BIOLOGY, 1988, 33 (09) :685-691

[28]

MORRE DJ, 1971, METHOD ENZYMOL, V22, P130

[29] USE OF LIGHT MICROSCOPIC IMMUNOTECHNIQUES IN SELECTING PREPARATION CONDITIONS AND IMMUNOPROBES FOR ULTRASTRUCTURAL IMMUNOLABELLING OF LACTOFERRIN [J].

MUTASA, HCF ;

PEARSON, EC .

HISTOCHEMICAL JOURNAL, 1988, 20 (10) :558-566

[30] DENTAL PHOSPHOPROTEIN-INDUCED FORMATION OF HYDROXYLAPATITE DURING INVITRO SYNTHESIS OF AMORPHOUS CALCIUM-PHOSPHATE [J].

NAWROT, CF ;

CAMPBELL, DJ ;

SCHROEDER, JK ;

VANVALKENBURG, M .

BIOCHEMISTRY, 1976, 15 (16) :3445-3449

← 1 2 3 4 5 →