Your search keyword '"M Inagaki"' showing total 52 results

1. Balance between Activities of Rho Kinase and Type 1 Protein Phosphatase Modulates Turnover of Phosphorylation and Dynamics of Desmin/Vimentin Filaments

Author

Hiroyasu Inada, Hideaki Togashi, Kozo Kaibuchi, Koh-ichi Nagata, M Inagaki, and Yu Nakamura

Subjects

inorganic chemicals, Time Factors, Immunoblotting, Molecular Sequence Data, macromolecular substances, Protein Serine-Threonine Kinases, Mitogen-activated protein kinase kinase, Biochemistry, Cell Line, Desmin, MAP2K7, Mice, Okadaic Acid, Phosphoprotein Phosphatases, Animals, Humans, Vimentin, Intermediate Filament Protein, Amino Acid Sequence, Enzyme Inhibitors, Phosphorylation, Oxazoles, Molecular Biology, Rho-associated protein kinase, rho-Associated Kinases, Microscopy, Confocal, Dose-Response Relationship, Drug, biology, Chemistry, Cell Cycle, Cyclin-dependent kinase 2, Intracellular Signaling Peptides and Proteins, 3T3 Cells, Cell Biology, Molecular biology, Recombinant Proteins, enzymes and coenzymes (carbohydrates), Rho kinase inhibitor, biology.protein, bacteria, Marine Toxins, Cyclin-dependent kinase 9

Abstract

To analyze the cell cycle-dependent desmin phosphorylation by Rho kinase, we developed antibodies specifically recognizing the kinase-dependent phosphorylation of desmin at Thr-16, Thr-75, and Thr-76. With these antibodies, phosphorylation of desmin was observed specifically at the cleavage furrow in late mitotic Saos-2 cells. We then found that treatment of the interphase cells with calyculin A revealed phosphorylation at all the three sites of desmin. We also found that an antibody, which specifically recognizes vimentin phosphorylated at Ser-71 by Rho kinase, became immunoreactive after calyculin A treatment. This calyculin A-induced interphase phosphorylation of vimentin at Ser-71 was blocked by Rho kinase inhibitor or by expression of the dominant-negative Rho kinase. Taken together, our results indicate that Rho kinase is activated not only in mitotic cells but also interphase ones, and phosphorylates intermediate filament proteins, although the apparent phosphorylation level is diminished to an undetectable level due to the constitutive action of type 1 protein phosphatase. The balance between intermediate filament protein phosphorylation by Rho kinase and dephosphorylation by type 1 protein phosphatase may affect the continuous exchange of intermediate filament subunits between a soluble pool and polymerized intermediate filaments.

Published

1999

2. The phosphorylation of kinesin regulates its binding to synaptic vesicles

Author

M Inagaki, Nobutaka Hirokawa, Hiroshi Yorifuji, and Reiko Sato-Yoshitake

Subjects

Microtubule-associated protein, Kinesins, macromolecular substances, Biology, Microtubules, Biochemistry, Synaptic vesicle, Microtubule, Animals, Phosphorylation, Protein kinase A, Molecular Biology, Cerebral Cortex, Vesicle, Brain, Cell Biology, Rats, Cell biology, Models, Structural, Kinetics, Microscopy, Electron, Axoplasmic transport, Kinesin, Synaptic Vesicles, Protein Binding

Abstract

Membrane organella are transported bidirectionally in cells, and the axonal transport system has provided an ideal model system for studying this bidirectional transport. Kinesin and cytoplasmic dynein were identified as candidates for the motor molecules of fast axonal transport, which transport organella along microtubules anterogradely and retrogradely. However, the mechanism that controls this bidirectional transport is unknown. Our previous work revealed that kinesin in axons was associated abundantly with anterogradely transported membranous organella, most of which are believed to be precursors of synaptic vesicles and axonal plasma membranes, while the fractions bound to retrogradely transported ones were very small (Hirokawa, N., Sato-Yoshitake, R., Kobayashi, N., Pfister, K. K., Bloom, G. S., and Brady, S. T. (1991) J. Cell Biol. 114, 295-302). Here we demonstrated in vitro that the binding of kinesin to synaptic vesicles was concentration-dependent and saturable and could be released by high salt concentration. When kinesin was phosphorylated by cAMP-dependent protein kinase, its binding to symaptic vesicles was significantly reduced. By motility assay and by statistical analysis using electron microscopy, we further revealed that synaptic vesicles preincubated with phosphorylated kinesin associated less frequently with microtubules than synaptic vesicles preincubated with unphosphorylated kinesin. The phosphorylation of kinesin should therefore play an essential role in regulating the direction of fast axonal transport by inhibiting its binding to membrane organella, thus releasing it from membrane organella at nerve terminals.

Published

1992

3. Purification and characterization of smooth muscle myosin-associated phosphatase from chicken gizzards

Author

Toshiaki Mitsui, Mitsuo Ikebe, and M Inagaki

Subjects

Myosin light-chain kinase, Phosphatase, macromolecular substances, Biochemistry, Chromatography, Affinity, Substrate Specificity, Dephosphorylation, Myosin-Light-Chain Phosphatase, chemistry.chemical_compound, Adenosine Triphosphate, Ethers, Cyclic, Enzyme Stability, Okadaic Acid, Myosin, Phosphoprotein Phosphatases, medicine, Animals, Molecular Biology, Heavy meromyosin, Chemistry, Skeletal muscle, Muscle, Smooth, Cell Biology, Okadaic acid, Kinetics, medicine.anatomical_structure, Gizzard, Avian, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Myosin-light-chain phosphatase, Chickens, Phosphorus Radioisotopes

Abstract

Myosin light chain phosphatase associated with smooth muscle myosin (MAPP) was isolated from chicken gizzard. The MAPP was tightly associated with myosin and was not dissociated from myosin under the physiological ionic conditions. The phosphatase was dissociated from myosin in the presence of high MgCl2, i.e. 80 mM MgCl2. The binding site of the enzyme on the myosin molecule was the subfragment-2 region, since the enzyme did bind to the myosin rod and heavy meromyosin but not to the subfragment-1 affinity column. MAPP was purified with a heparin-Sepharose 6B column, and two activity peaks were obtained, i.e. MAPP I and MAPP II. The major activity peak, MAPP I, was further purified to homogeneity by thiophosphorylated myosin light chain-Sepharose 4B column chromatography. MAPP I was a tetramer composed of four 34-kDa subunits. The enzyme preferentially dephosphorylated the beta-subunit of phosphorylase kinase and was strongly inhibited by the heat- and acid-stable protein phosphatase inhibitor-1, whereas it was partially inhibited by the inhibitor-2. The IC50 (concentration of inhibitor giving 50% inhibition) value for the inhibition of the enzyme by okadaic acid was 70 nM which was about eight times higher than skeletal muscle type-1 and 390 times higher than type-2 protein phosphatase. These results demonstrate that the MAPP I is a type-1-like protein phosphatase, although the properties are not the same as type-I phosphatase. The properties of the myosin-associated phosphatase were distinct from the phosphatases reported previously, although some properties were similar to smooth muscle phosphatase-IV. Therefore, it is concluded that MAPP I is a novel smooth muscle protein phosphatase. Since it strongly associated with smooth muscle myosin, it is likely that MAPP I is responsible for the dephosphorylation of smooth muscle myosin in situ.

Published

1992

4. Phosphorylation sites linked to glial filament disassembly in vitro locate in a non-alpha-helical head domain

Author

C Sato, Kunimi Kikuchi, Yoshimi Nishi, S Ando, Kimiko Nishizawa, Kazushi Tanabe, Shigeru Tsuiki, S Kitamura, Y Gonda, and M Inagaki

Subjects

Glial fibrillary acidic protein, Akt/PKB signaling pathway, macromolecular substances, Cell Biology, Biology, Biochemistry, MAP2K7, Cell biology, nervous system, biology.protein, Phosphorylation, Protein kinase A, Intermediate filament, Molecular Biology, cGMP-dependent protein kinase, Protein kinase C

Abstract

Glial fibrillary acidic protein (GFAP), the intermediate filament component of astroglial cells, can serve as an excellent substrate for both cAMP-dependent protein kinase and protein kinase C, in vitro. GFAP phosphorylated by each protein kinase does not polymerize, and the filaments that do polymerize tend to depolymerize after phosphorylation. Dephosphorylation of phospho-GFAP by phosphatase led to a recovery of the polymerization competence of GFAP. Most of the phosphorylation sites for cAMP-dependent protein kinase and protein kinase C on GFAP are the same, Ser-8, Ser-13, and Ser-34. cAMP-dependent protein kinase has one additional phosphorylation site, Thr-7. All the sites are located within the amino-terminal non-alpha-helical head domain of GFAP. These observations pave the way for in vivo studies on organization of glial filaments.

Published

1990

5. Protein Kinase C Phosphorylation of Desmin at Four Serine Residues within the Non-α-Helical Head Domain

Author

S Kitamura, M Shibata, Kazushi Tanabe, C Sato, S Ando, and M Inagaki

Subjects

biology, MAP kinase kinase kinase, Cyclin-dependent kinase 2, macromolecular substances, Cell Biology, Mitogen-activated protein kinase kinase, Biochemistry, Molecular biology, MAP2K7, biology.protein, Protein phosphorylation, Cyclin-dependent kinase 9, c-Raf, Protein kinase A, Molecular Biology

Abstract

We reported that phosphorylation by either cAMP-dependent protein kinase or protein kinase C (Ca2+/phospholipid-dependent enzyme) in vitro induces disassembly of the desmin filaments (Inagaki, M., Gonda, Y., Matsuyama, M., Nishizawa, K., Nishi, Y., and Sato, C. (1988) J. Biol. Chem. 263, 5970-5978). For this subunit protein, Ser-29, Ser-35, and Ser-50 within the non-alpha-helical head domain were shown to be the sites of phosphorylation for cAMP-dependent protein kinase (Geisler, N., and Weber, K. (1988) EMBO J. 7, 15-20). In the present work, we identified the sites of desmin phosphorylated in vitro by other protein kinase which affects the filament structure. The protein kinase C-phosphorylated desmin was hydrolyzed with trypsin, and the phosphorylated peptides were isolated by reverse-phase chromatography. Sequential analysis of the purified phosphopeptides, together with the known primary sequence, revealed that Ser-12, Ser-29, Ser-38, and Ser-56 were phosphorylated by protein kinase C. All four sites are located within the non-alpha-helical head domain of desmin. Ser-12, Ser-38, and Ser-56, specifically phosphorylated by protein kinase C, have arginine residues at the carboxyl-terminal side (Arg-14, Arg-42, and Arg-59, respectively). Ser-29 phosphorylated by both protein kinase C and cAMP-dependent protein kinase has arginine residues at the amino and carboxyl termini (Arg-27 and Arg-33). These findings support the view that the head domain-specific phosphorylation strongly influences desmin filament structure; however, each protein kinase differed with regard to site recognition on this domain.

Published

1989

6. Correlation of conformation and phosphorylation and dephosphorylation of smooth muscle myosin

Author

M Inagaki, Mitsuo Ikebe, Hiroyoshi Hidaka, and M Naka

Subjects

inorganic chemicals, Meromyosin, Myosin light-chain kinase, Heavy meromyosin, Phosphatase, macromolecular substances, Cell Biology, Biology, Biochemistry, Dephosphorylation, Myosin, Biophysics, Phosphorylation, Myosin-light-chain phosphatase, Molecular Biology

Abstract

The rate of phosphorylation and dephosphorylation of smooth muscle myosin by myosin light chain kinase and by two myosin light chain phosphatases (gizzard phosphatase IV and aorta phosphatase) are measured in various conditions; the relationship between the rate of phosphorylation and dephosphorylation of myosin and the myosin conformation is also studied. The rate of dephosphorylation of myosin was completely inhibited in the presence of 1 mM MgCl2 and ATP at low ionic strength where phosphorylated myosin forms a folded conformation. The inhibition was released when myosin formed either an extended monomer or filaments. The rate of phosphorylation of myosin was also affected by the conformation of myosin. The rate for a folded myosin was slower than those for an extended monomer and filamentous myosin. The phosphorylation and dephosphorylation of heavy meromyosin, subfragment-1, and the isolated 20,000-dalton light chain are not inhibited at low ionic strength, and the rate of phosphorylation and dephosphorylation was decreased with increasing ionic strength. KCl dependence of the rate of phosphorylation and dephosphorylation of myosin was normalized by using KCl dependence of subfragment-1, and it was found that the marked inhibition of the rate of phosphorylation and dephosphorylation of myosin is closely related to the change from an extended to a folded conformation of myosin.

Published

1988

7. Ca2+-dependent deimination-induced disassembly of intermediate filaments involves specific modification of the amino-terminal head domain

Author

Kiyoshi Sugawara, Y Nishi, Hidenari Takahara, C Sato, and M Inagaki

Subjects

biology, Citrullination, Vimentin, macromolecular substances, Cell Biology, Biochemistry, Protein filament, chemistry.chemical_compound, chemistry, biology.protein, Citrulline, Protein-Arginine Deiminase Type-4, Intermediate Filament Protein, Desmin, Intermediate filament, Molecular Biology

Abstract

Peptidylarginine deiminase (proteinarginine iminohydrolase, EC 3.5.3.15) converted some arginine residues to citrulline residues in soluble vimentin, in a micromolar Ca2+-dependent manner and resulted in the loss of polymerization competence of the intermediate filament protein. When about 8 mol of residues/mol of vimentin were deiminated, there was a complete loss of filament forming ability. This enzyme also deiminated vimentin filaments which had been polymerized, and deimination of vimentin filaments resulted in filament disassembly. Similar results were obtained with other intermediate filaments such as desmin and glial filaments. High performance liquid chromatography and amino acid analyses of lysine-specific protease-generated fragments from deiminated vimentin (about 8 mol of citrulline/mol of vimentin) showed a differential deimination of three structural domains. The head domain was predominant. These observations suggest that the head domain strongly influences integrity of the intermediate filament.

Published

1989

8. Intermediate filament reconstitution in vitro. The role of phosphorylation on the assembly-disassembly of desmin

Author

M Inagaki, Mutsushi Matsuyama, Y Gonda, Yoshimi Nishi, C Sato, and Kimiko Nishizawa

Subjects

Vimentin, macromolecular substances, Cell Biology, Biology, musculoskeletal system, Biochemistry, Cell biology, chemistry.chemical_compound, chemistry, Phosphoserine, Phosphoprotein, biology.protein, Intermediate Filament Protein, Phosphorylation, Desmin, Intermediate filament, Molecular Biology, Protein kinase C

Abstract

Desmin, the myogenic intermediate filament protein, is a phosphoprotein containing phosphoserine, in vivo. The role of phosphorylation on assembly-disassembly and organization of the desmin filament has remained obscure. We report here on a stable and purified system which enables a biochemical examination of desmin filament assembly and disassembly. Using this in vitro system, we carried out stoichiometrical phosphorylations by purified protein kinases. The extent of polymerization-depolymerization was estimated using procedures related to centrifugation and electron microscopy. The evidence we obtained suggests that disassembly of the desmin filament and inhibition of the NaCl-dependent polymerization of the soluble desmin can reversibly occur with either cAMP-dependent or Ca2+-activated, phospholipid-dependent desmin phosphorylation.

Published

1988

9. Cytokinetic Failure-induced Tetraploidy Develops into Aneuploidy, Triggering Skin Aging in Phosphovimentin-deficient Mice.

Author

Tanaka H, Goto H, Inoko A, Makihara H, Enomoto A, Horimoto K, Matsuyama M, Kurita K, Izawa I, and Inagaki M

Subjects

Animals, Blotting, Western, Cell Cycle, Cell Proliferation, Cells, Cultured, Cyclin-Dependent Kinase Inhibitor p21 metabolism, Fibroblasts cytology, Fibroblasts metabolism, Fluorescent Antibody Technique, Immunoenzyme Techniques, Mice, Mice, Inbred C57BL, Mice, Knockout, Mitosis physiology, Phosphorylation, Subcutaneous Fat metabolism, Tumor Suppressor Protein p53 metabolism, Wound Healing, Aneuploidy, Cytokinesis, Skin Aging pathology, Subcutaneous Fat pathology, Tetraploidy, Vimentin physiology

Abstract

Tetraploidy, a state in which cells have doubled chromosomal sets, is observed in ∼20% of solid tumors and is considered to frequently precede aneuploidy in carcinogenesis. Tetraploidy is also detected during terminal differentiation and represents a hallmark of aging. Most tetraploid cultured cells are arrested by p53 stabilization. However, the fate of tetraploid cells in vivo remains largely unknown. Here, we analyze the ability to repair wounds in the skin of phosphovimentin-deficient (VIM(SA/SA)) mice. Early into wound healing, subcutaneous fibroblasts failed to undergo cytokinesis, resulting in binucleate tetraploidy. Accordingly, the mRNA level of p21 (a p53-responsive gene) was elevated in a VIM(SA/SA)-specific manner. Disappearance of tetraploidy coincided with an increase in aneuploidy. Thereafter, senescence-related markers were significantly elevated in VIM(SA/SA) mice. Because our tetraploidy-prone mouse model also exhibited subcutaneous fat loss at the age of 14 months, another premature aging phenotype, our data suggest that following cytokinetic failure, a subset of tetraploid cells enters a new cell cycle and develops into aneuploid cells in vivo, which promote premature aging., (© 2015 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2015

10. Defect of mitotic vimentin phosphorylation causes microophthalmia and cataract via aneuploidy and senescence in lens epithelial cells.

Author

Matsuyama M, Tanaka H, Inoko A, Goto H, Yonemura S, Kobori K, Hayashi Y, Kondo E, Itohara S, Izawa I, and Inagaki M

Subjects

Alleles, Amino Acid Sequence, Amino Acid Substitution, Animals, Cataract genetics, Cataract pathology, Cell Nucleus pathology, Endophthalmitis genetics, Endophthalmitis pathology, Epithelial Cells metabolism, Gene Knock-In Techniques, Lens, Crystalline pathology, Mice, Molecular Sequence Data, Phosphorylation, Vimentin chemistry, Vimentin genetics, Aneuploidy, Cataract etiology, Cataract metabolism, Cellular Senescence, Endophthalmitis etiology, Endophthalmitis metabolism, Epithelial Cells pathology, Mitosis, Vimentin metabolism

Abstract

Vimentin, a type III intermediate filament (IF) protein, is phosphorylated predominantly in mitosis. The expression of a phosphorylation-compromised vimentin mutant in T24 cultured cells leads to cytokinetic failure, resulting in binucleation (multinucleation). The physiological significance of intermediate filament phosphorylation during mitosis for organogenesis and tissue homeostasis was uncertain. Here, we generated knock-in mice expressing vimentin that have had the serine sites phosphorylated during mitosis substituted by alanine residues. Homozygotic mice (VIM(SA/SA)) presented with microophthalmia and cataracts in the lens, whereas heterozygotic mice (VIM(WT/SA)) were indistinguishable from WT (VIM(WT/WT)) mice. In VIM(SA/SA) mice, lens epithelial cell number was not only reduced but the cells also exhibited chromosomal instability, including binucleation and aneuploidy. Electron microscopy revealed fiber membranes that were disorganized in the lenses of VIM(SA/SA), reminiscent of similar characteristic changes seen in age-related cataracts. Because the mRNA level of the senescence (aging)-related gene was significantly elevated in samples from VIM(SA/SA), the lens phenotype suggests a possible causal relationship between chromosomal instability and premature aging.

Published

2013

11. TGF-β-activated kinase 1 (Tak1) mediates agonist-induced Smad activation and linker region phosphorylation in embryonic craniofacial neural crest-derived cells.

Author

Yumoto K, Thomas PS, Lane J, Matsuzaki K, Inagaki M, Ninomiya-Tsuji J, Scott GJ, Ray MK, Ishii M, Maxson R, Mishina Y, and Kaartinen V

Subjects

Amino Acid Motifs, Animals, Cells, Cultured, Cleft Palate enzymology, Cleft Palate genetics, Ectoderm cytology, Female, Gene Expression Regulation, Developmental, Head embryology, MAP Kinase Kinase Kinases deficiency, MAP Kinase Kinase Kinases genetics, Male, Mandible abnormalities, Mice, Mice, Transgenic, Mitogen-Activated Protein Kinases metabolism, Phosphorylation, Protein Serine-Threonine Kinases metabolism, Receptor, Transforming Growth Factor-beta Type I, Receptors, Transforming Growth Factor beta metabolism, Signal Transduction, Smad Proteins, Receptor-Regulated metabolism, TGF-beta Superfamily Proteins physiology, Wnt1 Protein genetics, Wnt1 Protein metabolism, MAP Kinase Kinase Kinases physiology, Neural Crest cytology, Protein Processing, Post-Translational, Smad Proteins metabolism

Abstract

Background: The role of Smad-independent TGF-β signaling in craniofacial development is poorly elucidated., Results: In craniofacial mesenchymal cells, Tak1 regulates both R-Smad C-terminal and linker region phosphorylation in TGF-β signaling., Conclusion: Tak1 plays an irreplaceable role in craniofacial ecto-mesenchyme during embryogenesis., Significance: Understanding the mechanisms of TGF-β signaling contributes to knowledge of pathogenetic mechanisms underlying common craniofacial birth defects. Although the importance of TGF-β superfamily signaling in craniofacial growth and patterning is well established, the precise details of its signaling mechanisms are still poorly understood. This is in part because of the concentration of studies on the role of the Smad-dependent (so-called "canonical") signaling pathways relative to the Smad-independent ones in many biological processes. Here, we have addressed the role of TGF-β-activated kinase 1 (Tak1, Map3k7), one of the key mediators of Smad-independent (noncanonical) TGF-β superfamily signaling in craniofacial development, by deleting Tak1 specifically in the neural crest lineage. Tak1-deficient mutants display a round skull, hypoplastic maxilla and mandible, and cleft palate resulting from a failure of palatal shelves to appropriately elevate and fuse. Our studies show that in neural crest-derived craniofacial ecto-mesenchymal cells, Tak1 is not only required for TGF-β- and bone morphogenetic protein-induced p38 Mapk activation but also plays a role in agonist-induced C-terminal and linker region phosphorylation of the receptor-mediated R-Smads. Specifically, we demonstrate that the agonist-induced linker region phosphorylation of Smad2 at Thr-220, which has been shown to be critical for full transcriptional activity of Smad2, is dependent on Tak1 activity and that in palatal mesenchymal cells TGFβRI and Tak1 kinases mediate both overlapping and distinct TGF-β2-induced transcriptional responses. To summarize, our results suggest that in neural crest-derived ecto-mesenchymal cells, Tak1 provides a critical point of intersection in a complex dialogue between the canonical and noncanonical arms of TGF-β superfamily signaling required for normal craniofacial development.

Published

2013

12. Evidence that formation of vimentin mitogen-activated protein kinase (MAPK) complex mediates mast cell activation following FcεRI/CC chemokine receptor 1 cross-talk.

Author

Toda M, Kuo CH, Borman SK, Richardson RM, Inoko A, Inagaki M, Collins A, Schneider K, and Ono SJ

Subjects

Animals, Cell Line, Cell Line, Tumor, Cells, Cultured, Chemokine CCL2 metabolism, Electrophoresis, Gel, Two-Dimensional, Enzyme-Linked Immunosorbent Assay, Humans, Imidazoles pharmacology, Immunoprecipitation, Mast Cells drug effects, Mice, Mice, Inbred BALB C, Mitogen-Activated Protein Kinase 1 metabolism, Mitogen-Activated Protein Kinase 3 metabolism, Mitogen-Activated Protein Kinases antagonists & inhibitors, Organic Chemicals pharmacology, Phosphorylation, Protein Binding, Pyridines pharmacology, Rats, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, p38 Mitogen-Activated Protein Kinases antagonists & inhibitors, p38 Mitogen-Activated Protein Kinases metabolism, Mast Cells metabolism, Mitogen-Activated Protein Kinases metabolism, Receptors, CCR1 metabolism, Receptors, IgG metabolism, Vimentin metabolism

Abstract

Accumulating evidence points to cross-talk between FcεRI and CC chemokine receptor (CCR)-mediated signaling pathways in mast cells. Here, we propose that vimentin, a protein comprising type III intermediate filament, participates in such cross-talk for CCL2/monocyte chemotactic protein 1 (MCP-1) production in mast cells, which is a mechanism for allergic inflammation. Co-stimulation via FcεRI, using IgE/antigen, and CCR1, using recombinant CCL3/macrophage inflammatory protein-1α (MIP-1α), increased expression of phosphorylated, disassembled, and soluble vimentin in rat basophilic leukemia (RBL)-2H3 cells expressing human CCR1 (RBL-CCR1 cells) and bone marrow-derived murine mast cells, both models of mucosal type mast cells. Furthermore, co-stimulation enhanced production of CCL2 as well as phosphorylation of MAPK. Treating the cells with p38 MAPK inhibitor SB203580, but not with MEK inhibitor PD98058, reduced CCL2 production, suggesting that p38 MAPK, but not ERK1/2, plays a critical role in the chemokine production. Immunoprecipitation analysis showed that vimentin interacts with phosphorylated ERK1/2 and p38 MAPKs in the co-simulated cells. Preventing disassembly of the vimentin by aggregating vimentin filaments using β,β'-iminodipropionitrile reduced the interaction of vimentin with phosphorylated MAPKs as well as CCL2 production in the cells. Taken together, disassembled vimentin interacting with phosphorylated p38 MAPK could mediate CCL2 production in mast cells upon FcεRI and CCR1 activation.

Published

2012

13. Withaferin A targets intermediate filaments glial fibrillary acidic protein and vimentin in a model of retinal gliosis.

Author

Bargagna-Mohan P, Paranthan RR, Hamza A, Dimova N, Trucchi B, Srinivasan C, Elliott GI, Zhan CG, Lau DL, Zhu H, Kasahara K, Inagaki M, Cambi F, and Mohan R

Subjects

Animals, Astrocytes cytology, Astrocytes drug effects, Astrocytes metabolism, Cell Cycle drug effects, Cells, Cultured, Cyclin D3 metabolism, Cyclin-Dependent Kinase Inhibitor p27 metabolism, Ergosterol chemistry, Ergosterol metabolism, Ergosterol pharmacology, Glial Fibrillary Acidic Protein genetics, Humans, Mice, Mice, Knockout, Models, Molecular, Protein Structure, Secondary, Recombinant Proteins genetics, Recombinant Proteins metabolism, Vimentin chemistry, Vimentin genetics, Withanolides, Ergosterol analogs & derivatives, Glial Fibrillary Acidic Protein metabolism, Gliosis metabolism, Gliosis pathology, Retina drug effects, Retina metabolism, Retina pathology, Retinal Degeneration metabolism, Retinal Degeneration pathology, Vimentin metabolism

Abstract

Gliosis is a biological process that occurs during injury repair in the central nervous system and is characterized by the overexpression of the intermediate filaments (IFs) glial fibrillary acidic protein (GFAP) and vimentin. A common thread in many retinal diseases is reactive Müller cell gliosis, an untreatable condition that leads to tissue scarring and even blindness. Here, we demonstrate that the vimentin-targeting small molecule withaferin A (WFA) is a novel chemical probe of GFAP. Using molecular modeling studies that build on the x-ray crystal structure of tetrameric vimentin rod 2B domain we reveal that the WFA binding site is conserved in the corresponding domain of tetrameric GFAP. Consequently, we demonstrate that WFA covalently binds soluble recombinant tetrameric human GFAP at cysteine 294. In cultured primary astrocytes, WFA binds to and down-regulates soluble vimentin and GFAP expression to cause cell cycle G(0)/G(1) arrest. Exploiting a chemical injury model that overexpresses vimentin and GFAP in retinal Müller glia, we demonstrate that systemic delivery of WFA down-regulates soluble vimentin and GFAP expression in mouse retinas. This pharmacological knockdown of soluble IFs results in the impairment of GFAP filament assembly and inhibition of cell proliferative response in Müller glia. We further show that a more severe GFAP filament assembly deficit manifests in vimentin-deficient mice, which is partly rescued by WFA. These findings illustrate WFA as a chemical probe of type III IFs and illuminate this class of withanolide as a potential treatment for diverse gliosis-dependent central nervous system traumatic injury conditions and diseases, and for orphan IF-dependent pathologies.

Published

2010

14. Novel positive feedback loop between Cdk1 and Chk1 in the nucleus during G2/M transition.

Author

Enomoto M, Goto H, Tomono Y, Kasahara K, Tsujimura K, Kiyono T, and Inagaki M

Subjects

Active Transport, Cell Nucleus, Cell Cycle, Cell Division, Checkpoint Kinase 1, Cyclin B1 metabolism, Cytoplasm metabolism, G2 Phase, HeLa Cells, Humans, Mitosis, Phosphorylation, Vimentin metabolism, CDC2 Protein Kinase metabolism, Cell Nucleus metabolism, Gene Expression Regulation, Protein Kinases metabolism

Abstract

Chk1, one of the critical transducers in DNA damage/replication checkpoints, prevents entry into mitosis through inhibition of Cdk1 activity. However, it has remained unclear how this inhibition is cancelled at the G(2)/M transition. We reported recently that Chk1 is phosphorylated at Ser(286) and Ser(301) by Cdk1 during mitosis. Here, we show that mitotic Chk1 phosphorylation is accompanied by Chk1 translocation from the nucleus to the cytoplasm in prophase. This translocation advanced in accordance with prophase progression and was regulated by Crm-1-dependent nuclear export. Exogenous Chk1 mutated at Ser(286) and Ser(301) to Ala (S286A/S301A) was observed mainly in the nuclei of prophase cells, although such nuclear accumulation was hardly observed in wild-type Chk1. Induction of S286A/S301A resulted in the delay of mitotic entry. Biochemical analyses using immunoprecipitated cyclin B(1)-Cdk1 complexes revealed S286A/S301A expression to block the adequate activation of Cdk1. In support of this, S286A/S301A expression retained Wee1 at higher levels and Cdk1-induced phosphorylation of cyclin B(1) and vimentin at lower levels. A kinase-dead version of S286A/S301A also localized predominantly in the nucleus but lost the ability to delay mitotic entry. These results indicate that Chk1 phosphorylation by Cdk1 participates in cytoplasmic sequestration of Chk1 activity, which releases Cdk1 inhibition in the nucleus and promotes mitotic entry.

Published

2009

15. TAK1-binding protein 1, TAB1, mediates osmotic stress-induced TAK1 activation but is dispensable for TAK1-mediated cytokine signaling.

Author

Inagaki M, Omori E, Kim JY, Komatsu Y, Scott G, Ray MK, Yamada G, Matsumoto K, Mishina Y, and Ninomiya-Tsuji J

Subjects

Adaptor Proteins, Signal Transducing genetics, Animals, Cell Line, Embryo, Mammalian cytology, Enzyme Activation physiology, Fibroblasts cytology, MAP Kinase Kinase Kinases genetics, Mice, Mice, Knockout, Osmotic Pressure physiology, Protein Structure, Tertiary physiology, Adaptor Proteins, Signal Transducing metabolism, Cytokines metabolism, Embryo, Mammalian metabolism, Fibroblasts metabolism, MAP Kinase Kinase Kinases metabolism, Signal Transduction physiology

Abstract

TAK1 kinase is an indispensable intermediate in several cytokine signaling pathways including tumor necrosis factor, interleukin-1, and transforming growth factor-beta signaling pathways. TAK1 also participates in stress-activated intracellular signaling pathways such as osmotic stress signaling pathway. TAK1-binding protein 1 (TAB1) is constitutively associated with TAK1 through its C-terminal region. Although TAB1 is known to augment TAK1 catalytic activity when it is overexpressed, the role of TAB1 under physiological conditions has not yet been identified. In this study, we determined the role of TAB1 in TAK1 signaling by analyzing TAB1-deficient mouse embryonic fibroblasts (MEFs). Tumor necrosis factor- and interleukin-1-induced activation of TAK1 was entirely normal in Tab1-deficient MEFs and could activate both mitogen-activated protein kinases and NF-kappaB. In contrast, we found that osmotic stress-induced activation of TAK1 was largely impaired in Tab1-deficient MEFs. Furthermore, we showed that the C-terminal 68 amino acids of TAB1 were sufficient to mediate osmotic stress-induced TAK1 activation. Finally, we attempted to determine the mechanism by which TAB1 activates TAK1. We found that TAK1 is spontaneously activated when the concentration is increased and that it is totally dependent on TAB1. Cell shrinkage under the osmotic stress condition increases the concentration of TAB1-TAK1 and may oligomerize and activate TAK1 in a TAB1-dependent manner. These results demonstrate that TAB1 mediates TAK1 activation only in a subset of TAK1 pathways that are mediated through spontaneous oligomerization of TAB1-TAK1.

Published

2008

16. Calcium/calmodulin-dependent protein kinase II (CaMKII) localization acts in concert with substrate targeting to create spatial restriction for phosphorylation.

Author

Tsui J, Inagaki M, and Schulman H

Subjects

Calcium-Calmodulin-Dependent Protein Kinase Type 2, Cell Line, Humans, Kinetics, Membrane Microdomains enzymology, Phosphorylation, Polymerase Chain Reaction, Protein Transport, Recombinant Fusion Proteins metabolism, Signal Transduction, Transfection, Calcium-Calmodulin-Dependent Protein Kinases metabolism

Abstract

Ca2+/calmodulin-dependent protein kinase II (CaMKII) acts in diverse cell types by phosphorylating proteins with key calcium-dependent functions such as synaptic plasticity, electrical excitability, and neurotransmitter synthesis. CaMKII displays calcium-dependent binding to proteins in vitro and translocation to synaptic sites after glutamatergic activity in neurons. We therefore hypothesized that subcellular targeting of CaMKII can direct its substrate specificity in an activity-dependent fashion. Here, we examined whether activity-dependent colocalization of CaMKII and its substrates could result in regulation of substrate phosphorylation in cells. We find that substrates localized at cellular membranes required CaMKII translocation to these compartments to achieve effective phosphorylation. Spatial barriers to phosphorylation could be overcome by translocation and anchoring to the substrate itself or to nearby target proteins within the membrane compartment. In contrast, phosphorylation of a cytoplasmic counterpart of the substrate does not require CaMKII translocation or stable protein-protein binding. Cytosolic phosphorylation is more permissive, exhibiting partial calcium-independence. Localization-dependent substrate specificity can also show more graded levels of regulation within signaling microdomains. We find that colocalization of translocated CaMKII and its substrate to lipid rafts in the plasma membrane can modulate the magnitude of phosphorylation. Thus, dynamic regulation of both substrate and kinase localization provides a powerful and nuanced way to regulate CaMKII signal specificity.

Published

2005

17. Biochemical and cell biological analyses of a mammalian septin complex, Sept7/9b/11.

Author

Nagata K, Asano T, Nozawa Y, and Inagaki M

Subjects

Animals, Blotting, Western, COS Cells, Cell Cycle Proteins chemistry, Cell Line, DNA, Complementary metabolism, Fibroblasts metabolism, GTP Phosphohydrolases chemistry, Glutathione Transferase metabolism, HeLa Cells, Humans, Immunoprecipitation, Microscopy, Fluorescence, Plasmids metabolism, Protein Binding, Protein Structure, Tertiary, Rats, Recombinant Proteins chemistry, Septins, Cell Cycle Proteins physiology, GTP Phosphohydrolases physiology

Abstract

Septins are members of a conserved family of cytoskeletal GTPases present in organisms as diverse as yeast and mammals. Unlike lower eukaryotic cells, the physiological significance of mammalian septin complexes is largely unknown. Using specific antibodies, we found at least five septins, Sept2, Sept7, Sept8, Sept9b, and Sept11, in septin complexes affinity-purified with anti-Sept7 antibody-conjugated column from rat embryonic fibroblast REF52 cells. Immunofluorescence studies revealed co-localization of Sept7, Sept9b, and Sept11 along stress fibers in REF52 cells. Biochemical and immunoprecipitation analyses revealed that the three septins directly bind with each other through their N- or C-terminal divergent regions. These septins per se formed distinct and characteristic filament structures when transiently expressed in COS7 cells. When two of the three septins were co-expressed in COS7 cells, combination-dependent filament elongation, bundling, or disruption was observed. Taken together, our results suggest that septin filament structures may be affected by interactions with other septins included in the complex.

Published

2004

18. Unique catabolic pathway of glycosphingolipids in a hydrozoan, Hydra magnipapillata, involving endoglycoceramidase.

Author

Horibata Y, Sakaguchi K, Okino N, Iida H, Inagaki M, Fujisawa T, Hama Y, and Ito M

Subjects

Amino Acid Sequence, Animals, Base Sequence, CHO Cells, Ceramides metabolism, Cloning, Molecular, Cricetinae, G(M1) Ganglioside metabolism, Glycoside Hydrolases chemistry, Glycoside Hydrolases genetics, Hydrogen-Ion Concentration, Immunohistochemistry, In Situ Hybridization, Molecular Sequence Data, Oligosaccharides metabolism, Sequence Alignment, Transfection, Glycoside Hydrolases metabolism, Glycosphingolipids metabolism, Hydra enzymology

Abstract

Endoglycoceramidase (EGCase; EC 3.2.1.123) is an enzyme capable of cleaving the glycosidic linkage between oligosaccharides and ceramides of various glycosphingolipids. We detected strong EGCase activity in animals belonging to Cnidaria, Mollusca, and Annelida and cloned the enzyme from a hydra, Hydra magnipapillata. The hydra EGCase, consisting of 517 amino acid residues, showed 19.2% and 50.2% identity to the Rhodcoccus and jellyfish EGCases, respectively. The recombinant hydra enzyme, expressed in CHOP (Chinese hamster ovary cells expressing polyoma LT antigen) cells, hydrolyzed [14C]GM1a to produce [14C]ceramide with a pH optimum at 3.0-3.5. Whole mount in situ hybridization and immunocytochemical analysis revealed that EGCase was widely expressed in the endodermal layer, especially in digestive cells. GM1a injected into the gastric cavity was incorporated and then directly catabolized by EGCase to produce GM1a-oligosaccharide and ceramide, which were further degraded by exoglycosidases and ceramidase, respectively. However, hydra exoglycosidases did not hydrolyze GM1a directly. These results indicate that the EGCase is indispensable for the catabolic processing of dietary glycosphingolipids in hydra, demonstrating the unique catabolic pathway for glyosphingolipids in the animal.

Published

2004

19. Autophosphorylation of a newly identified site of Aurora-B is indispensable for cytokinesis.

Author

Yasui Y, Urano T, Kawajiri A, Nagata K, Tatsuka M, Saya H, Furukawa K, Takahashi T, Izawa I, and Inagaki M

Subjects

Alanine chemistry, Amino Acid Sequence, Animals, Aurora Kinase B, Aurora Kinases, Binding Sites, COS Cells, Cell Division, Cell Nucleus metabolism, Chromosomes ultrastructure, HeLa Cells, Histones chemistry, Humans, Mass Spectrometry, Microscopy, Fluorescence, Mitosis, Molecular Sequence Data, Mutation, Phosphorylation, Plasmids metabolism, Protein Binding, Sequence Homology, Amino Acid, Threonine chemistry, Time Factors, Transfection, Vimentin chemistry, Protein Serine-Threonine Kinases chemistry

Abstract

Mitotic kinases regulate cell division and its checkpoints, errors of which can lead to aneuploidy or genetic instability. One of these is Aurora-B, a key kinase that is required for chromosome alignment at the metaphase plate and for cytokinesis in mammalian cells. We report here that human Aurora-B is phosphorylated at Thr-232 through interaction with the inner centromere protein (INCENP) in vivo. The phosphorylation of Thr-232 occurs by means of an autophosphorylation mechanism, which is indispensable for the Aurora-B kinase activity. The activation of Aurora-B spatio-temporally correlated with the site-specific phosphorylation of its physiological substrates, histone H3 and vimentin. Overexpression of the TA mutant of Aurora-B, in which Thr-232 was changed into alanine, frequently induced multinuclearity in cells. These results indicate that the phosphorylation of Thr-232 is an essential regulatory mechanism for Aurora-B activation.

Published

2004

20. Cohesin-dockerin interactions within and between Clostridium josui and Clostridium thermocellum: binding selectivity between cognate dockerin and cohesin domains and species specificity.

Author

Jindou S, Soda A, Karita S, Kajino T, Béguin P, Wu JH, Inagaki M, Kimura T, Sakka K, and Ohmiya K

Subjects

Amino Acid Sequence, Bacterial Proteins metabolism, Cell Cycle Proteins, Cellulase metabolism, Chromosomal Proteins, Non-Histone, Electrophoresis, Polyacrylamide Gel, Escherichia coli metabolism, Fungal Proteins, Kinetics, Membrane Proteins metabolism, Molecular Sequence Data, Nuclear Proteins metabolism, Peptides chemistry, Plasmids metabolism, Protein Binding, Protein Structure, Tertiary, Recombinant Proteins chemistry, Sequence Homology, Amino Acid, Species Specificity, Substrate Specificity, Surface Plasmon Resonance, Time Factors, Cohesins, Bacterial Proteins chemistry, Cellulase chemistry, Clostridium metabolism, Membrane Proteins chemistry, Nuclear Proteins chemistry

Abstract

The cellulosome components are assembled into the cellulosome complex by the interaction between one of the repeated cohesin domains of a scaffolding protein and the dockerin domain of an enzyme component. We prepared five recombinant cohesin polypeptides of the Clostridium thermocellum scaffolding protein CipA, two dockerin polypeptides of C. thermocellum Xyn11A and Xyn10C, four cohesin polypeptides of Clostridium josui CipA, and two dockerin polypeptides of C. josui Aga27A and Cel8A, and qualitatively and quantitatively examined the cohesin-dockerin interactions within C. thermocellum and C. josui, respectively, and the species specificity of the cohesin-dockerin interactions between these two bacteria. Surface plasmon resonance (SPR) analysis indicated that there was a certain selectivity, with a maximal 34-fold difference in the K(D) values, in the cohesin-dockerin interactions within a combination of C. josui, although this was not detected by qualitative analysis. Affinity blotting analysis suggested that there was at least one exception to the species specificity in the cohesin-dockerin interactions, although species specificity was generally conserved among the cohesin and dockerin polypeptides from C. thermocellum and C. josui, i.e. the dockerin polypeptides of C. thermocellum Xyn11A exceptionally bound to the cohesin polypeptides from C. josui CipA. SPR analysis confirmed this exceptional binding. We discuss the relationship between the species specificity of the cohesin-dockerin binding and the conserved amino acid residues in the dockerin domains.

Published

2004

21. An autocrine/paracrine loop linking keratin 14 aggregates to tumor necrosis factor alpha-mediated cytotoxicity in a keratinocyte model of epidermolysis bullosa simplex.

Author

Yoneda K, Furukawa T, Zheng YJ, Momoi T, Izawa I, Inagaki M, Manabe M, and Inagaki N

Subjects

Annexin A5 pharmacology, Apoptosis, Carrier Proteins metabolism, Caspases metabolism, Cell Line, Coloring Agents pharmacology, Cysteine Endopeptidases metabolism, Disease Models, Animal, Endoplasmic Reticulum Chaperone BiP, Humans, Immunoblotting, In Situ Nick-End Labeling, Keratin-14, Microscopy, Fluorescence, Molecular Chaperones metabolism, Multienzyme Complexes metabolism, Mutation, Phosphorylation, Plasmids metabolism, Proteasome Endopeptidase Complex, Protein Binding, Protein Folding, Proteins metabolism, TNF Receptor-Associated Factor 1, Transfection, Tumor Necrosis Factor-alpha metabolism, Up-Regulation, Epidermolysis Bullosa Simplex metabolism, Heat-Shock Proteins, Keratinocytes metabolism, Keratins chemistry, Proteins physiology, Tumor Necrosis Factor-alpha chemistry

Abstract

Epidermolysis bullosa simplex (EBS) is a blistering cutaneous disease featuring protein aggregates. Here we investigate the molecular mechanisms linking protein aggregates to cell death in a cellular model of EBS in which HaCaT keratinocytes are transfected with plasmids expressing various mutant forms of keratin 14 (K14). In HaCaT cells, mutant K14 was found to form ubiquitinated protein aggregates that suppressed 20 S proteasome function instead of being degraded by 20 S proteasome. Keratinocytes with mutant K14-induced phosphorylation of the stress-activated kinase c-Jun, as well as up-regulation of unfolding protein Bip, indicates induction of endoplasmic reticulum stress. HaCaT cells were susceptible to apoptosis by activation of caspases-3, and -8, but not caspase-9 or -12. Tumor necrosis factor-alpha (TNFalpha) in the culture medium was increased in keratinocytes with mutant K14 compared with wild K14, and the addition of neutralizing anti-TNFalpha antibody to the culture medium rescued keratinocytes from cell death. Thus, TNFalpha release and the subsequent activation of the TNFalpha receptor by an autocrine/paracrine pathway links protein aggregates to cell death in this keratinocyte EBS cellular model. Furthermore, mutation in K14 reduced its affinity to TNFalpha receptor-associated death domain (TRADD), suggesting that the susceptibility of keratinocytes to caspase-8-mediated apoptosis is increased in mutated K14 because of impairment of the cytoprotective mechanism mediated by K14-TRADD interaction.

Published

2004

22. Filament formation of MSF-A, a mammalian septin, in human mammary epithelial cells depends on interactions with microtubules.

Author

Nagata K, Kawajiri A, Matsui S, Takagishi M, Shiromizu T, Saitoh N, Izawa I, Kiyono T, Itoh TJ, Hotani H, and Inagaki M

Subjects

Amino Acid Motifs, Animals, COS Cells, Cell Line, Cells, Cultured, Cytochalasin B pharmacology, Cytoplasm metabolism, Cytoskeletal Proteins metabolism, Demecolcine pharmacology, GTP Phosphohydrolases metabolism, GTP-Binding Proteins metabolism, HeLa Cells, Humans, Microscopy, Fluorescence, Microtubules metabolism, Mitosis, Mutation, Plasmids metabolism, Protein Binding, RNA Interference, Recombinant Proteins metabolism, Reverse Transcriptase Polymerase Chain Reaction, Transfection, Tubulin chemistry, Breast metabolism, Cytoskeletal Proteins chemistry, Epithelial Cells metabolism, GTP-Binding Proteins chemistry

Abstract

Septins are a family of conserved proteins implicated in a variety of cellular functions such as cytokinesis and vesicle trafficking, but their properties and modes of action are largely unknown. Here we now report findings of immunocytochemical and biochemical characterization of a mammalian septin, MSF-A. Using an antibody specific for MSF subfamily proteins, MSF-A was found to be expressed predominantly in mammary human mammary epithelial cells (HMEC). MSF-A was associated with microtubules in interphase HMEC cells as it localized with the mitotic spindle and the bundle of microtubule at midzone during mitosis. Biochemical analysis revealed direct binding of MSF-A with polymerized tubulin through its central region containing guanine nucleotide-interactive motifs. GTPase activity, however, was not required for the association. Conditions that disrupt the microtubule network also disrupted the MSF-A-containing filament structure, resulting in a punctate cytoplasmic pattern. Depletion of MSF-A using small interfering RNAs caused incomplete cell division and resulted in the accumulation of binucleated cells. Unlike Nedd5, an MSF mutant deficient in GTPase activity forms filament indistinguishable from that of the wild type in COS cells. These results strongly suggest that septin filaments may interact not only with actin filaments but also with microtubule networks and that GTPase activity of MSF-A is not indispensable to incorporation of MSF-A into septin filaments.

Published

2003

23. Aurora-B regulates the cleavage furrow-specific vimentin phosphorylation in the cytokinetic process.

Author

Goto H, Yasui Y, Kawajiri A, Nigg EA, Terada Y, Tatsuka M, Nagata K, and Inagaki M

Subjects

Amino Acid Sequence, Animals, Aurora Kinase B, Aurora Kinases, Mice, Molecular Sequence Data, Phosphorylation, Recombinant Proteins metabolism, Vimentin chemistry, Cell Cycle, Protein Serine-Threonine Kinases metabolism, Vimentin metabolism

Abstract

Aurora-B is an evolutionally conserved protein kinase that regulates several mitotic events including cytokinesis. We previously demonstrated the possible existence of a protein kinase that phosphorylates at least Ser-72 on vimentin, the most widely expressed intermediate filament protein, in the cleavage furrow-specific manner. Here we showed that vimentin-Ser-72 phosphorylation occurred specifically at the border of the Aurora-B-localized area from anaphase to telophase. Expression of a dominant-negative mutant of Aurora-B led to a reduction of this vimentin-Ser-72 phosphorylation. In vitro analyses revealed that Aurora-B phosphorylates vimentin at approximately 2 mol phosphate/mol of substrate for 30 min and that this phosphorylation dramatically inhibits vimentin filament formation. We further identified eight Aurora-B phosphorylation sites, including Ser-72 on vimentin, and then constructed the mutant vimentin in which these identified sites are changed into Ala. Cells expressing this mutant formed an unusually long bridge-like intermediate filament structure between unseparated daughter cells. We then identified important phosphorylation sites for the bridge phenotype. Our findings indicate that Aurora-B regulates the cleavage furrow-specific vimentin phosphorylation and controls vimentin filament segregation in cytokinetic process.

Published

2003

24. Expression of L-histidine decarboxylase in mouse male germ cells.

Author

Safina F, Tanaka S, Inagaki M, Tsuboi K, Sugimoto Y, and Ichikawa A

Subjects

Acrosome Reaction, Animals, Blotting, Northern, Calcimycin pharmacology, Epididymis enzymology, Histidine Decarboxylase metabolism, Immunoblotting, Immunohistochemistry, Ionophores pharmacology, Male, Mice, Mice, Inbred ICR, RNA, Messenger metabolism, Reverse Transcriptase Polymerase Chain Reaction, Testis enzymology, Testis metabolism, Histidine Decarboxylase biosynthesis, Spermatids enzymology, Spermatozoa enzymology

Abstract

Histamine synthesis in male reproductive tissues remains largely unknown. The interaction between stem cell factor and its receptor, c-Kit, has been found to be essential for the maturation of male germ cells and peripheral mast cells. Based on this analogy, we investigated the expression of histidine decarboxylase (HDC), the rate-limiting enzyme of histamine synthesis, in mouse male germ cells. Immunohistochemical analyses revealed that HDC is localized in the acrosomes of spermatids and spermatozoa. In the testis, epididymis, and spermatozoa, a significant amount of histamine and HDC activity were detected. W/W(V) mice, known to lack most of their germ cells in the seminiferous tubules, were found to lack HDC protein expression as well as HDC activity in the testis. An in vitro acrosome reaction induced by a calcium ionophore, caused the release of histamine from epididymal spermatozoa. Our observations indicate that histamine is produced in and released from the acrosomes.

Published

2002

25. Densin-180 interacts with delta-catenin/neural plakophilin-related armadillo repeat protein at synapses.

Author

Izawa I, Nishizawa M, Ohtakara K, and Inagaki M

Subjects

Animals, Armadillo Domain Proteins, Biotinylation, Brain metabolism, Cadherins metabolism, Catenins, Cell Adhesion Molecules, Cell Membrane metabolism, Cells, Cultured, Cloning, Molecular, Cytoskeletal Proteins chemistry, Cytosol metabolism, DNA, Complementary metabolism, Gene Library, Hippocampus cytology, Hippocampus metabolism, Humans, Immunoblotting, Microscopy, Fluorescence, Molecular Sequence Data, Nerve Tissue Proteins metabolism, Neurons metabolism, Phosphoproteins, Precipitin Tests, Protein Binding, Protein Biosynthesis, Protein Structure, Tertiary, Rats, Recombinant Fusion Proteins metabolism, Recombinant Proteins metabolism, Synapses metabolism, Transfection, Two-Hybrid System Techniques, Delta Catenin, Cytoskeletal Proteins metabolism, Nerve Tissue Proteins chemistry, Sialoglycoproteins chemistry, Sialoglycoproteins metabolism

Abstract

Densin-180, a protein purified from the postsynaptic density fraction of the rat forebrain, is the founding member of a newly described family of proteins termed the LAP (leucine-rich repeats and PSD-95/Dlg-A/ZO-1 (PDZ) domains) family that plays essential roles in establishment of cell polarity. To identify Densin-180-binding proteins, we screened a yeast two-hybrid library using the carboxyl-terminal fragment of Densin-180 containing PDZ domain as bait, and we isolated delta-catenin/neural plakophilin-related armadillo repeat protein (NPRAP) as a Densin-180-interacting protein. delta-catenin/NPRAP, a member of the armadillo repeat family, is a nervous system-specific adherens junction protein originally discovered as an interactor with presenilin-1, a protein involved in Alzheimer's disease. Densin-180 PDZ domain binds the COOH terminus of delta-catenin/NPRAP containing the PDZ domain-binding sequence. Endogenous Densin-180 was co-immunoprecipitated with delta-catenin/NPRAP and N-cadherin. Although Densin-180 was reported to be a transmembrane protein, Densin-180 was not accessible to surface biotinylation in dissociated hippocampal neurons; hence Densin-180 may be a cytosolic protein. Densin-180 co-localized with delta-catenin/NPRAP at synapses in delta-catenin/NPRAP and may be involved in organization of the synaptic cell-cell junction through interaction with the delta-catenin/NPRAP-N-cadherin complex.

Published

2002

26. Ultraviolet B-induced phosphorylation of histone H3 at serine 28 is mediated by MSK1.

Author

Zhong S, Jansen C, She QB, Goto H, Inagaki M, Bode AM, Ma WY, and Dong Z

Subjects

Animals, Cell Line, Chromatin metabolism, Chromatin radiation effects, Enzyme Activation, Enzyme Inhibitors pharmacology, Epidermis, Histones chemistry, Isoquinolines pharmacology, Mice, Nucleosomes drug effects, Nucleosomes metabolism, Nucleosomes radiation effects, Phosphorylation, Proto-Oncogene Proteins metabolism, Proto-Oncogene Proteins c-akt, Recombinant Proteins metabolism, Ribosomal Protein S6 Kinases metabolism, Ribosomal Protein S6 Kinases radiation effects, Transfection, Calcium-Calmodulin-Dependent Protein Kinases metabolism, Histones metabolism, Histones radiation effects, Protein Serine-Threonine Kinases, Ribosomal Protein S6 Kinases, 90-kDa, Serine, Sulfonamides, Ultraviolet Rays

Abstract

N-terminal tail phosphorylation of histone H3 plays an important role in gene expression, chromatin remodeling, and chromosome condensation. Phosphorylation of histone H3 at serine 10 was shown to be mediated by RSK2, mitogen- and stress-activated protein kinase-1 (MSK1), and mitogen-activated protein kinases depending on the specific stimulation or stress. Our previous study showed that mitogen-activated protein kinases MAP kinases are involved in ultraviolet B-induced phosphorylation of histone H3 at serine 28 (Zhong, S., Zhong, Z., Jansen, J., Goto, H., Inagaki, M., and Dong, Z., J. Biol. Chem. 276, 12932-12937). However, downstream effectors of MAP kinases remain to be identified. Here, we report that H89, a selective inhibitor of the nucleosomal response, totally inhibits ultraviolet B-induced phosphorylation of histone H3 at serine 28. H89 blocks MSK1 activity but does not inhibit ultraviolet B-induced activation of MAP kinases p70/85(S6K), p90(RSK), Akt, and protein kinase A. Furthermore, MSK1 markedly phosphorylated serine 28 of histone H3 and chromatin in vitro. Transfection experiments showed that an N-terminal mutant MSK1 or a C-terminal mutant MSK1 markedly blocked MSK1 activity. Compared with wild-type MSK1, cells transfected with N-terminal or C-terminal mutant MSK1 strongly blocked ultraviolet B-induced phosphorylation of histone H3 at serine 28 in vivo. These data illustrate that MSK1 mediates ultraviolet B-induced phosphorylation of histone H3 at serine 28.

Published

2001

27. MAP kinases mediate UVB-induced phosphorylation of histone H3 at serine 28.

Author

Zhong S, Zhang Y, Jansen C, Goto H, Inagaki M, and Dong Z

Subjects

Animals, Cell Line, Chromatin metabolism, Chromatin radiation effects, Enzyme Inhibitors pharmacology, Flavonoids pharmacology, Histones chemistry, MAP Kinase Kinase 1, Mitogen-Activated Protein Kinase 1 metabolism, Mitogen-Activated Protein Kinase 3, Mitogen-Activated Protein Kinase 8, Mitogen-Activated Protein Kinase 9, Mitogen-Activated Protein Kinase Kinases metabolism, Phosphorylation, Protein Serine-Threonine Kinases metabolism, p38 Mitogen-Activated Protein Kinases, Histones metabolism, Histones radiation effects, Mitogen-Activated Protein Kinases metabolism, Serine

Abstract

Histone H3 phosphorylation is related closely to chromatin remodeling and chromosome condensation. H3 phosphorylation at serine 28 is coupled with mitotic chromosome condensation in diverse mammalian cell lines. However, the pathway that mediates phosphorylation of H3 at serine 28 is unknown. In the present study, ERK1, ERK2, or p38 kinase strongly phosphorylated H3 at serine 28 in vitro. JNK1 or JNK2 was able also to phosphorylate H3 at serine 28 in vitro but to a lesser degree. UVB irradiation markedly induced phosphorylation of H3 at serine 28 in JB6 Cl 41 cells. PD 98059, a MEK1 inhibitor, and SB 202190, a p38 kinase inhibitor, efficiently repressed UVB-induced H3 phosphorylation at serine 28. Expression of dominant negative mutant (DNM) ERK2 in JB6 Cl 41 cells totally blocked UVB-induced phosphorylation of H3 at serine 28. Additionally, DNM p38 kinase or DNM JNK1 partially blocked UVB-induced H3 phosphorylation at serine 28. Furthermore, UVB-induced H3 phosphorylation at serine 28 was inhibited in Jnk1(-/-) cells but not in Jnk2(-/-) cells. These results suggest that UVB-induced H3 phosphorylation at serine 28 may be mediated by mitogen-activated protein kinases.

Published

2001

28. Identification of Mrj, a DnaJ/Hsp40 family protein, as a keratin 8/18 filament regulatory protein.

Author

Izawa I, Nishizawa M, Ohtakara K, Ohtsuka K, Inada H, and Inagaki M

Subjects

Antibodies immunology, DNA, Complementary, HSP40 Heat-Shock Proteins, HeLa Cells, Humans, Keratins genetics, Microinjections, Molecular Chaperones genetics, Molecular Chaperones immunology, Sequence Deletion, Intermediate Filaments metabolism, Keratins metabolism, Molecular Chaperones metabolism, Nerve Tissue Proteins

Abstract

To elucidate the function of keratins 8 and 18 (K8/18), major components of the intermediate filaments of simple epithelia, we searched for K8/18-binding proteins by screening a yeast two-hybrid library. We report here that human Mrj, a DnaJ/Hsp40 family protein, directly binds to K18. Among the interactions between DnaJ/Hsp40 family proteins and various intermediate filament proteins that we tested using two-hybrid methods, Mrj specifically interacted with K18. Immunostaining with anti-Mrj antibody showed that Mrj colocalized with K8/18 filaments in HeLa cells. Mrj was immunoprecipitated not only with K18, but also with the stress-induced and constitutively expressed heat shock protein Hsp/c70. Mrj bound to K18 through its C terminus and interacted with Hsp/c70 via its N terminus, which contains the J domain. Microinjection of anti-Mrj antibody resulted in the disorganization of K8/18 filaments, without effects on the organization of actin filaments and microtubules. Taken together, these results suggest that Mrj may play an important role in the regulation of K8/18 filament organization as a K18-specific co-chaperone working together with Hsp/c70.

Published

2000

29. Functions of a rho-specific guanine nucleotide exchange factor in neurite retraction. Possible role of a proline-rich motif of KIAA0380 in localization.

Author

Togashi H, Nagata K, Takagishi M, Saitoh N, and Inagaki M

Subjects

Animals, Cell Line, Growth Cones physiology, Intracellular Signaling Peptides and Proteins, Mice, Neurons cytology, Neurons physiology, rho-Associated Kinases, Guanine Nucleotide Exchange Factors physiology, Neurites physiology, Protein Serine-Threonine Kinases physiology, Signal Transduction physiology, rho GTP-Binding Proteins physiology

Abstract

The Rho/Rho kinase signaling pathway plays an essential role in neurite retraction and cell rounding in response to G(12/13)-coupled receptor activation in neuronal cells. The Rho guanine nucleotide exchange factor involved in these processes has not been identified. To monitor the activation state of Rho kinase, we developed a vimentin head/Rho kinase chimera, which is intramolecularly phosphorylated in a Rho-dependent manner at Ser(71) of the fused vimentin head. Using this system, we identified a clone termed KIAA0380, which contains the G alpha(12/13)-binding domain as well as a tandem of the Dbl homology/pleckstrin homology (DH/PH) domain, as an activator of Rho/Rho kinase signaling. Molecular dissection analyses revealed that a proline-rich motif C-terminally adjacent to DH/PH domain is essential for plasma membrane localization of KIAA0380 and cortical actin reorganization followed by cell rounding. In contrast, the DH/PH domain of KIAA0380 is localized in the cytoplasm, where it activates Rho/Rho kinase and induces stress fiber formation, consistent with results using p115 Rho guanine nucleotide exchange factor, which has a similar structure to KIAA0380 but lacks a proline-rich motif. These results suggest that upon stimulation, KIAA0380 translocates to the plasma membrane via the proline-rich motif and there activates Rho/Rho kinase signaling. In neuroblastoma Neuro2a cells, KIAA0380 was observed in the tips of neurites, a location where cortical actin reorganization is induced upon stimulation with lysophosphatidic acid. Ectopic expression of the N-terminal fragment inhibited lysophosphatidic acid-induced neurite retraction of Neuro2a cells. These results suggest that KIAA0380 plays an important role in neurite retraction through Rho-dependent signaling.

Published

2000

30. Activation of Ca2+/calmodulin-dependent protein kinase II within post-synaptic dendritic spines of cultured hippocampal neurons.

Author

Inagaki N, Nishizawa M, Arimura N, Yamamoto H, Takeuchi Y, Miyamoto E, Kaibuchi K, and Inagaki M

Subjects

Amino Acid Sequence, Animals, Base Sequence, Calcium-Calmodulin-Dependent Protein Kinase Type 2, Cells, Cultured, DNA Primers, Enzyme Activation, Hippocampus cytology, Molecular Sequence Data, Organelles enzymology, Rats, Calcium-Calmodulin-Dependent Protein Kinases metabolism, Dendrites enzymology, Hippocampus enzymology, Synapses enzymology

Abstract

To understand the cell signaling of protein kinases, it is essential to monitor their activity in each of the subcellular compartments. Here we developed a method to visualize the activities of Ca(2+)/calmodulin-dependent protein kinase II (CaMKII) in the cytoplasm, plasma membrane, and nucleus, separately, by utilizing targeted phosphorylation motifs and phosphorylation-specific antibodies. This approach was used to monitor the activities of post-synaptic CaMKII in cultured hippocampal neurons. Strong stimulation of the neurons by N-methyl-d-aspartate led to global activations of CaMKII in the cell bodies and dendrites. On the other hand, weak stimulation by removal of Mg(2+) block of N-methyl-d-aspartate receptors induced CaMKII signaling localized within single dendritic spines. Post-synaptic CaMKII is thought to modify synaptic efficiency. The present data for the first time demonstrate the activation of CaMKII localized within single dendritic spines and are consistent with the notion that synaptic efficiency is modified by CaMKII in single or multiple spine level depending on the strength of receptor activation.

Published

2000

31. Identification of a novel phosphorylation site on histone H3 coupled with mitotic chromosome condensation.

Author

Goto H, Tomono Y, Ajiro K, Kosako H, Fujita M, Sakurai M, Okawa K, Iwamatsu A, Okigaki T, Takahashi T, and Inagaki M

Subjects

Amino Acid Sequence, Animals, Chromosomes ultrastructure, DNA Mutational Analysis, Histones genetics, Molecular Sequence Data, Phosphorylation, Rats, Tetrahymena, Chromosomes metabolism, Histones metabolism, Mitosis

Abstract

Histone H3 (H3) phosphorylation at Ser(10) occurs during mitosis in eukaryotes and was recently shown to play an important role in chromosome condensation in Tetrahymena. When producing monoclonal antibodies that recognize glial fibrillary acidic protein phosphorylation at Thr(7), we obtained some monoclonal antibodies that cross-reacted with early mitotic chromosomes. They reacted with 15-kDa phosphoprotein specifically in mitotic cell lysate. With microsequencing, this phosphoprotein was proved to be H3. Mutational analysis revealed that they recognized H3 Ser(28) phosphorylation. Then we produced a monoclonal antibody, HTA28, using a phosphopeptide corresponding to phosphorylated H3 Ser(28). This antibody specifically recognized the phosphorylation of H3 Ser(28) but not that of glial fibrillary acidic protein Thr(7). Immunocytochemical studies with HTA28 revealed that Ser(28) phosphorylation occurred in chromosomes predominantly during early mitosis and coincided with the initiation of mitotic chromosome condensation. Biochemical analyses using (32)P-labeled mitotic cells also confirmed that H3 is phosphorylated at Ser(28) during early mitosis. In addition, we found that H3 is phosphorylated at Ser(28) as well as Ser(10) when premature chromosome condensation was induced in tsBN2 cells. These observations suggest that H3 phosphorylation at Ser(28), together with Ser(10), is a conserved event and is likely to be involved in mitotic chromosome condensation.

Published

1999

32. Cell cycle regulation of human CDC6 protein. Intracellular localization, interaction with the human mcm complex, and CDC2 kinase-mediated hyperphosphorylation.

Author

Fujita M, Yamada C, Goto H, Yokoyama N, Kuzushima K, Inagaki M, and Tsurumi T

Subjects

Chromatin metabolism, HeLa Cells, Humans, Minichromosome Maintenance Complex Component 7, Phosphorylation, Precipitin Tests, Cell Cycle, Cell Cycle Proteins metabolism, DNA-Binding Proteins metabolism, Nuclear Proteins metabolism, Saccharomyces cerevisiae Proteins

Abstract

The binding of mammalian MCM complexes to chromatin is cell cycle-regulated and under CDC2 kinase negative control. Here, we investigated the properties of mammalian CDC6 protein, a candidate regulator of MCM. The levels of CDC6 were relatively constant during the HeLa cell cycle. In asynchronous cells, CDC6 was mainly detected in the nuclei with immunostaining, but some CDC6 was not extractable with nonionic detergent. In contrast to the chromatin-bound MCM, this fraction of CDC6 was resistant to DNase I treatment, suggesting that it binds to the detergent- and nuclease-resistant nuclear structure. In S phase cells, CDC6 became detectable in the cytoplasm with immunostaining; however, the level of the bound CDC6 was unchanged. In G(2)/M phase cells, the level of the bound CDC6 was still maintained, which was hyperphosphorylated by CDC2 kinase. These data suggest that some CDC6 protein is associated with the specific nuclear structure throughout the cell cycle and that major binding sites on chromatin differ between MCM and CDC6. However, co-immunoprecipitation assays with chemical cross-linking indicated that a small part of the chromatin-bound MCM is present close to the bound CDC6.

Published

1999

33. Cell cycle- and chromatin binding state-dependent phosphorylation of human MCM heterohexameric complexes. A role for cdc2 kinase.

Author

Fujita M, Yamada C, Tsurumi T, Hanaoka F, Matsuzawa K, and Inagaki M

Subjects

Biopolymers, Cyclin B metabolism, HeLa Cells, Humans, Phosphorylation, Protein Binding, CDC2 Protein Kinase metabolism, Cell Cycle, Cell Cycle Proteins metabolism, Chromatin metabolism, Nuclear Proteins metabolism

Abstract

The mammalian MCM protein family, presently with six members, exists in the nuclei in two forms, chromatin-bound and unbound. The former dissociates from chromatin with progression through the S phase. Recently, we have established a procedure to isolate chromatin-bound and unbound complexes containing all six human MCM (hMCM) proteins by immunoprecipitation. In the present study, we applied this procedure to HeLa cells synchronized in each of the G1, S, and G2/M phases and could detect hMCM heterohexameric complexes in all three. In addition, depending on the cell cycle and the state of chromatin association, hMCM2 and 4 in the complexes were found to variously change their phosphorylation states. Concentrating attention on G2/M phase hyperphosphorylation, we found hMCM2 and 4 in the complexes to be good substrates for cdc2/cyclin B in vitro. Furthermore, when cdc2 kinase was inactivated in temperature-sensitive mutant murine FT210 cells, the G2/M hyperphosphorylation of the murine MCM2 and MCM4 and release of the MCMs from chromatin in the G2 phase were severely impaired. Taken together, the data suggest that the six mammalian MCM proteins function and undergo cell cycle-dependent regulation as heterohexameric complexes and that phosphorylation of the complexes by cdc2 kinase may be one of mechanisms negatively regulating the MCM complex-chromatin association.

Published

1998

34. Phosphorylation of vimentin by Rho-associated kinase at a unique amino-terminal site that is specifically phosphorylated during cytokinesis.

Author

Goto H, Kosako H, Tanabe K, Yanagida M, Sakurai M, Amano M, Kaibuchi K, and Inagaki M

Subjects

Amino Acid Sequence, Anaphase, Animals, COS Cells, Cattle, Fluorescent Antibody Technique, Indirect, GTP-Binding Proteins metabolism, Guanosine Triphosphate metabolism, Immunologic Techniques, Intermediate Filaments ultrastructure, Intracellular Signaling Peptides and Proteins, Microscopy, Confocal, Molecular Sequence Data, Phosphorylation, Phosphoserine metabolism, rho GTP-Binding Proteins, rho-Associated Kinases, Cell Division, Protein Serine-Threonine Kinases metabolism, Vimentin metabolism

Abstract

We found that vimentin, the most widely expressed intermediate filament protein, served as an excellent substrate for Rho-associated kinase (Rho-kinase) and that vimentin phosphorylated by Rho-kinase lost its ability to form filaments in vitro. Two amino-terminal sites on vimentin, Ser38 and Ser71, were identified as the major phosphorylation sites for Rho-kinase, and Ser71 was the most favored and unique phosphorylation site for Rho-kinase in vitro. To analyze the vimentin phosphorylation by Rho-kinase in vivo, we prepared an antibody GK71 that specifically recognizes the phosphorylation of vimentin-Ser71. Ectopic expression of constitutively active Rho-kinase in COS-7 cells induced phosphorylation of vimentin at Ser71, followed by the reorganization of vimentin filament networks. During the cell cycle, the phosphorylation of vimentin-Ser71 occurred only at the cleavage furrow in late mitotic cells but not in interphase or early mitotic cells. This cleavage furrow-specific phosphorylation of vimentin-Ser71 was observed in the various types of cells we examined. All these accumulating observations increase the possibility that Rho-kinase may have a definite role in governing regulatory processes in assembly-disassembly and turnover of vimentin filaments at the cleavage furrow during cytokinesis.

Published

1998

35. Spatial patterns of Ca2+ signals define intracellular distribution of a signaling by Ca2+/Calmodulin-dependent protein kinase II.

Author

Inagaki N, Goto H, Ogawara M, Nishi Y, Ando S, and Inagaki M

Subjects

Actin Cytoskeleton metabolism, Actin Cytoskeleton ultrastructure, Amino Acid Sequence, Animals, Animals, Newborn, Antibodies, Astrocytes cytology, Astrocytes drug effects, Calcium-Calmodulin-Dependent Protein Kinase Type 2, Cells, Cultured, Cerebral Cortex cytology, Cytoplasmic Granules metabolism, Cytoplasmic Granules ultrastructure, Immunohistochemistry, Ionomycin pharmacology, Microscopy, Immunoelectron, Peptide Fragments chemical synthesis, Peptide Fragments chemistry, Peptide Fragments metabolism, Phosphorylation, Rats, Serine, Vimentin chemistry, Astrocytes metabolism, Calcium metabolism, Calcium-Calmodulin-Dependent Protein Kinases metabolism, Cerebral Cortex metabolism, Signal Transduction, Vimentin metabolism

Abstract

Ca2+ plays a central role in cell signaling, and Ca2+/calmodulin-dependent protein kinase II (CaMKII) is a major mediator of Ca2+ actions. The spatial distribution of intracellular Ca2+ signaling is not homogenous, rather it is dynamically organized, and it has been speculated that spatial patterns of Ca2+ signals may function as a form of cellular information transmitted to downstream molecules. To address this issue, we studied the intracellular distributions of the signalings by CaMKII and Ca2+ in the same astrocytes. The former was visualized by monitoring site-specific phosphorylation of a cytoskeletal protein vimentin, using site- and phosphorylation-specific antibodies, while the latter was examined by fura-2-based Ca2+ microscopy. Local Ca2+ signals induced vimentin phosphorylation by CaMKII localized in the same area. On the other hand, Ca2+ waves in astrocytes induced global phosphorylation of vimentin by CaMKII. A small population of vimentin filaments highly phosphorylated by CaMKII underwent structural alteration into short filaments at electron microscopic level. These results indicate that CaMKII transmits spatial patterns of Ca2+ signals to vimentin as cellular information. The possibility is discussed that spatial patterns of vimentin phosphorylation may be important for intracellular organization of vimentin filament networks.

Published

1997

36. Phosphorylation of glial fibrillary acidic protein at the same sites by cleavage furrow kinase and Rho-associated kinase.

Author

Kosako H, Amano M, Yanagida M, Tanabe K, Nishi Y, Kaibuchi K, and Inagaki M

Subjects

Antibodies, Antibodies, Monoclonal, Astrocytoma, Glial Fibrillary Acidic Protein chemistry, Glutathione Transferase, Guanosine 5'-O-(3-Thiotriphosphate) metabolism, Guanosine Diphosphate metabolism, Humans, Intracellular Signaling Peptides and Proteins, Kinetics, Phosphopeptides chemistry, Phosphopeptides isolation & purification, Phosphorylation, Recombinant Fusion Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Substrate Specificity, Tumor Cells, Cultured, rho-Associated Kinases, Glial Fibrillary Acidic Protein metabolism, Protein Kinases metabolism, Protein Serine-Threonine Kinases metabolism

Abstract

Site- and phosphorylation state-specific antibodies are useful to analyze spatiotemporal distribution of site-specific phosphorylation of target proteins in vivo. Using several polyclonal and monoclonal antibodies that can specifically recognize four phosphorylated sites on glial fibrillary acidic protein (GFAP), we have previously reported that Thr-7, Ser-13, and Ser-34 on this intermediate filament protein are phosphorylated at the cleavage furrow during cytokinesis. This observation suggests that there exists a protein kinase named cleavage furrow kinase specifically activated at metaphase-anaphase transition (Matsuoka, Y., Nishizawa, K., Yano, T., Shibata, M., Ando, S., Takahashi, T., and Inagaki, M. (1992) EMBO J. 11, 2895-2902; Sekimata, M., Tsujimura, K., Tanaka, J., Takeuchi, Y., Inagaki, N., and Inagaki, M. (1996) J. Cell Biol. 132, 635-641). Here we report that GFAP is phosphorylated specifically at Thr-7, Ser-13, and Ser-34 by Rho-associated kinase (Rho-kinase), which binds to the small GTPase Rho in its GTP-bound active form. The kinase activity of Rho-kinase toward GFAP is dramatically stimulated by guanosine 5'-(3-O-thio)-triphosphate-bound RhoA. Furthermore, the phosphorylation of GFAP by Rho-kinase results in a nearly complete inhibition of its filament formation in vitro. The possibility that Rho-kinase is a candidate for cleavage furrow kinase is discussed.

Published

1997

37. Visualization and function of vimentin phosphorylation by cdc2 kinase during mitosis.

Author

Tsujimura K, Ogawara M, Takeuchi Y, Imajoh-Ohmi S, Ha MH, and Inagaki M

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal biosynthesis, Cytoplasm metabolism, Fluorescent Antibody Technique, Metaphase, Mice, Microscopy, Immunoelectron, Molecular Sequence Data, Phosphorylation, Serine metabolism, Tumor Cells, Cultured, Vimentin immunology, CDC2 Protein Kinase metabolism, Mitosis, Vimentin metabolism

Abstract

To investigate the role of intermediate filament (IF) protein phosphorylation by cdc2 kinase during mitosis, we developed a monoclonal antibody 4A4 recognizing Ser55-phosphorylated vimentin. Western blotting indicated that this antibody reacted with vimentin phosphorylated by cdc2 kinase but not with non-phosphorylated vimentin or with vimentin phosphorylated by other kinases such as cAMP-dependent protein kinase, protein kinase C, or Ca(2+)-calmodulin-dependent protein kinase II. Immunofluorescence and immunoelectron microscopy showed that vimentin Ser55 residues distributed in the entire cytoplasmic vimentin filament system are phosphorylated when the cells enter mitosis and dephosphorylated in cytokinesis. All cell lines examined showed a similar appearance of immunoreactivity with antibody 4A4. Fractionation of mitotic cell extracts on Mono-Q Sepharose revealed a single peak of vimentin Ser55 kinase activity, and the anti-p34cdc2 antibody reacted with the 34 kDa band in the kinase containing fractions. Vimentin Ser55 kinase activities were nil in the interphase cell extract. Immunofluorescent evidence using antibody 4A4 and biochemical analysis using vimentin Ser55 peptide showed that the degree of disassembly of vimentin filament of various cell types at early mitotic phase correlated well with the amount of mitotically activated cdc2 kinase.

Published

1994

38. The phosphorylation of kinesin regulates its binding to synaptic vesicles.

Author

Sato-Yoshitake R, Yorifuji H, Inagaki M, and Hirokawa N

Subjects

Animals, Kinesins isolation & purification, Kinesins ultrastructure, Kinetics, Microscopy, Electron, Microtubules metabolism, Microtubules ultrastructure, Models, Structural, Phosphorylation, Protein Binding, Rats, Synaptic Vesicles ultrastructure, Brain metabolism, Cerebral Cortex metabolism, Kinesins metabolism, Synaptic Vesicles metabolism

Abstract

Membrane organella are transported bidirectionally in cells, and the axonal transport system has provided an ideal model system for studying this bidirectional transport. Kinesin and cytoplasmic dynein were identified as candidates for the motor molecules of fast axonal transport, which transport organella along microtubules anterogradely and retrogradely. However, the mechanism that controls this bidirectional transport is unknown. Our previous work revealed that kinesin in axons was associated abundantly with anterogradely transported membranous organella, most of which are believed to be precursors of synaptic vesicles and axonal plasma membranes, while the fractions bound to retrogradely transported ones were very small (Hirokawa, N., Sato-Yoshitake, R., Kobayashi, N., Pfister, K. K., Bloom, G. S., and Brady, S. T. (1991) J. Cell Biol. 114, 295-302). Here we demonstrated in vitro that the binding of kinesin to synaptic vesicles was concentration-dependent and saturable and could be released by high salt concentration. When kinesin was phosphorylated by cAMP-dependent protein kinase, its binding to symaptic vesicles was significantly reduced. By motility assay and by statistical analysis using electron microscopy, we further revealed that synaptic vesicles preincubated with phosphorylated kinesin associated less frequently with microtubules than synaptic vesicles preincubated with unphosphorylated kinesin. The phosphorylation of kinesin should therefore play an essential role in regulating the direction of fast axonal transport by inhibiting its binding to membrane organella, thus releasing it from membrane organella at nerve terminals.

Published

1992

39. Purification and characterization of smooth muscle myosin-associated phosphatase from chicken gizzards.

Author

Mitsui T, Inagaki M, and Ikebe M

Subjects

Adenosine Triphosphate metabolism, Animals, Chickens, Chromatography, Affinity, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Enzyme Stability, Ethers, Cyclic pharmacology, Kinetics, Myosin-Light-Chain Phosphatase, Okadaic Acid, Phosphoprotein Phosphatases antagonists & inhibitors, Phosphorus Radioisotopes, Substrate Specificity, Gizzard, Avian enzymology, Muscle, Smooth enzymology, Phosphoprotein Phosphatases isolation & purification, Phosphoprotein Phosphatases metabolism

Abstract

Myosin light chain phosphatase associated with smooth muscle myosin (MAPP) was isolated from chicken gizzard. The MAPP was tightly associated with myosin and was not dissociated from myosin under the physiological ionic conditions. The phosphatase was dissociated from myosin in the presence of high MgCl2, i.e. 80 mM MgCl2. The binding site of the enzyme on the myosin molecule was the subfragment-2 region, since the enzyme did bind to the myosin rod and heavy meromyosin but not to the subfragment-1 affinity column. MAPP was purified with a heparin-Sepharose 6B column, and two activity peaks were obtained, i.e. MAPP I and MAPP II. The major activity peak, MAPP I, was further purified to homogeneity by thiophosphorylated myosin light chain-Sepharose 4B column chromatography. MAPP I was a tetramer composed of four 34-kDa subunits. The enzyme preferentially dephosphorylated the beta-subunit of phosphorylase kinase and was strongly inhibited by the heat- and acid-stable protein phosphatase inhibitor-1, whereas it was partially inhibited by the inhibitor-2. The IC50 (concentration of inhibitor giving 50% inhibition) value for the inhibition of the enzyme by okadaic acid was 70 nM which was about eight times higher than skeletal muscle type-1 and 390 times higher than type-2 protein phosphatase. These results demonstrate that the MAPP I is a type-1-like protein phosphatase, although the properties are not the same as type-I phosphatase. The properties of the myosin-associated phosphatase were distinct from the phosphatases reported previously, although some properties were similar to smooth muscle phosphatase-IV. Therefore, it is concluded that MAPP I is a novel smooth muscle protein phosphatase. Since it strongly associated with smooth muscle myosin, it is likely that MAPP I is responsible for the dephosphorylation of smooth muscle myosin in situ.

Published

1992

40. Phosphorylation by actin kinase of the pointed end domain on the actin molecule.

Author

Furuhashi K, Hatano S, Ando S, Nishizawa K, and Inagaki M

Subjects

Actins chemistry, Amino Acids analysis, Animals, Chromatography, High Pressure Liquid, Electrophoresis, Polyacrylamide Gel, Heparin, Low-Molecular-Weight metabolism, Peptide Mapping, Phosphorylation, Physarum metabolism, Protein Conformation, Substrate Specificity, Trypsin metabolism, Actins metabolism, Protein Kinases metabolism, Protein Serine-Threonine Kinases

Abstract

Fragmin from plasmodium of Physarum polycephalum binds G-actin and severs F-actin in the presence of Ca2+ over 10(-6) M. The fragmin-actin complex consisting of fragmin and G-actin nucleates actin polymerization and caps the barbed (fast growing) end of F-actin, regardless of the concentrations of Ca2+, and the actin filaments are shortened. Actin kinase purified from plasmodium abolishes the nucleation and capping activities of the complex by phosphorylating actin of the fragmin-actin complex (Furuhashi, K., and Hatano, S. (1990) J. Cell. Biol. 111, 1081-1087). This inactivation of the complex leads to production of long actin filaments. We obtained evidence that Physarum actin is phosphorylated by actin kinase at Thr-201, and probably at Thr-202 and/or Thr-203, with 1 mol of phosphate distributed among them. This finding raises the possibility that the site of phosphorylation, Thr-201 to Thr-203, is positioned on the pointed (slow growing) end domain of the actin molecule, because growth of actin filaments from the fragmin-actin complex occurs only from the pointed end. These observations are consistent with a model of the three-dimensional structure of G-actin. Inactivation of the fragmen-actin complex may follow phosphorylation of the pointed end domain of actin.

Published

1992

41. Inactivation of DNA polymerase beta by in vitro phosphorylation with protein kinase C.

Author

Tokui T, Inagaki M, Nishizawa K, Yatani R, Kusagawa M, Ajiro K, Nishimoto Y, Date T, and Matsukage A

Subjects

Alkaline Phosphatase metabolism, Amino Acid Sequence, Animals, Binding Sites, Brain enzymology, Chromatography, Affinity, DNA Polymerase I antagonists & inhibitors, DNA Polymerase I isolation & purification, DNA, Single-Stranded metabolism, Escherichia coli genetics, Kinetics, Macromolecular Substances, Molecular Sequence Data, Myocardium enzymology, Phosphorylation, Rats, Recombinant Proteins antagonists & inhibitors, Recombinant Proteins isolation & purification, Substrate Specificity, DNA Polymerase I metabolism, Protein Kinase C metabolism, Recombinant Proteins metabolism

Abstract

The Mr = 38,300 polypeptide of the purified recombinant rat DNA polymerase beta served as an excellent substrate for protein kinase C (PKC) in vitro but not for the catalytic subunit of cAMP-dependent protein kinase. The phosphorylation by PKC resulted in inactivation of DNA polymerase beta activity, and recovery was achieved by dephosphorylation with alkaline phosphatase. Since the phosphorylated DNA polymerase beta was retained with use of a single-stranded DNA-cellulose column, inactivation might occur at a site different from that for the DNA binding. Amino acid sequence analysis of the phosphopeptides revealed that the phosphorylated sites were 2 serine residues at positions 44 and 55 from the NH2 terminus, either or both of which might be involved in the catalytic activity of DNA polymerase beta. Thus, the inactivation of the DNA repair enzyme, DNA polymerase beta, by PKC may be an important process in the modification of DNA metabolism in the nucleus through signal transduction processes.

Published

1991

42. Specific localization of phosphointermediate filament protein in the constricted area of dividing cells.

Author

Nishizawa K, Yano T, Shibata M, Ando S, Saga S, Takahashi T, and Inagaki M

Subjects

Amino Acid Sequence, Blotting, Western, Fluorescent Antibody Technique, Microscopy, Fluorescence, Molecular Sequence Data, Neuroglia metabolism, Phosphorylation, Substrate Specificity, Cell Division, Glial Fibrillary Acidic Protein metabolism

Abstract

We developed antibodies pG1 and pG2 which recognize glial fibrillary acidic protein (GFAP) in its phosphorylated state. Antibodies pG1 and pG2 were produced against two synthetic peptides, Arg-Arg-Arg-Val-Thr-phosphoSer-Ala-Ala-Arg-Arg-phosphoSer (residues 3-13) and Pro-Gly-Pro-Arg-Leu-phosphoSer-Leu-Ala-Arg-Met-Pro (residues 29-39), respectively. The phosphorylation of these serine residues on the intact GFAP induces disassembly of glial filaments in vitro (Inagaki, M., Gonda, Y., Nishizawa, K., Kitamura, S., Sato, C., Ando, S., Tanabe, K., Kikuchi, K., Tsuiki, S., and Nishi, Y. (1990) J. Biol. Chem. 265, 4722-4729). Immunofluorescence and immunoblotting studies demonstrate that both antibodies react specifically with mitotic astroglial cells, thereby supporting the notion that increased phosphorylation during mitosis may directly influence intracellular organization of the glial filaments. The specific distribution pattern of the phosphoGFAP in the mitotic cells reveals that site-specific phosphorylation events may make way for the locally controlled breakdown of glial filaments in the constricted area, before the final separation of daughter cells.

Published

1991

43. Phosphorylation sites linked to glial filament disassembly in vitro locate in a non-alpha-helical head domain.

Author

Inagaki M, Gonda Y, Nishizawa K, Kitamura S, Sato C, Ando S, Tanabe K, Kikuchi K, Tsuiki S, and Nishi Y

Subjects

Animals, Binding Sites, Brain Chemistry, Cattle, Cyclic AMP pharmacology, Desmin metabolism, Hydrogen-Ion Concentration, Intermediate Filaments ultrastructure, Kinetics, Microscopy, Electron, Phosphorylation, Polymers metabolism, Protein Kinase C metabolism, Protein Kinases metabolism, Rats, Swine, Vimentin metabolism, Cytoskeleton metabolism, Glial Fibrillary Acidic Protein metabolism, Intermediate Filaments metabolism, Neuroglia ultrastructure, Phosphates metabolism

Abstract

Glial fibrillary acidic protein (GFAP), the intermediate filament component of astroglial cells, can serve as an excellent substrate for both cAMP-dependent protein kinase and protein kinase C, in vitro. GFAP phosphorylated by each protein kinase does not polymerize, and the filaments that do polymerize tend to depolymerize after phosphorylation. Dephosphorylation of phospho-GFAP by phosphatase led to a recovery of the polymerization competence of GFAP. Most of the phosphorylation sites for cAMP-dependent protein kinase and protein kinase C on GFAP are the same, Ser-8, Ser-13, and Ser-34. cAMP-dependent protein kinase has one additional phosphorylation site, Thr-7. All the sites are located within the amino-terminal non-alpha-helical head domain of GFAP. These observations pave the way for in vivo studies on organization of glial filaments.

Published

1990

44. Correlation of conformation and phosphorylation and dephosphorylation of smooth muscle myosin.

Author

Ikebe M, Inagaki M, Naka M, and Hidaka H

Subjects

Animals, Gizzard, Avian enzymology, Kinetics, Magnesium pharmacology, Magnesium Chloride, Myosin-Light-Chain Phosphatase, Phosphorylation, Potassium Chloride pharmacology, Protein Conformation, Turkeys, Muscle, Smooth enzymology, Myosin-Light-Chain Kinase metabolism, Myosins metabolism, Phosphoprotein Phosphatases metabolism

Abstract

The rate of phosphorylation and dephosphorylation of smooth muscle myosin by myosin light chain kinase and by two myosin light chain phosphatases (gizzard phosphatase IV and aorta phosphatase) are measured in various conditions; the relationship between the rate of phosphorylation and dephosphorylation of myosin and the myosin conformation is also studied. The rate of dephosphorylation of myosin was completely inhibited in the presence of 1 mM MgCl2 and ATP at low ionic strength where phosphorylated myosin forms a folded conformation. The inhibition was released when myosin formed either an extended monomer or filaments. The rate of phosphorylation of myosin was also affected by the conformation of myosin. The rate for a folded myosin was slower than those for an extended monomer and filamentous myosin. The phosphorylation and dephosphorylation of heavy meromyosin, subfragment-1, and the isolated 20,000-dalton light chain are not inhibited at low ionic strength, and the rate of phosphorylation and dephosphorylation was decreased with increasing ionic strength. KCl dependence of the rate of phosphorylation and dephosphorylation of myosin was normalized by using KCl dependence of subfragment-1, and it was found that the marked inhibition of the rate of phosphorylation and dephosphorylation of myosin is closely related to the change from an extended to a folded conformation of myosin.

Published

1988

45. Intermediate filament reconstitution in vitro. The role of phosphorylation on the assembly-disassembly of desmin.

Author

Inagaki M, Gonda Y, Matsuyama M, Nishizawa K, Nishi Y, and Sato C

Subjects

Animals, Calcium pharmacology, Cattle, Chickens, Cyclic AMP pharmacology, Kinetics, Magnesium pharmacology, Magnesium Chloride, Mice, Microscopy, Electron, Phosphorylation, Phosphoserine metabolism, Polymers, Protein Kinase C metabolism, Protein Kinases metabolism, Sodium Chloride pharmacology, Vimentin metabolism, Desmin metabolism, Phosphoproteins metabolism

Abstract

Desmin, the myogenic intermediate filament protein, is a phosphoprotein containing phosphoserine, in vivo. The role of phosphorylation on assembly-disassembly and organization of the desmin filament has remained obscure. We report here on a stable and purified system which enables a biochemical examination of desmin filament assembly and disassembly. Using this in vitro system, we carried out stoichiometrical phosphorylations by purified protein kinases. The extent of polymerization-depolymerization was estimated using procedures related to centrifugation and electron microscopy. The evidence we obtained suggests that disassembly of the desmin filament and inhibition of the NaCl-dependent polymerization of the soluble desmin can reversibly occur with either cAMP-dependent or Ca2+-activated, phospholipid-dependent desmin phosphorylation.

Published

1988

46. Ca2+-dependent deimination-induced disassembly of intermediate filaments involves specific modification of the amino-terminal head domain.

Author

Inagaki M, Takahara H, Nishi Y, Sugawara K, and Sato C

Subjects

Amino Acids analysis, Animals, Chromatography, High Pressure Liquid, Intermediate Filament Proteins isolation & purification, Kinetics, Mice, Microscopy, Electron, Peptide Fragments isolation & purification, Phosphorylation, Protein Kinase C metabolism, Protein Kinases metabolism, Protein-Arginine Deiminase Type 4, Protein-Arginine Deiminases, Vimentin ultrastructure, Calcium pharmacology, Hydrolases metabolism, Intermediate Filament Proteins metabolism, Muscles enzymology, Vimentin metabolism

Abstract

Peptidylarginine deiminase (proteinarginine iminohydrolase, EC 3.5.3.15) converted some arginine residues to citrulline residues in soluble vimentin, in a micromolar Ca2+-dependent manner and resulted in the loss of polymerization competence of the intermediate filament protein. When about 8 mol of residues/mol of vimentin were deiminated, there was a complete loss of filament forming ability. This enzyme also deiminated vimentin filaments which had been polymerized, and deimination of vimentin filaments resulted in filament disassembly. Similar results were obtained with other intermediate filaments such as desmin and glial filaments. High performance liquid chromatography and amino acid analyses of lysine-specific protease-generated fragments from deiminated vimentin (about 8 mol of citrulline/mol of vimentin) showed a differential deimination of three structural domains. The head domain was predominant. These observations suggest that the head domain strongly influences integrity of the intermediate filament.

Published

1989

47. Protein kinase C phosphorylation of desmin at four serine residues within the non-alpha-helical head domain.

Author

Kitamura S, Ando S, Shibata M, Tanabe K, Sato C, and Inagaki M

Subjects

Amino Acid Sequence, Amino Acids analysis, Animals, Brain enzymology, Molecular Sequence Data, Phosphopeptides isolation & purification, Phosphorylation, Protein Conformation, Rats, Substrate Specificity, Desmin metabolism, Protein Kinase C metabolism, Serine

Abstract

We reported that phosphorylation by either cAMP-dependent protein kinase or protein kinase C (Ca2+/phospholipid-dependent enzyme) in vitro induces disassembly of the desmin filaments (Inagaki, M., Gonda, Y., Matsuyama, M., Nishizawa, K., Nishi, Y., and Sato, C. (1988) J. Biol. Chem. 263, 5970-5978). For this subunit protein, Ser-29, Ser-35, and Ser-50 within the non-alpha-helical head domain were shown to be the sites of phosphorylation for cAMP-dependent protein kinase (Geisler, N., and Weber, K. (1988) EMBO J. 7, 15-20). In the present work, we identified the sites of desmin phosphorylated in vitro by other protein kinase which affects the filament structure. The protein kinase C-phosphorylated desmin was hydrolyzed with trypsin, and the phosphorylated peptides were isolated by reverse-phase chromatography. Sequential analysis of the purified phosphopeptides, together with the known primary sequence, revealed that Ser-12, Ser-29, Ser-38, and Ser-56 were phosphorylated by protein kinase C. All four sites are located within the non-alpha-helical head domain of desmin. Ser-12, Ser-38, and Ser-56, specifically phosphorylated by protein kinase C, have arginine residues at the carboxyl-terminal side (Arg-14, Arg-42, and Arg-59, respectively). Ser-29 phosphorylated by both protein kinase C and cAMP-dependent protein kinase has arginine residues at the amino and carboxyl termini (Arg-27 and Arg-33). These findings support the view that the head domain-specific phosphorylation strongly influences desmin filament structure; however, each protein kinase differed with regard to site recognition on this domain.

Published

1989

48. Conformational studies of myosin phosphorylated by protein kinase C.

Author

Umekawa H, Naka M, Inagaki M, Onishi H, Wakabayashi T, and Hidaka H

Subjects

Animals, Chickens, Electrophoresis, Polyacrylamide Gel, Gizzard, Avian analysis, Microscopy, Electron, Molecular Weight, Muscle, Smooth analysis, Myosin-Light-Chain Kinase, Phosphorylation, Potassium Chloride pharmacology, Protein Conformation, Protein Kinase C, Myosins metabolism, Protein Kinases metabolism

Abstract

Smooth muscle myosin from chicken gizzard is phosphorylated by Ca2+-activated phospholipid-dependent protein kinase, protein kinase C, as well as by Ca2+/calmodulin-dependent kinase, myosin light chain kinase (Endo, T., Naka, M., and Hidaka, H. (1982) Biochem. Biophys. Res. Commun. 105, 942-948). We have now demonstrated the effect of phosphorylation by protein kinase C on the smooth muscle myosin molecule. In glycerol/urea polyacrylamide gel electrophoresis the 20,000-dalton light chain phosphorylated by protein kinase C co-migrated with that phosphorylated by myosin light chain kinase. Moreover, the light chain phosphorylated by both kinases migrated more rapidly than did the light chain phosphorylated by either myosin light chain kinase or protein kinase C alone. Myosin phosphorylated by protein kinase C formed a bent 10 S monomer while that phosphorylated by myosin light chain kinase was an unfolded and extended 6 S monomer in the presence of 0.2 M KCl. In addition, myosin phosphorylated by kinases had a sedimentation velocity of 7.3 S, thereby suggesting that the myosin was partially unfolded. The unfolded myosin was visualized electron microscopically. The fraction in the looped form was higher when for myosin phosphorylated by both kinases higher than for that phosphorylated by light chain kinase alone. Therefore, phosphorylation by protein kinase C does not lead to the change in myosin conformation seen with myosin light chain kinase.

Published

1985

49. Phosphorylation of smooth muscle myosin light chain kinase by Ca2+-activated, phospholipid-dependent protein kinase.

Author

Ikebe M, Inagaki M, Kanamaru K, and Hidaka H

Subjects

Animals, Binding Sites, Calmodulin metabolism, Electrophoresis, Polyacrylamide Gel, Gizzard, Avian enzymology, Myosin-Light-Chain Kinase, Peptide Fragments analysis, Phosphorylation, Protein Kinase C, Time Factors, Trypsin metabolism, Turkeys, Muscle, Smooth enzymology, Protein Kinases metabolism

Abstract

Protein kinase C incorporates phosphate into two sites of myosin light chain kinase (MLC-kinase) in the absence of calmodulin. Phosphorylation is all but abolished in the presence of Ca2+ and calmodulin, suggesting that both sites of phosphorylation are close to the calmodulin binding site. The phosphorylation of MLC-kinase results in an approximately 10-fold increase in the dissociation constant of MLC-kinase for calmodulin. Following phosphorylation (2 mol/mol of enzyme) of MLC-kinase by protein kinase C, an additional 2 mol of phosphate can be incorporated into the MLC-kinase apoenzyme by the cAMP-dependent protein kinase. Different maps of phosphopeptides were obtained by tryptic hydrolysis from MLC-kinase preparations phosphorylated by each kinase. The phosphorylation sites for the cAMP-dependent kinase were located in a fragment of approximately 25,000 daltons. In contrast the phosphorylation sites for protein kinase C are found in a much smaller tryptic peptide. These results suggest that the phosphorylation sites on MLC-kinase are different for protein kinase C and for cAMP-dependent protein kinase. However, phosphorylation in both regions results in a reduced affinity for calmodulin.

Published

1985

50. N-(2-Aminoethyl)-5-isoquinolinesulfonamide, a newly synthesized protein kinase inhibitor, functions as a ligand in affinity chromatography. Purification of Ca2+-activated, phospholipid-dependent and other protein kinases.

Author

Inagaki M, Watanabe M, and Hidaka H

Subjects

Animals, Chromatography, Affinity methods, Chromatography, Gel, Cyclic AMP metabolism, Cyclic GMP metabolism, Electrophoresis, Polyacrylamide Gel, Molecular Weight, Rabbits, Swine, Calcium metabolism, Enzyme Inhibitors, Isoquinolines, Phospholipids metabolism, Protein Kinases isolation & purification, Sulfonamides

Abstract

We designed a simple procedure for the purification of Ca2+-activated, phospholipid-dependent protein kinase (protein kinase C) from rabbit brain, using affinity chromatography with a new affinity adsorbent. The adsorbent was synthesized by attaching the amino residue of N-(2-aminoethyl)-5-isoquinolinesulfonamide (H-9) to cyanogen bromide-activated Sepharose. H-9 is a potent competitive inhibitor of protein kinase C, cGMP-, and cAMP-dependent protein kinase with respect to ATP and exhibits inhibition constants of 18, 0.87, and 1.9 microM, respectively (Hidaka, H., Inagaki, M., Kawamoto, S., and Sasaki, Y. (1984) Biochemistry, 23, 5036). A 960-fold purification was achieved in the two-step procedure, which entailed DEAE-cellulose and the affinity chromatography. The resultant preparation was essentially homogeneous, as indicated by polyacrylamide gel electrophoresis under conditions of denaturation with sodium dodecyl sulfate. The affinity of protein kinase C for the H-9-Sepharose was high, and the enzyme could not be eluted either by a high concentration of sodium chloride or by 40% glycerol. The protein kinase C could be eluted from H-9-Sepharose by the buffer containing both 0.2 M NaCl and 20% glycerol, thereby suggesting that the binding between protein kinase C and H-9-Sepharose was due to both hydrophobic and electrostatic interactions. H-9 coupled to Sepharose retained both cyclic nucleotide-dependent protein kinases and protein kinase C, and these enzymes could be eluted separately by the buffer containing L-arginine, a potent inhibitor of these three kinases. The novel aspects of these three multifunctional protein kinases can thus be investigated using isoquinolinesulfonamide derivatives.

Published

1985