Your search keyword '"Toriumi H"' showing total 116 results

101. Monoclonal antibody #3-9-16 recognizes one of the two isoforms of rabies virus matrix protein that exposes its N-terminus on the virion surface.

Author

Ameyama S, Toriumi H, Takahashi T, Shimura Y, Nakahara T, Honda Y, Mifune K, Uchiyama T, and Kawai A

Subjects

Animals, Antibodies, Viral immunology, Antigens, Viral immunology, Cell Line, Cell Membrane virology, Complement System Proteins immunology, Cricetinae, Epitopes, Glycoproteins analysis, Protein Conformation, Protein Isoforms analysis, Protein Isoforms chemistry, Protein Isoforms immunology, Viral Envelope Proteins analysis, Viral Matrix Proteins chemistry, Antibodies, Monoclonal immunology, Golgi Apparatus virology, Rabies virus immunology, Viral Matrix Proteins analysis, Viral Matrix Proteins immunology, Virion chemistry

Abstract

We investigated behaviors of the rabies virus matrix (M) protein using a monoclonal antibody (mAb), #3-9-16, that recognized a linear epitope located at the N-terminus of the protein. Based on the reactivity with this mAb, M proteins could be divided into at least two isoforms; an ordinary major form (Malpha) whose 3-9-16 epitope is hidden, and an N-terminal-exposed epitope-positive form (Mbeta). The Mbeta protein accounted for about 25-30% of the total M proteins in the virion, while its content in the cell ranged from 10 to 15% of total M protein. Fluorescent antibody (FA) staining showed that the Mbeta antigen distributed in the Golgi area where the colocalized viral glycoprotein antigen was also detected. Mbeta antigen was shown to be exposed on the surface of infected cells by both immunoprecipitation and FA staining with the mAb, whereby the cells might have become sensitive to the mAb-dependent complement-mediated cytolysis. Similarly, the Mbeta antigen was shown to be exposed on the virion surface, and the infectivity of the virus was destroyed by the mAb in the presence of a complement. Together with these results, we think that the M protein molecule takes either of two conformations, one (Mbeta) of which exposes the 3-9-16 epitope located in the N-terminal region of the M protein, that are also exposed on the surface of the virion and infected cells, whereby it might play a certain important role(s) in the virus replication process differently from the other form (Malpha), probably through its intimate association with the Golgi area and/or the cell membrane.

Published

2003

102. Characterization of a slow-migrating component of the rabies virus matrix protein strongly associated with the viral glycoprotein.

Author

Nakahara T, Toriumi H, Irie T, Takahashi T, Ameyama S, Mizukoshi M, and Kawai A

Subjects

Animals, Antibodies, Monoclonal, Cell Line, Cricetinae, Dimerization, Electrophoresis, Polyacrylamide Gel, Electrophoretic Mobility Shift Assay, Epitopes, Glycoproteins immunology, Isoelectric Point, Molecular Weight, Protein Binding, Protein Conformation, Viral Envelope Proteins immunology, Viral Matrix Proteins immunology, Viral Proteins chemistry, Viral Proteins immunology, Antigens, Viral, Glycoproteins chemistry, Rabies virus chemistry, Viral Envelope Proteins chemistry, Viral Matrix Proteins chemistry

Abstract

We investigated multiple forms of rabies virus matrix (M) protein. Under non-reducing electrophoretic conditions, we detected, in addition to major bands of monomer forms (23- and 24-kDa) of M protein, an M antigen-positive slow-migrating minor band (about 54 kDa) in both the virion and infected cells. Relative contents of the 54-kDa and monomer components in the virion were about 20-30% and 70-80% of the whole M protein, respectively, while the content of the 54-kDa component was smaller (about 10-20% of the total M protein) in the cell than in the virion. The 54-kDa components could be extracted from the infected cells with sodium deoxycholate, but they were quite resistant to extraction with 1% nonionic detergents by which most monomer components were solubilized. The 54-kDa component was precipitated more efficiently than the monomer by a monoclonal antibody (mAb; #3-9-16), which recognized a linear epitope located at the N-terminal of the M protein. The mAb #3-9-16 coprecipitated the viral glycoprotein (G), which was demonstrated to be due to strong association between the G and 54-kDa component of the M protein. Monomers and the 54-kDa polypeptide migrated to the same isoelectric point (pI) in twodimensional (2-D) gel electrophoresis, implicating that the 54-kDa component was composed of component(s) of the same pI as that of the M protein monomers. From these results, we conclude that the M antigen-positive 54-kDa polypeptide is a homodimer of M protein, taking an N-terminal-exposed conformation, and is strongly associated with the viral glycoprotein. Possible association with a membrane microdomain of the cell will be discussed.

Published

2003

103. Structural relationship between nucleocapsid-binding activity of the rabies virus phosphoprotein (P) and exposure of epitope 402-13 located at the C terminus.

Author

Toriumi H, Honda Y, Morimoto K, Tochikura TS, and Kawai A

Subjects

Animals, Antibodies, Monoclonal immunology, Antigens, Viral immunology, Cell Line, Cricetinae, Molecular Chaperones, Nucleocapsid Proteins, Phosphoproteins genetics, Protein Conformation, Rabies virus immunology, Structure-Activity Relationship, Viral Structural Proteins genetics, Epitope Mapping, Epitopes chemistry, Nucleocapsid metabolism, Phosphoproteins chemistry, Phosphoproteins metabolism, Rabies virus metabolism, Viral Structural Proteins chemistry, Viral Structural Proteins metabolism

Abstract

The structural changes of the nominal phosphoprotein (P) of rabies virus using a monoclonal antibody, mAb #402-13, was investigated. This mAb recognized a linear epitope that was mapped roughly to a C-terminal region of the P protein, ranging from aa 256 to 297. The P gene products were detected by the mAb in immunoblot assays, the products of which were produced either in BHK-21 cells or in Escherichia coli cells. The mAb, however, detected very low levels of P gene products in immunoprecipitation assays. The mAb recognized the nucleocapsid (NC)-associated P proteins but recognized free P protein and free N-P complex produced in the infected cells much less efficiently. When the P proteins were released from the NC, however, they were no longer recognized by the mAb. Similar results were obtained from BHK-21 cells co-transfected with P and N cDNAs. Furthermore, studies with C-terminally truncated P protein mutants revealed that the NC-binding ability of the P protein was dependent on the presence of the C-terminal epitope region. From these results, it is thought that the 402-13 epitope region is concealed when the P protein is present in a free form or free N-P complex but is exposed when it is associated with the NC. The C-terminal epitope region seemed to be essential for the P protein to be associated with the NC but not for the formation of free N-P complexes with newly synthesized N protein.

Published

2002

104. Lower ulnar nerve palsy related to fracture of the pisiform bone in patients with multiple injuries.

Author

Matsunaga D, Uchiyama S, Nakagawa H, Toriumi H, Kamimura M, and Miyasaka T

Subjects

Accidental Falls, Fractures, Bone diagnostic imaging, Fractures, Bone therapy, Fractures, Malunited diagnostic imaging, Fractures, Malunited surgery, Humans, Male, Middle Aged, Multiple Trauma complications, Radiography, Ulnar Neuropathies surgery, Wrist Injuries diagnostic imaging, Fractures, Bone complications, Fractures, Malunited complications, Multiple Trauma diagnosis, Ulnar Neuropathies etiology, Wrist Injuries complications

Published

2002

105. Studies on the rabies virus RNA polymerase: 3. Two-dimensional electrophoretic analysis of the multiplicity of non-catalytic subunit (P protein).

Author

Eriguchi Y, Toriumi H, and Kawai A

Subjects

Cells, Cultured, DNA-Directed RNA Polymerases genetics, Electrophoresis, Gel, Two-Dimensional, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression Regulation, Bacterial, Models, Genetic, Molecular Chaperones, Nucleocapsid analysis, Nucleocapsid classification, Nucleocapsid Proteins, Okadaic Acid metabolism, Phosphoproteins genetics, Phosphoproteins metabolism, Phosphoric Monoester Hydrolases metabolism, Rabies virus genetics, Viral Structural Proteins genetics, Viral Structural Proteins metabolism, DNA-Directed RNA Polymerases analysis, Phosphoproteins analysis, Rabies virus enzymology, Viral Structural Proteins analysis

Abstract

We described previously (Takamatsu et al., 1998. Microbiol. Immunol. 42: 761-771) the rabies virus P protein as being composed of several components of different sizes, among which the full-sized major components were termed as p40 and p37 according to their electrophoretic mobilities, and radiolabeling studies with [32P]phosphate implied that p40 was a hyperphosphorylated form. We further examined here these proteins by two-dimensional (2-D) gel electrophoresis and immunoblotting, showing that a major component, p37, was composed of multiply modified subcomponents of different pIs (termed p37-1, p37-2, p37-3, etc., based on their acidity) in the virion and infected cells, but the unmodified precursor (termed p37-0) was little in amount. The viral nucleocapsid (NC)-bound P proteins were composed of multiple forms of p37 (the major one was p37-1) and also a minor component, p40-1. P proteins which were bound to newly synthesized free N proteins were mostly composed of p37-1, indicating that hyperphosphorylation of P proteins occurred after their being used for the encapsidation. Treatment of the infected cells with okadaic acid induced accumulation of the more acidic forms of P proteins, suggesting that heterogeneity in the full-sized P proteins is a reflection of their dynamic aspects of multiple cycles of phosphorylations and dephosphorylations in the cell. Two-D gel analyses demonstrated also that p40 was not so acidic as we expected, and implied that our previous data of apparent hyperphosphorylation of p40 was due to very frequently recycled utilization of the protein, and preformed non-labeled P proteins were also 32P-phosphorylated in a radiolabeling period and were converted to the p40.

Published

2002

106. Longitudinal Median Nerve Conduction Studies After Endoscopic Carpal Tunnel Release.

Author

Nakamura Y, Uchiyama S, Toriumi H, Nakagawa H, and Miyasaka Ta

Abstract

Forty hands of 36 patients who had undergone endoscopic carpal tunnel release (ECTR), utilising Chow's two-portal technique after being diagnosed with idiopathic carpal tunnel syndrome, were subjected to longitudinal median nerve conduction studies. The distal motor latency (DML) was examined pre-operatively on all the hands, which were re-examined at the post-operative 1st, 3rd, 6th and 12th months. Rapid improvement of DML was observed post-operatively in the first three months. These improvements patterns are not much different from those after open carpal tunnel release (OCTR) reported in the literatures. We consider that the data reported herein can be used as standards of DML course after ECTR.

Published

1999

107. Nucleocapsid formation and/or subsequent conformational change of rabies virus nucleoprotein (N) is a prerequisite step for acquiring the phosphatase-sensitive epitope of monoclonal antibody 5-2-26.

Author

Kawai A, Toriumi H, Tochikura TS, Takahashi T, Honda Y, and Morimoto K

Subjects

Animals, Antigens, Viral chemistry, Antigens, Viral genetics, Antigens, Viral immunology, Antigens, Viral metabolism, Blotting, Western, Cell Fractionation, Cell Line, Cricetinae, Fluorescent Antibody Technique, Molecular Chaperones, Nucleocapsid chemistry, Nucleocapsid genetics, Nucleocapsid Proteins, Phosphates metabolism, Phosphoproteins metabolism, Phosphorylation, Precipitin Tests, Protein Binding, Protein Conformation, Rabies virus genetics, Rabies virus immunology, Solubility, Time Factors, Viral Structural Proteins metabolism, Antibodies, Monoclonal immunology, Epitopes immunology, Nucleocapsid immunology, Nucleocapsid metabolism, Phosphoric Monoester Hydrolases metabolism, Rabies virus metabolism

Abstract

We investigated the antigenic maturation of rabies virus N protein, for which we used some conformational epitope-specific monoclonal antibodies (MAbs) and an MAb (5-2-26) against a phosphorylation-dependent linear epitope. Infected cells were lysed with a deoxycholate-free lysis buffer and separated by ultracentrifugation into the soluble top and the nucleocapsid fractions. None of the study MAbs recognized N proteins in the top fraction, whereas nucleocapsid-associated N proteins were recognized by all of the MAbs. Immunoprecipitation with polyclonal anti-N antibodies coprecipitated the P proteins from the top fraction, indicating that soluble N proteins are mostly associated with the P protein. The N proteins dissociated from both the N-P complex and nucleocapsids were recognized by none of the study MAbs, whereas the MAb 5-2-6 recognized the SDS-denatured N proteins of the nucleocapsid but not of the top fraction. In addition, the phosphorylation-deficient mutant N proteins were shown to be similarly accumulated as the wild-type N proteins into the viral inclusion bodies, defined as the virus-specific structures composed of viral nucleocapsids, that are produced in the cytoplasm of the infected cells. Based on these results, we believe that newly synthesized N proteins are not immediately phosphorylated at serine-389 (a common phosphorylation site) but are first associated with the P protein. After being used for encapsidation of the viral RNA, the N proteins undergo conformational changes, whereby epitopes for the conformation-specific MAbs are formed and become phosphorylated at serine-389., (Copyright 1999 Academic Press.)

Published

1999

108. Nontraumatic bilateral first rib fractures.

Author

Tsukada A, Uchiyama S, Toriumi H, Nakagawa H, and Miyasaka T

Subjects

Adult, Female, Fractures, Spontaneous diagnostic imaging, Humans, Pain etiology, Radiography, Rib Fractures diagnostic imaging, Fractures, Spontaneous etiology, Rib Fractures etiology

Abstract

The authors report the case of a 21-year old woman who presented bilateral spontaneous fractures of the first ribs, in the posterior portion on the right side, in the anterior portion on the left side. The pathogenesis of spontaneous fractures of the first rib is discussed.

Published

1998

109. Studies on the rabies virus RNA polymerase: 2. Possible relationships between the two forms of the non-catalytic subunit (P protein).

Author

Takamatsu F, Asakawa N, Morimoto K, Takeuchi K, Eriguchi Y, Toriumi H, and Kawai A

Subjects

Amino Acid Sequence, Animals, Antibodies, Viral biosynthesis, Base Sequence, Cells, Cultured, Cricetinae, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases immunology, Immunoblotting, Molecular Sequence Data, Molecular Weight, Phosphorylation, Rabbits, DNA-Directed RNA Polymerases chemistry, Rabies virus enzymology

Abstract

We investigated the relationship between the two forms of rabies virus P protein, a non-catalytic subunit of rabies virus RNA polymerase. The two displayed different electrophoretic mobilities as 37- and 40-kDa polypeptides, hence termed as p37 and p40, respectively. Double labeling experiments with [3H]leucine and [32P]orthophosphate demonstrated that p40 was much more phosphorylated than p37. Treatment of the virion proteins with alkaline phosphatase eliminated only p40, and not 37-kDa polypeptide. The p37 was a major product of the P gene, and was accumulated in the infected cell and incorporated into the virion. On the other hand, p40 was apparently detected only in the virion, and little detected in the cells. Treatment of infected cells with okadaic acid, however, resulted in significant accumulation of p40 in the cell, suggesting that p40 was continuously produced in the cell but dephosphorylated quickly. We detected both 37- and 40-kDa products in P cDNA-transfected animal cells, while only a 37-kDa product was produced in Escherichia coli. Incubation of 37-kDa products from E. coli with the lysates of animal cells in vitro resulted in the production of a 40-kDa product, which was also shown to be suppressed by the heparin. From these results, it is suggested that p40 is produced by the hyperphosphorylation of a 37-kDa polypeptide, which depends on certain heparin-sensitive cellular enzyme(s) and occurs even in the absence of the other viral gene products, and that p40 is reverted quickly to p37 in the infected cells, probably being dependent on some virus-induced factor(s).

Published

1998

110. A histochemical study of anionic sites in the intermediate layer of rat femoral cartilage using polyethyleneimine at different pH levels.

Author

Ueda H, Toriumi H, Leng CG, and Ohno S

Subjects

Animals, Cartilage, Articular ultrastructure, Femur Head chemistry, Femur Head ultrastructure, Hydrogen-Ion Concentration, Male, Rats, Rats, Wistar, Anions analysis, Cartilage, Articular chemistry, Coloring Agents, Polyethyleneimine

Abstract

Anionic sites in the intermediate layer of young rat hyaline cartilages were examined using a cationic dye, polyethyleneimine (PEI), at different pH levels. Femoral heads were resected and fixed in 2.5% glutaraldehyde and treated with 0.5% PEI at pH 7.4, pH 2.5 or pH 1.0. Some cartilage samples were first digested with chondroitinase ABC or hyaluronidase. The PEI deposits at pH 7.4 appeared to be irregular shapes. Their sizes seemed to be larger than those at pH 2.5 or pH 1.0. The PEI deposits were also found on the surface of collagen fibrils at both pH 7.4 and pH 2.5 even after the chondroitinase ABC digestion, but were not found at pH 1.0. Moreover, they disappeared after hyaluronidase digestion. Accordingly, it is suggested that PEI-positive structures varied depending on pH levels. In addition, hyaluronan may be localized near collagen fibrils, but most sulphated proteoglycans may not.

Published

1997

111. Effects of smoking on spontaneous and induced sister chromatid exchanges in lymphocytes.

Author

Nagaya T and Toriumi H

Subjects

Adult, Environmental Pollutants toxicity, Humans, Male, Middle Aged, Mitomycin, Mitomycins toxicity, Lymphocytes ultrastructure, Mutagens, Sister Chromatid Exchange drug effects, Smoking

Abstract

Spontaneous and mitomycin C-induced sister chromatid exchanges (SCEs) in lymphocytes were analyzed in 24 non-smokers and 24 sex- and age-matched smokers. Mean spontaneous SCE frequency for non-smokers was 9.8 SCEs/cell, and that for smokers was 11.5 SCEs/cell. The difference was statistically significant (P less than 0.001 by t-test). These results suggest that spontaneous SCE frequency in lymphocytes is useful for evaluation of biological effects of environmental mutagens. However, we could not find any effects of smoking on the sensitivities of lymphocytes to mitomycin C in vitro. The effects of mutagens on humans may be independent of one another.

Published

1985

112. [A lesson from the interactions with a child with Down's syndrome hospitalized for the treatment of leukemia].

Author

Toriumi H

Subjects

Down Syndrome complications, Humans, Leukemia complications, Down Syndrome nursing, Leukemia nursing, Nurse-Patient Relations

Published

1982

113. Efficacy of ivermectin against live mites and eggs of Sarcoptes scabiei in pigs.

Author

Ohba S, Toriumi H, Takeishi M, and Noda R

Subjects

Animals, Female, Parasite Egg Count, Scabies drug therapy, Scabies parasitology, Swine parasitology, Swine Diseases parasitology, Ivermectin therapeutic use, Sarcoptes scabiei drug effects, Scabies veterinary, Swine Diseases drug therapy

Abstract

Sows infested with Sarcoptes scabiei var. suis (ssvs) were treated with 75, 150 and 300 micrograms/kg of ivermectin by a single subcutaneous injection at the neck region. Compared to the numbers of mites and eggs just before injection, those on post treatment weeks (PTW) 1, 2 and 4 showed significant decreases. Especially at 300 micrograms/kg, the counts showed almost all mites and eggs were eradicated on PTW 1, manifesting ivermectin to possess potential effect on ssve without apparent abnormal side effect. Potential mitocide effect of ivermectin on ssvs was revealed.

Published

1989

114. Spontaneous and induced sister chromatid exchanges in lymphocytes of healthy persons.

Author

Nagaya T and Toriumi H

Subjects

Adult, Aging, Humans, Male, Middle Aged, Mitomycin, Lymphocytes drug effects, Mitomycins adverse effects, Mutagens, Sister Chromatid Exchange drug effects

Abstract

Spontaneous and mitomycin C-induced sister chromatid exchanges (SCEs) in lymphocytes were analyzed in 46 healthy persons. Our results suggest that the frequency of spontaneous SCE in lymphocytes is useful for evaluation of the biological effects of environmental mutagens, and that the induced-SCE test with a mutagen and lymphocytes may be used to detect persons with a high sensitivity to the mutagen.

Published

1986

115. Free erythrocyte protoporphyrin (FEP) in a general population, workers exposed to low-level lead, and organic-solvent workers.

Author

Toriumi H and Kawai M

Subjects

Adolescent, Adult, Anemia, Hypochromic blood, Erythrocytes metabolism, Female, Hemoglobins metabolism, Humans, Male, Middle Aged, Sex Factors, Lead Poisoning blood, Occupational Diseases blood, Porphyrins blood, Protoporphyrins blood, Solvents poisoning

Published

1981

116. [Sister chromatid exchanges in lymphocytes and smoking habits].

Author

Nagaya T, Aritaki M, Toriumi H, and Sarai S

Subjects

Adult, Humans, Male, Middle Aged, Lymphocytes ultrastructure, Sister Chromatid Exchange, Smoking

Published

1984