Your search keyword '"Seiji Shibuya"' showing total 63 results

1. Aquaporin 9 expression and its localization in normal skeletal myofiber

Author

Hiroko Kojima, Seiji Shibuya, Yoko Matsuzaki, Shoji Iijima, Takahiro Jimi, Hiroaki Oniki, Masahiko Inoue, Hajime Hara, Yoshihiro Wakayama, and Hisatsugu Masaki

Subjects

Histology, Physiology, Immunoblotting, Muscle Fibers, Skeletal, Immunocytochemistry, Aquaporin, Biology, Aquaporins, Antibodies, Mice, medicine, Animals, Humans, Myocyte, Gel electrophoresis, Messenger RNA, Reverse Transcriptase Polymerase Chain Reaction, Skeletal muscle, Cell Biology, General Medicine, Immunohistochemistry, Molecular biology, Mice, Inbred C57BL, Protein Transport, medicine.anatomical_structure, Real-time polymerase chain reaction, Gene Expression Regulation

Abstract

The examination was performed whether aquaporin (AQP) 9 is expressed in normal skeletal muscle at mRNA and protein levels. Gel electrophoresis of the reverse transcription-polymerase chain reaction (RT-PCR) product of total RNA samples of human normal muscles by oligonucleotide primers for human AQP9 showed a band of 221 basepairs, which corresponded to the basepair length between two primers of AQP9. The nucleotide sequence of RT-PCR product coincided with that of human AQP9. Immunoblot analysis revealed that the rabbit and sheep antibodies against the synthetic peptide of the C-terminal cytoplasmic domain of human AQP9 molecule reacted with a protein of approximately 30 kDa molecular weight in extracts of human normal skeletal muscles. Immunohistochemistry with our anti-AQP9 antibodies showed an immunoreaction at the myofiber surface of both type 1 and type 2 fibers with almost equal staining intensity in human skeletal muscles. The implication of AQP9 expression in skeletal myofibers was discussed.

Published

2009

2. Generation of muscle aquaporin 4 overexpressing transgenic mouse: Its characterization at RNA and protein levels including freeze-fracture study

Author

Seiji Shibuya, Hiroaki Oniki, Teruo Shimizu, Satoru Arata, Takahiro Jimi, Hiroko Ohi, Seiji Shioda, Joji Takahashi, Yoshihiro Wakayama, Masahiko Inoue, Hiroko Kojima, Yoshihide Sunada, and Hajime Hara

Subjects

Genetically modified mouse, Immunoblotting, Gene Expression, General Physics and Astronomy, Mice, Transgenic, Biology, Mice, Structural Biology, Gene expression, Myosin, medicine, Animals, Freeze Fracturing, Myocyte, General Materials Science, RNA, Messenger, Muscle, Skeletal, Aquaporin 4, Reverse Transcriptase Polymerase Chain Reaction, Myocardium, Cardiac muscle, Proteins, Skeletal muscle, Cell Biology, musculoskeletal system, Immunohistochemistry, Molecular biology, Reverse transcription polymerase chain reaction, Microscopy, Electron, medicine.anatomical_structure, Microscopy, Fluorescence, Immunostaining

Abstract

We generated the muscle aquaporin 4 (AQP4) overexpressing transgenic mice in order to investigate the skeletal muscle pathology at RNA and protein levels. At RNA level, the AQP4 mRNA expression of soleus, EDL and cardiac muscles in Tg mice was statistically significantly higher than that in wild mice by the real-time reverse transcription polymerase chain reaction method. At protein level examinations, we used the immunoblot, immunohistochemistry and freeze-fracture electron microscopy. The immunoblot showed the single band of 31kDa with anti-AQP4 antibody in the extracts of soleus and EDL muscles of wild mice but not in extract of wild cardiac muscle; while the reaction band was noted in cardiac muscle of Tg mice and the reaction band was stronger in the extracts of soleus and EDL muscles of Tg mice. The immunohistochemistry showed that the expression of AQP4 at the myofiber surface of soleus and EDL muscles of Tg mice was more marked than that of wild mice and, interestingly, the AQP4 expression of these muscles of Tg mice appeared to be more remarkable in type 1 slow twitch myofibers as judged by the positive slow myosin immunostaining of adjacent serial sections. The immunofluorescence staining with anti-AQP4 antibody of cardiac muscles of wild mice revealed the scarcely immunopositive myofibers; whereas the immunostaining cardiac muscles of Tg mice contained the numerous AQP4 immunopositive myofibers. The freeze-fracture electron microscopy demonstrated that the orthogonal array densities in soleus and EDL muscle plasma membranes of Tg mice were significantly higher than those of wild mice and that the orthogonal array like particle density of cardiac muscle plasma membranes of Tg mice appeared to be more numerous than that of cardiac myofibers of wild mice. Finally the clinical phenotype of Tg mice appeared to be similar to that of wild mice. Further physiological examination with devices may suggest some about the physiological difference.

Published

2007

3. Aquaporin 1: Examination of Its Expression and Localization in Normal Human Skeletal Muscle Tissue

Author

Yoko Matsuzaki, Hiroko Kojima, Hiroaki Oniki, Masahiko Inoue, Yoshihiro Wakayama, Joji Takahashi, Hajime Hara, Seiji Shibuya, and Takahiro Jimi

Subjects

Histology, Immunoelectron microscopy, Biology, Antibodies, Reference Values, Immunoblot Analysis, Image Processing, Computer-Assisted, medicine, Humans, Myocyte, Microscopy, Immunoelectron, Muscle, Skeletal, Aquaporin 1, Reverse Transcriptase Polymerase Chain Reaction, Cell Membrane, Infant, Newborn, Skeletal muscle, Immunogold labelling, Immunohistochemistry, Molecular biology, medicine.anatomical_structure, Gene Expression Regulation, RNA, Endothelium, Vascular, Anatomy, ITGA7

Abstract

To examine aquaporin 1 (AQP1) expression in skeletal muscle tissue precisely, we performed reverse transcription-polymerase chain reaction (RT-PCR) at RNA level and immunoblot analysis, immunohistochemistry and immunoelectron microscopy at protein level. The RT-PCR study of total RNA from normal human skeletal muscle showed a strong single band of AQP1. At the protein level we used two commercially available antibodies, both of which recognize the cytoplasmic domain of the AQP1 molecule. One antibody gave positive results. Immunoblot of muscle extract showed a 30-kDa band protein, the molecular weight of which corresponded to that of AQP1. Immunohistochemically, AQP1 was immunostained at the myofiber surface both in type 1 and type 2 myofibers with almost the same intensity, and its staining pattern was rather diffuse and irregular compared with that of the anti-dystrophin antibody. The endomysial endothelial cells were also immunolabeled. Immunoelectron microscopy revealed that the immunogold particles indicating the presence of the AQP1 molecule were present along the inside surface of the muscle plasma membrane. However, another antibody showed negative results except for the endomysial endothelial cells which were positively stained. We drew the conclusion that AQP1 is expressed at the endomysial capillary endothelial cell and further AQP1 may be expressed at the human skeletal myofiber plasma membrane.

Published

2006

4. Expression of Myoferlin in Skeletal Muscles of Patients with Dysferlinopathy

Author

Hiroko Kojima, Masahiko Inoue, Hiroaki Oniki, Ichizo Nishino, Yoshihiro Wakayama, Seiji Shibuya, Takahiro Jimi, and Ikuya Nonaka

Subjects

Dysferlinopathy, Pathology, medicine.medical_specialty, Biopsy, Immunoblotting, Muscle Proteins, Gene mutation, Muscular Dystrophies, General Biochemistry, Genetics and Molecular Biology, Quadriceps Muscle, Dysferlin, Utrophin, medicine, Humans, Myocyte, Fluorescent Antibody Technique, Indirect, Microscopy, Immunoelectron, biology, Calcium-Binding Proteins, Membrane Proteins, General Medicine, medicine.disease, Immunohistochemistry, biology.protein, Dystrophin, Immunostaining, Limb-girdle muscular dystrophy

Abstract

Myoferlin is a novel protein of unknown function with high homology to dysferlin, the gene mutations of which cause limb girdle muscular dystrophy type 2B and Miyoshi myopathy. The myoferlin gene seems to be a candidate for the modifier, and because of the high homology to dysferlin myoferlin may work as a compensator for the absence of dysferlin in dysferlinopathy. This hypothesis is based on the observation that utrophin, which has 80% homology with dystrophin, is overexpressing in the dystrophin deficient myofibers. To test this hypothesis, we investigated the myoferlin expression by immunoblot and immunohistochemical analysis in muscles of five patients with dysferlinopathy. For this aim, we generated a myoferlin specific antibody that does not cross react with dysferlin, and performed the immunoblot, immunohistochemical and immunoelectron microscopic studies. Immunohistochemical analysis showed that the antibodies against myoferlin and dysferlin clearly stained the normal human myofiber surface membranes. The electron microscopy of single immunogold labeled samples for myoferlin showed the presence of the molecular signal along the normal muscle cell membrane. Immunoblot analysis showed that the intensity of 230-kDa myoferlin band of dysferlinopathy muscle extracts was similar to that of normal muscle extracts. The immunostaining of dysferlinopathy muscles with anti-myoferlin antibody revealed a weak immunoreactivity along the muscle cell surface. Thus, the compensatory overexpression of myoferlin was not detected in muscles with dysferlinopathy.

Published

2006

5. Alterations of molecular architectures in skeletal muscle plasma membranes of dehydrated and water-loaded mice

Author

Hiroaki Oniki, Masahiko Inoue, Yoshihiro Wakayama, and Seiji Shibuya

Subjects

Male, Dehydration, Cell Membrane, Water, Skeletal muscle, General Medicine, Biology, Caveolae, Molecular medicine, Pathology and Forensic Medicine, Cell biology, Mice, Membrane, Aquaporin 4, medicine.anatomical_structure, Biochemistry, Intramembranous ossification, Ultrastructure, medicine, Animals, Muscle, Skeletal, Molecular Biology, Homeostasis

Abstract

It is likely that orthogonal arrays (OAs) and caveolae seen on the replicas of freeze-fractured muscle plasma membranes are involved in maintaining osmotic homeostasis. Therefore, using the freeze-fracture technique, we examined the ultrastructural changes in OAs and caveolae of the skeletal muscle plasma membrane of dehydrated and water-loaded mice. In the muscle plasma membranes of 6 dehydrated and 6 water-loaded mice, caveolar distribution was not altered, and the densities of caveolae and OAs did not show statistically significant differences when compared with those in 6 control mice, although the skeletal muscles of water-loaded mice sometimes had muscle plasma membranes with extremely numerous OAs. In contrast, the muscle plasma membranes of dehydrated mice often revealed changes in the distribution of OAs, which existed in a group at the confined area of the muscle plasma membranes and were frequently accompanied by the aggregations of intramembranous particles (IMPs) around OAs. Thus, on the basis of the present study, we suggest that OAs in skeletal muscles as well as those in brain may play an important role in maintaining osmotic homeostasis of these organs under abnormal water balance.

Published

2005

6. Altered aquaporin 4 expression in muscles of Fukuyama-type congenital muscular dystrophy

Author

Takahiro Jimi, Sumimasa Yamashita, Makoto Murahashi, Hiroko Kojima, Seiji Shibuya, Manabu Inoue, Hajime Hara, Yoshihiro Wakayama, and T Kumagai

Subjects

medicine.medical_specialty, Pathology, Immunoblotting, Aquaporins, Muscular Dystrophies, Pathology and Forensic Medicine, medicine, Humans, RNA, Messenger, Muscular dystrophy, Muscle, Skeletal, Molecular Biology, Aquaporin 4, Messenger RNA, biology, Reverse Transcriptase Polymerase Chain Reaction, Anatomical pathology, Cell Biology, General Medicine, medicine.disease, Immunohistochemistry, biology.protein, Congenital muscular dystrophy, sense organs, Antibody, Immunostaining

Abstract

This study was undertaken to investigate the expression of aquaporin 4 (AQP4) in the muscle plasma membrane of children with Fukuyama-type congenital muscular dystrophy (FCMD) at protein and mRNA levels. The biopsied six muscles with FCMD, six histochemically normal muscles and eight disease control muscles were analyzed by means of immunoblots, immunohistochemistry and reverse-transcription polymerase chain reaction (RT-PCR). Immunoblots showed that the band of FCMD muscle extracts stained with anti-AQP4 antibody was faint in comparison with that of normal muscle extracts. The immunohistochemistry revealed that most of the FCMD myofibers showed negative immunostaining with anti-AQP4 antibody, although the partially positive immunostaining of sporadic FCMD myofibers was noted. The immunoreactivity was positive with anti-dystrophin and anti-beta-spectrin antibodies in almost all FCMD myofibers. The quantitative RT-PCR demonstrated that the AQP4 mRNA level of the FCMD muscles was markedly reduced. On the basis of these findings, we conclude that the expression of AQP4 in FCMD myofibers is reduced and the reduced content of AQP4 mRNA in FCMD muscles may be related to the decreased expression of AQP4 at the muscle plasma membrane of FCMD myofibers.

Published

2003

7. Reduced density of intramembranous particle clusters: freeze-fracture study of mdx mouse muscle plasma membrane

Author

Hiroaki Oniki, Seiji Shibuya, and Yoshihiro Wakayama

Subjects

mdx mouse, Protein subunit, Mice, polycyclic compounds, Animals, Freeze Fracturing, Muscle, Skeletal, Integral membrane protein, chemistry.chemical_classification, biology, Chemistry, Cell Membrane, biochemical phenomena, metabolism, and nutrition, musculoskeletal system, Mice, Inbred C57BL, Muscular Dystrophy, Duchenne, Protoplasm, Disease Models, Animal, Microscopy, Electron, enzymes and coenzymes (carbohydrates), Membrane, Membrane protein, Biochemistry, Mice, Inbred mdx, biology.protein, Biophysics, bacteria, Anatomy, Dystrophin, Glycoprotein

Abstract

Our previous freeze-fracture study demonstrated the decreased density of intramembranous particles (IMPs) on the protoplasmic (P) face of muscle plasma membranes in mdx mice. However, the molecular mechanism is unknown. In the present freeze-fracture study, we examined whether the reduced P-face IMP density in mdx mice would be caused by depletion of the rosette-like IMP clusters, which are IMP aggregations differing from crystal-like orthogonal arrays (OAs). By comparison with control mice, the P-face plasma membranes of extensor digitorum longus (EDL) and soleus (SOL) muscles of mdx mice demonstrated the following findings: (1) decreased IMP density with subunit particles of OAs and IMP clusters, (2) decreased IMP density without subunit particles of OAs, (3) normal IMP density without subunit particles of OAs and IMP clusters, (4) decreased OA density in EDL muscles and normal OA density in SOL muscles, and (5) decreased IMP cluster densities in both muscles. Thus, the reduced IMP density of P-face muscle plasma membranes in mdx mice may result from the decreased IMP clusters, suggesting the relationship between IMP clusters and the integral membrane proteins is influenced by dystrophin deficiency such as that of dystrophin-associated glycoproteins or other membrane proteins.

Published

2003

8. Changes in the distribution and density of caveolin 3 molecules at the plasma membrane of mdx mouse skeletal muscles: a fracture-label electron microscopic study

Author

Seiji Shibuya, Yoshihiro Wakayama, Masahiko Inoue, Eiki Kominami, and Hiroaki Oniki

Subjects

mdx mouse, Caveolin 3, Ratón, Caveolins, Dystrophin, Mice, Sarcolemma, Caveolae, medicine, Animals, Muscle, Skeletal, biology, General Neuroscience, Cell Membrane, Skeletal muscle, musculoskeletal system, Microscopy, Electron, Membrane, medicine.anatomical_structure, Biochemistry, Mice, Inbred mdx, biology.protein, Biophysics

Abstract

To analyze the molecular mechanism of the increased caveolin 3 activities in dystrophin-deficient muscles, we investigated three-dimensionally the changes in caveolin 3 molecular distribution and density at the sarcolemma of mdx mice by the fracture-label electron microscopic technique. At the sarcolemma of skeletal muscles from mdx mice, the densities of gold particles associated with caveolae, non-associated with caveolae and arranged circularly without caveolae were higher than those in control mice (P

Published

2002

9. [Untitled]

Author

Seiji Shibuya, Masahiko Inoue, Hiroaki Oniki, Yoshihiro Wakayama, Hiroko Kojima, Takahiro Jimi, Makoto Murahashi, and Hajime Hara

Subjects

Gel electrophoresis, Messenger RNA, Nucleic acid sequence, Skeletal muscle, Cell Biology, Immunogold labelling, Biology, Molecular biology, Reverse transcription polymerase chain reaction, medicine.anatomical_structure, Aquaporin 3, Biochemistry, Immunoblot Analysis, medicine, Anatomy

Abstract

The question whether aquaporin 3 (AQP3) is expressed in normal human skeletal muscle at mRNA and protein levels has been examined, since AQP3 has been reported to be coexpressed with AQP4 in various kinds of tissues other than skeletal muscle. The gel electrophoresis of the reverse transcription polymerase chain reaction (RT-PCR) product of total RNA samples extracted from normal human muscle specimens by using the oligonucleotide primers for AQP3 contained a band of 629 base pairs which corresponded to the base pair length between two primers of AQP3. The nucleotide sequence of this RT-PCR product coincided with that of AQP3. At the protein level, immunoblot, immunohistochemical and immunoelectron microscopical studies were done by using rabbit antibody against the synthetic peptide of the cytoplasmic domain of the human AQP3 molecule. Immunoblot analysis showed that rabbit antibody against the human AQP3 reacted with a protein of approximately 30 kDa molecular weight in extracts of normal human skeletal muscles. The immunoreaction for the anti-AQP3 antibody with normal human muscle was noted at the myofibre surface. Immunogold labelling electron microscopy revealed that the gold particles indicating the presence of AQP3 molecules were located mainly at the inside surface of muscle plasma membrane.

Published

2002

10. Aciculin and its relation to dystrophin: immunocytochemical studies in human normal and Duchenne dystrophy quadriceps muscles

Author

Hiroaki Oniki, Hiroko Kojima, Manabu Inoue, Yoshihiro Wakayama, Makoto Murahashi, Seiji Shibuya, and Sumimasa Yamashita

Subjects

Male, musculoskeletal diseases, medicine.drug_class, Duchenne muscular dystrophy, Muscle Fibers, Skeletal, Biology, Monoclonal antibody, Epitope, Pathology and Forensic Medicine, Dystrophin, Cellular and Molecular Neuroscience, medicine, Humans, Myocyte, Child, Muscle, Skeletal, Infant, Immunogold labelling, medicine.disease, Molecular biology, Muscular Dystrophy, Duchenne, Cytoskeletal Proteins, Phosphoglucomutase, Thigh, Child, Preschool, biology.protein, Immunohistochemistry, Neurology (clinical), Antibody

Abstract

Aciculin is a novel adherens junction antigen extracted from human uterine smooth muscle that is reported to associate biochemically with dystrophin. We attempted to determine (i) the immunostainability of anti-aciculin antibody for the 6 histochemically normal human muscles and seven muscles from boys with Duchenne muscular dystrophy (DMD) and 11 disease control muscles, (ii) the ultrastructural localization of aciculin in normal skeletal myofibers, (iii) aciculin's spacial relationship with dystrophin and beta-spectrin, and (iv) if the aciculin is ultrastructurally colocalized with dystrophin, the distance from the aciculin epitope to the epitope of the dystrophin N- or C-terminal domain. For this, rabbit anti-aciculin antibody was generated against the synthetic peptide of aciculin fragment D [4]. Immunohistochemical staining showed that the immunostainability of DMD muscles for anti-aciculin antibody was markedly decreased as compared with normal and disease control muscles. Single and double immunogold labeling electron microscopy of 6 histochemically normal human quadriceps femoris muscles revealed that aciculin was present along the inner surface of muscle plasma membrane and that aciculin formed doublets more frequently with dystrophin (23.5 +/- 1.8%; group mean +/- SE) than with beta-spectrin (12.8 +/- 1.1%; P0.01 two tailed t test). Rabbit anti-aciculin antibody frequently formed doublets with monoclonal antibodies against the N- or C-terminal domain of dystrophin at the muscle cell surface. These results suggest that aciculin is associated with dystrophin and may interact with both the N- and C-terminal domains of dystrophin.

Published

2000

11. Aquaporin-4 is absent at the sarcolemma and at perivascular astrocyte endfeet in α1-syntrophin knockout mice

Author

Shuhei Kameya, Yuko Miyagoe, Kayoko Tsukita, Toshifumi Yokota, Yukio Hosaka, Shin'ichi Takeda, Ryoichi Matsuda, Seiji Shibuya, and Yoshihiro Wakayama

Subjects

Kidney, Sarcolemma, PDZ domain, General Physics and Astronomy, General Medicine, Biology, musculoskeletal system, Cell biology, medicine.anatomical_structure, Aquaporin 4, Knockout mouse, Immunology, cardiovascular system, medicine, Immunohistochemistry, sense organs, General Agricultural and Biological Sciences, tissues, Astrocyte, Syntrophin

Abstract

α1-Syntrophin, a member of dystrophin-associated proteins, is expressed at the sarcolemma and at perivascular astrocytes, and participates in protein-protein interactions through its PDZ domain. Aquaporin-4 (AQP4) is the predominant water channel protein in the brain, and also expressed at the sarcolemma of fast-twitch muscle fibers. AQP4 is concentrated in orthogonal array particles (OAPs), and its expression has been reported to be decreased at the sarcolemma of dystrophin-deficient mdx mice. We examined whether α1-syntrophin targets AQP4 at the sarcolemma. Immunohistochemistry showed that AQP4 is absent at the sarcolemma in α1-syntrophin knockout mice and that its expression is also lost from the perivascular astrocyte endfeet. On the other hand, expression of AQP4 is not decreased at the sarcolemma of the knockout mice in the neonatal stage. Moreover, AQP4 is expressed in lung, stomach, and kidney of wild-type and α1-syntrophin null mice. Our results show that α1-syntrophin is a key molecule to localize AQP4 to the sarcolemma of mature fast myofibers and astrocyte endfeet, but AQP4 is targeted to the plasma membrane by different molecules in lung, stomach, and kidney.

Published

2000

12. A Study of Swallowing Function in Stroke Patients Using Videofluorography and Double Contrast Pharyngogram by Computed Radiography

Author

Seiji Shibuya, Tsukasa Fujimoto, Yoshihiro Wakayama, Jun-ichiro Asai, and Makoto Murahashi

Subjects

medicine.medical_specialty, Swallowing, Stroke patient, business.industry, media_common.quotation_subject, Contrast (vision), Medicine, Radiology, Pharyngogram, Computed radiography, business, media_common

Published

1999

13. Freeze-fracture studies of muscle plasma membranes in myopathic patients with hypo-and hyperthyroidism

Author

Masahiko Inoue, Seiji Shibuya, Yoshihiro Wakayama, Makoto Murahasi, and Hiroaki Oniki

Subjects

endocrine system, medicine.medical_specialty, endocrine system diseases, Chemistry, Thyroid, Skeletal muscle, General Medicine, Pathology and Forensic Medicine, chemistry.chemical_compound, Endocrinology, Digitonin, medicine.anatomical_structure, Membrane, Caveolae, Internal medicine, medicine, Cytochemistry, Anatomy, medicine.symptom, Myopathy, Molecular Biology, Hormone

Abstract

To examine the influence of thyroid hormone on the skeletal muscle plasma membrane, we analyzed the changes in ultrastructural architecture and membrane area complexed with digitonin of muscle plasma membrane in myopathic patients with hypo-and hyperthyroidism by the conventional freeze-fracture (F-F) technique and F-F cytochemistry using the sterol-specific ligand digitonin. The densities of flask-shaped invaginations, which are mainly thought to correspond to caveolae, intramembranous particles, and orthogonal arrays, and the changes of digitoninreacted membrane areas in the muscle plasma membranes in three patients with hypothyroid myopathy and one patient with both myasthenia gravis and hyperthyroidism were compared with those in age-matched controls. In the conventional F-F study, the muscle plasma membrane of hypothyroid patients showed increased invagination density, whereas that of the hyperthyroid patient was normal ultrastructurally. In the F-F cytochemistry study, however, the ratio of digitonin-reacted membrane areas versus fractured membrane areas was not different between hypothyroid patients and controls, whereas that of the hyperthyroid patient was lowered in comparison with that of control. These results suggest that thyroid hormone may alter the biochemical properties and ultrastructural architecture of muscle plasma membrane.

Published

1998

14. Electron microscopic observations of triple immunogold labelling for dystrophin, β-dystroglycan and adhalin in human skeletal myofibers

Author

Takahiro Jimi, Hiroaki Oniki, Hiroko Kojima, Seiji Shibuya, Masahiko Inoue, Yoshihiro Wakayama, and Makoto Murahashi

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, Duchenne muscular dystrophy, Immunoblotting, Muscle Fibers, Skeletal, Pathology and Forensic Medicine, Dystrophin, Cellular and Molecular Neuroscience, Sarcoglycans, Utrophin, medicine, Humans, Dystroglycans, Microscopy, Immunoelectron, Muscle, Skeletal, Cytoskeleton, chemistry.chemical_classification, Membrane Glycoproteins, biology, Immunogold labelling, musculoskeletal system, medicine.disease, Immunohistochemistry, Molecular biology, Transmembrane protein, Cytoskeletal Proteins, Microscopy, Electron, chemistry, Membrane protein, biology.protein, Neurology (clinical), Glycoprotein

Abstract

Dystrophin is the Duchenne muscular dystrophy gene product and is a membrane cytoskeletal protein present in the network of the plasma membrane undercoat. Adhalin (50 kDa dystrophin-associated glycoprotein) and beta-dystroglycan (43 kDa dystrophin-associated glycoprotein) are the transmembrane components of the normal muscle plasma membrane, and beta-dystroglycan has been demonstrated to bind dystrophin at the inside surface of normal muscle plasma membrane. This investigation was undertaken to test whether the epitopes of dystrophin, beta-dystroglycan and adhalin are closely associated with each other by using triple immunogold labelling electron microscopy on normal human skeletal myofibers. Although closely associated signals of triplet immunogold particles were observed, there were less numerous than expected. However, closely associated signals of two epitopes of dystrophin and beta-dystroglycan, dystrophin and adhalin, or adhalin and beta-dystroglycan were frequently observed. These ultrastructural findings are consistent with biochemical evidence implying that dystrophin, beta-dystroglycan and adhalin are closely associated with each other at the normal muscle plasma membrane.

Published

1996

15. Ultrastructural localization of adhalin in normal murine skeletal myofiber

Author

Makoto Murahashi, Takahiro Jimi, Hiroko Kojima, Seiji Shibuya, Masahiko Inoue, Hiroaki Oniki, and Yoshihiro Wakayama

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, animal structures, Immunoelectron microscopy, Blotting, Western, Muscle Fibers, Skeletal, Sarcoplasm, Biology, law.invention, Dystrophin, Mice, Reference Values, law, Sarcoglycans, Animals, Myocyte, Tissue Distribution, Dystroglycans, Microscopy, Immunoelectron, Muscle, Skeletal, Membrane Glycoproteins, Spectrin, musculoskeletal system, Immunohistochemistry, Molecular biology, Cell biology, Mice, Inbred C57BL, Cytoskeletal Proteins, Neurology, Ultrastructure, biology.protein, Neurology (clinical), Electron microscope, Myofibril

Abstract

The ultrastructural localization of adhalin and its relations to dystrophin, beta-dystroglycan, and beta-spectrin were studied in normal murine skeletal myofibers. The C-terminal peptides of adhalin and beta-dystroglycan were synthesized based on their cDNAs, and the affinity-purified antibodies against these peptides were produced. Single-immunolabeling electron microscopy showed that the adhalin was located just inside the muscle plasma membrane or inside the myofiber a short distance from the plasma membrane. The adhalin signal was also noted at the sarcoplasmic side of plasmalemmal invaginations or at vesicular structures in subsarcolemmal areas. Double-immunogold-labeling electron microscopy disclosed a similar localization of dystrophin, beta-dystroglycan, and beta-spectrin. The close association of adhalin with dystrophin or beta-dystroglycan was demonstrated by formation of doublets by signals of antibodies of adhalin with those of dystrophin or beta-dystroglycan and was confirmed by statistical analyses. This study demonstrated that the location of adhalin is close to that of dystrophin and beta-dystroglycan at the muscle plasma membrane.

Published

1996

16. Observations of muscle plasma membrane undercoats in Duchenne and fukuyama muscula dystrophies

Author

Takuya Kobayashi, Sumimasa Yamashita, Shota Miyake, Hiroaki Oniki, Nobuko Misugi, Takahiro Jimi, Makoto Murahashi, Seiji Shibuya, Yoshihiro Wakayama, and Toshiyuki Kumagai

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, Membrane, Chemistry, Duchenne muscular dystrophy, Fukuyama congenital muscular dystrophy, medicine, General Medicine, Anatomy, medicine.disease, Molecular Biology, Pathology and Forensic Medicine

Abstract

Muscle plasma membrane undercoats were investigated by conventional electron microscopy in both Duchenne muscular dystrophy (DMD) and Fukuyama congenital muscular dystrophy (FCMD). The densities of the plasma membrane undercoats were rarefied in the parts of the plasma membranes overlying the degenerating focus in both DMD and FCMD myofibers. The degree of rarefaction tended to be parallel to the degree of degeneration in the myofibers. It was hard to distinguish the undercoat densities of normal-looking myofibers of DMD and FCMD muscles from those of control myofibers from histochemically-normal muscles. On the other hand, the undercoats of regenerating myofibers in DMD and FCMD muscles were denser than normal.

Published

1995

17. Altered distribution of ?-Dystroglycan in sarcolemma of human dystrophic muscles: An immunohistochemical study

Author

Nobuko Misugi, Takahiro Jimi, Yoshiyuki Kuroiwa, Sumimasa Yamashita, Atsushi Takeda, Osamu Hasegawa, Yume Suzuki, Seiji Shibuya, Toshiyuki Kumagai, Yoshihiro Wakayama, and Takuya Kobayashi

Subjects

medicine.medical_specialty, Physiology, Biopsy, Duchenne muscular dystrophy, Blotting, Western, Muscular Dystrophies, Dystrophin, Dystroglycans, Cellular and Molecular Neuroscience, Sarcolemma, Physiology (medical), Internal medicine, medicine, Animals, Humans, Muscle, Skeletal, Cytoskeleton, chemistry.chemical_classification, Membrane Glycoproteins, Sheep, biology, medicine.disease, Immunohistochemistry, Cell biology, Cytoskeletal Proteins, Membrane glycoproteins, Endocrinology, chemistry, biology.protein, Neurology (clinical), Glycoprotein

Published

1995

18. Freeze–fracture analysis of muscle plasma membrane in Becker's muscular dystrophy

Author

Yoshiyuki Kuroiwa, Takahiro Jimi, Seiji Shibuya, T. Kobayashi, Yoshihiro Wakayama, T Kumagai, Yume Suzuki, N Misugi, Hiroaki Oniki, and Osamu Hasegawa

Subjects

Adult, musculoskeletal diseases, medicine.medical_specialty, Histology, Adolescent, Becker's muscular dystrophy, Muscular Dystrophies, Pathology and Forensic Medicine, Physiology (medical), Internal medicine, medicine, Extracellular, Freeze Fracturing, Humans, Clinical severity, Muscular dystrophy, Diminution, biology, Chemistry, Muscles, musculoskeletal, neural, and ocular physiology, Cell Membrane, Skeletal muscle, Anatomy, medicine.disease, Microscopy, Electron, Membrane, medicine.anatomical_structure, Endocrinology, Neurology, biology.protein, Neurology (clinical), Dystrophin

Abstract

The intramembranous particle (IMP), orthogonal array (OA) and orthogonal array subunit particle (OASP) densities in skeletal muscle plasma membranes from eight patients with Becker's muscular dystrophy (BMD) were analysed by the freeze-fracture technique. The results showed almost normal IMP density with the significant decrease of OA and OASP densities in BMD. The group mean densities +/- SE of IMPs on the protoplasmic faces with and without OASPs, and on extracellular faces/microns 2 were 2137 +/- 207, 1839 +/- 68 and 895 +/- 108, respectively in controls; whereas those of BMD were 1989 +/- 259, 1837 +/- 203 and 900 +/- 239, respectively (P > 0.1 by two-tailed t-test). The group median density of OAs and their pits/microns 2 was 4.89 with mid-ranges (25-75% values of the counts) of 2.66-10.18 in controls; whereas that in BMD was 2.15 with mid-ranges of 1.14-4.31 (P < 0.01 by Wilcoxon rank-sum test). The group mean density +/- SE of OASPs in controls was 15.99 +/- 1.83; whereas that in BMD was 13.47 +/- 1.07 (P < 0.01 by two-tailed t-test). However, the diminution of OA and OASP densities in BMD muscle plasma membranes was not as severe as in Duchenne's muscular dystrophy. There was a relationship between OA density and clinical severity in BMD patients; the decrease of OA density in a severe BMD patient was more marked than that in mildly affected BMD patients. Therefore, it seems that marked depletion of OA density may lead to the severe disability in muscular dystrophies.

Published

1994

19. STRONG IMMUNOREACTIVITY OF CATHEPSIN L AT THE SITE OF RIMMED VACUOLES IN DISEASED MUSCLES

Author

Takahiro Jimi, Yoshihiro Wakayama, Seiji Shibuya, Atsushi Takeda, Koujiro Sugita, and Yutaka Satoh

Subjects

Adult, Male, Pathology, medicine.medical_specialty, Cathepsin L, Immunoblotting, Vacuole, Cathepsin B, Muscular Diseases, Cathepsin H, Endopeptidases, medicine, Humans, Aged, Cathepsin, biology, Rimmed vacuoles, Skeletal muscle, Middle Aged, Cathepsins, Immunohistochemistry, Cysteine Endopeptidases, medicine.anatomical_structure, Vacuoles, biology.protein, Female, Neurology (clinical), Lysosomes, Immunostaining

Abstract

Skeletal muscle samples from four patients with myopathies showing autophagic vacuole formation were examined by immunohistochemical, biochemical and immunoblot analyses. Immunochemical studies demonstrated strongly positive reactions of cathepsins B and L in and around the rimmed vacuoles and weak reactions in intramyofibral portions of degenerating muscle fibres. Faint staining of cathepsin H was also seen at the sites of rimmed vacuoles. Biochemical analyses showed increased activity of cathepsin B and L in muscle specimens from the patients with rimmed vacuole formation. However, there was no remarkable cathepsin H activity in the muscle specimens from these patients. Cathepsin L immunoblot analysis of muscle extracts showed three bands with molecular masses of 30 kDa, 36 kDa and 39 kDa. The immunostaining of cathepsin L from patients with rimmed vacuole formation was stronger than that of normal controls. Cathepsin B immunoblot analysis showed only faint bands in samples from patients with rimmed vacuole formation and normal controls. This study demonstrated, for the first time, strong immunoreactivity of cathepsin L at the sites of rimmed vacuoles. Possible mechanisms of rimmed vacuole formation are discussed.

Published

1992

20. Skeletal muscle syntrophin interactors revealed by yeast two-hybrid assay

Author

Masahiko, Inoue, Yoshihiro, Wakayama, Takahiro, Jimi, Seiji, Shibuya, Hajime, Hara, Akihiko, Unaki, and Kiyokazu, Kenmochi

Subjects

Aquaporin 4, Mice, Base Sequence, Two-Hybrid System Techniques, Dystrophin-Associated Proteins, Animals, Humans, Protein Isoforms, Protein Interaction Domains and Motifs, In Vitro Techniques, Muscle, Skeletal, Recombinant Proteins, DNA Primers

Abstract

Syntrophins are the cytoplasmic peripheral proteins of dystrophin glycoprotein complex, of which five (alpha l, beta 1, beta 2, gamma 1 and gamma 2) isoforms have been identified so far. Respective syntrophin isoforms are encoded by different genes but have similar domain structures. At the sarcolemma of skeletal muscle, the most abundant alpha l-syntrophin was shown to interact at its PDZ domain with many membrane proteins. Among them, the AQP4 interaction with alpha 1-syntrophin PDZ domain was demonstrated by a Tg mouse study, prompting us to investigate the interaction between mouse alpha l-syntrophin (BC018546: nt.267-492, PDZ domain) pEXP-AD502 as prey vector and mouse AQP4 (NM009700: nt.805-969) pDBLeu as bait vector by the yeast two-hybrid assay, resulting in a negative study. We further studied the binding partner of another sarcolemma located beta 1-syntrophin, and performed a yeast two-hybrid experiment. With human beta 1-syntrophin as bait and human skeletal muscle cDNA library as prey, we obtained one positive clone which turned out to be alpha-dystrobrevin. Although the interaction of human beta 1-syntrophin with alpha-dystrobrevin has already been shown by immunoprecipitation assay, we have here confirmed this interaction by a yeast two-hybrid experiment.

Published

2008

21. Aquaporin 4 mRNA levels in neuromuscular tissues of wild-type and dystrophin-deficient mice

Author

Yoko Matsuzaki, Hajime Hara, Masahiko Inoue, Takahiro Jimi, Yoshihiro Wakayama, and Seiji Shibuya

Subjects

Muscle tissue, mdx mouse, medicine.medical_specialty, Pathology, Duchenne muscular dystrophy, General Biochemistry, Genetics and Molecular Biology, Dystrophin, Mice, Internal medicine, medicine, Animals, RNA, Messenger, Muscular dystrophy, Muscle, Skeletal, DNA Primers, Aquaporin 4, biology, Reverse Transcriptase Polymerase Chain Reaction, Skeletal muscle, Brain, Heart, General Medicine, Muscular Dystrophy, Animal, musculoskeletal system, medicine.disease, Quadriceps femoris muscle, medicine.anatomical_structure, Endocrinology, biology.protein, sense organs

Abstract

Aquaporin (AQP) 4 is a water-specific channel protein and is abundant in central nervous tissues and skeletal muscles. Recently, the AQP4 molecule has been increasingly highlighted in its pathophysiological role of several neurological diseases, such as stroke, muscular dystrophy and neuromyelitis optica. We therefore measured the levels of AQP4 mRNA and glyceraldehyde-3 phosphate dehydrogenase mRNA (an internal control) in muscle and brain tissues of wild-type mice (C57BL10/ScSn) and age-matched dystrophin-deficient mdx mice (C57BL10/ScSn mdx) by real-time quantitative RT-PCR. The relative AQP4 mRNA level was highest in the spinal cord among the neuromuscular tissues examined in wild-type mice. Among the muscle tissues of wild-type mice, the relative AQP4 mRNA level was higher in extensor digitorum longus (EDL) muscles, and its descending order was EDL, quadriceps femoris, soleus and heart muscles. It is noteworthy that there was no difference in the relative AQP4 mRNA levels in the brain tissues between wild-type mice and age-matched mdx mice. In contrast, the AQP4 mRNA level in the quadriceps femoris muscle was significantly lower in mdx mice than in wild-type mice. The fact that the spinal cord contains the highest AQP4 mRNA may be related to the pathogenesis of neuromyelitis optica, in which AQP4 protein is the target antigen. In addition, the low expression level of AQP4 mRNA in the mdx mouse muscle suggests a functional link between AQP4 and dystrophin in the muscle tissue. We suggest that a similar pathomechanism may underlie the phenotypic consequences of the mdx mouse and Duchenne muscular dystrophy.

Published

2008

22. The relationship between intramembranous particles and aquaporin molecules in the plasma membranes of normal rat skeletal muscles: a fracture-label study

Author

Yoshihiro Wakayama, Hiroaki Oniki, Masahiko Inoue, Seiji Shibuya, and Hiroko Kojima

Subjects

Immunoblotting, Aquaporin, Biology, medicine, Animals, Freeze Fracturing, Microscopy, Immunoelectron, Muscle, Skeletal, Instrumentation, Aquaporin 4, Aquaporin 3, Cell Membrane, Skeletal muscle, Rats, Membrane, medicine.anatomical_structure, Membrane protein, Biochemistry, Intramembranous ossification, Biophysics, sense organs, Gold, Rabbits, Homeostasis

Abstract

The plasma membrane of skeletal muscles contains water channels such as aquaporin 4 (AQP4), aquaporin 3 (AQP3) and aquaporin 7 (AQP7). In dehydrated mice, we have recently reported the altered distribution of the aggregations of intramembranous particles (IMPs), such as orthogonal array (a crystal-like structure) and IMP cluster (a rosette-like structure) on the freeze-fractured skeletal muscle plasma membranes. In this fracture-label study, we first tested whether the orthogonal arrays (OAs) were composed of AQP4 in skeletal muscles and further analyzed the relationship between IMPs including IMP clusters and AQP3 molecules. As a result, many of the gold particles indicating AQP4 was associated with OAs (79%) by our fracture-label technique. On the other hand, approximately 50% of gold particles indicating AQP3 were associated with IMP clusters. Thus we confirmed that the OAs are composed of AQP4 in skeletal muscles, and further demonstrated that some of the IMP clusters are composed of AQP3 and may participate in maintaining osmotic homeostasis in skeletal myofibers. The fracture-label method is useful in investigating the molecular identification of membrane proteins such as AQP3 and AQP4.

Published

2006

23. Sarcospan: ultrastructural localization and its relation to the sarcoglycan subcomplex

Author

Masahiko Inoue, Hajime Hara, Hiroaki Oniki, Hiroko Kojima, Takahiro Jimi, Seiji Shibuya, Yoshihiro Wakayama, and Koutarou Hayashi

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, General Physics and Astronomy, Biology, Immunofluorescence, Antibodies, Sarcospan, Structural Biology, Sarcoglycans, medicine, Myocyte, Animals, Humans, General Materials Science, Microscopy, Immunoelectron, Muscle, Skeletal, chemistry.chemical_classification, Sheep, medicine.diagnostic_test, Membrane Proteins, Cell Biology, Immunogold labelling, musculoskeletal system, Molecular biology, Transmembrane protein, Cell biology, Neoplasm Proteins, Sarcoglycan, chemistry, Microscopy, Fluorescence, Polyclonal antibodies, biology.protein, Rabbits, Glycoprotein, Carrier Proteins

Abstract

Sarcospan is a 25 kDa transmembrane component of dystrophin-associated glycoprotein. We generated a rabbit polyclonal antibody against synthetic peptide of the N-terminal domain of human sarcospan. Using this antibody we investigated the localization of sarcospan and its spacial relation to the components of sarcoglycan subcomplex in normal human skeletal myofibers by immunofluorescent microscopy and immunogold electron microscopy. In immunofluorescence the reaction was observed continuously at the myofiber surface. Ultrastructurally the gold signals of rabbit anti sarcospan antibody were present along the muscle plasma membrane, mainly at its inside surface. The triple immunogold labeled muscle samples showed that the signals of rabbit or sheep polyclonal anti alpha-, beta-, gamma- and delta-sarcoglycan antibodies and/or mouse monoclonal anti beta-, gamma- and delta-sarcoglycan antibodies were located along the muscle plasma membrane, and the cluster formation of different two or three sarcoglycan molecules was observed. The triple immunogold labeling also revealed that the signal of sarcospan molecules are present frequently in doublets and/or triplets with the components of sarcoglycan subcomplex, resulting in the cluster formation of signals of sarcoglycan and sarcospan molecules. The result of this study showed that sarcospan was expressed at the myofiber surface and that sarcospan was present in close association with alpha-, beta-, gamma- and delta-sarcoglycans and formed a functional unit with sarcoglycan subcomplex.

Published

2005

24. Reduced expression of aquaporin 4 in human muscles with amyotrophic lateral sclerosis and other neurogenic atrophies

Author

Masahiko Inoue, Seiji Shibuya, Yoshihiro Wakayama, Takahiro Jimi, Hajime Hara, and Yoko Matsuzaki

Subjects

Muscle tissue, Pathology, medicine.medical_specialty, Duchenne muscular dystrophy, Muscle Fibers, Skeletal, Gene Expression, Aquaporins, Pathology and Forensic Medicine, Dystrophin, Atrophy, medicine, Myocyte, Humans, RNA, Messenger, Amyotrophic lateral sclerosis, Fluorescent Antibody Technique, Indirect, Muscle, Skeletal, Muscle contracture, Aquaporin 4, biology, business.industry, Reverse Transcriptase Polymerase Chain Reaction, Amyotrophic Lateral Sclerosis, Skeletal muscle, Cell Biology, Anatomy, Middle Aged, Water-Electrolyte Balance, medicine.disease, Muscular Dystrophy, Duchenne, Muscular Atrophy, medicine.anatomical_structure, biology.protein, sense organs, business

Abstract

Aquaporin 4 (AQP4) is a water channel protein that is widely distributed in human tissues. However, the precise functional role of AQP4 in skeletal muscle tissue has not yet been determined. Expression of AQP4 was reported to be reduced in muscle tissue from Duchenne muscular dystrophy patients. In the regenerating phase of skeletal muscle, AQP4 expression was reduced when nerve supply was not present. However, in diseased human muscles with neurogenic atrophy including amyotrophic lateral sclerosis, there has been no data on the changes in AQP4 expression. In the present study, we investigated the expression of AQP4 at mRNA and protein levels in human muscles with neurogenic atrophy. The mean level of AQP4 mRNA was significantly lower in muscles with neurogenic atrophy than that in muscles from normal controls. The myofiber surface immunostaining with anti-AQP4 antibody in muscles with neurogenic atrophy was reduced on the surface of scattered myofibers, small angulated myofibers, and myofibers in small- and large-group atrophy despite the presence of dystrophin. Based on the present findings, we conclude that the expression of AQP4 is affected by nerve supply and is down-regulated in human muscles with neurogenic atrophy.

Published

2004

25. [Siblings with dysferlinopathy presenting different clinical course]

Author

Masakazu, Kaneko, Seiji, Shibuya, and Yoshihiro, Wakayama

Subjects

Male, Phenotype, Siblings, Mutation, Humans, Membrane Proteins, Muscle Proteins, Female, Muscle, Skeletal, Dysferlin, Muscular Dystrophies

Published

2003

26. Merosin (laminin-2) localization in basal lamina of normal skeletal muscle fibers and changes in plasma membrane of merosin-deficient skeletal muscle fibers

Author

Seiji Shibuya, Hiroaki Oniki, Masahiko Inoue, Hiroko Kojima, and Yoshihiro Wakayama

Subjects

medicine.medical_specialty, Duchenne muscular dystrophy, Basement Membrane, Mice, Mice, Neurologic Mutants, Laminin, Internal medicine, medicine, Animals, Muscle, Skeletal, biology, Chemistry, Cell Membrane, Dystrophy, Muscular Dystrophy, Animal, medicine.disease, Lamina lucida, Cell biology, Microscopy, Electron, medicine.anatomical_structure, Endocrinology, Congenital muscular dystrophy, biology.protein, Basal lamina, Anatomy, ITGA7, Dystrophin

Abstract

Primary deficiency of merosin causes a severe congenital muscular dystrophy (CMD) and a mouse dystrophy (dy/dy mouse). Also, its secondary deficiency is seen in some CMD with abnormal glycosylation of Alpha-dystroglycan, an extracellular membrane protein, which is the receptor of merosin and binds to dystrophin underlying the sarcolenma via Beta-dystroglycan, a transmembrane protein. In immunogold and freeze-etch electron microscopic studies, merosin in basal lamina of normal skeletal muscles has a zonation in the distribution and is localized at the lamina lucida of muscle basal lamina, and dystrophin molecules are often closed to merosin molecules at the inside and outside surface of muscle plasma membrane. Moreover, merosin molecules exist as the short fine cross-bridge fibrils connecting the basal lamina to the neighboring outer leaflet of the muscle plasma membrane. In freeze-fracture studies, the changes in muscle plasma membranes of dy/dy mice reveal a markedly decreased density of orthogonal arrays (OAs) but normal density of intramembranous particles (IMPs), whereas depletions of IMPs with decreased OAs have been found in Fukyama-type congenital muscular dystrophy, Duchenne muscular dystrophy, and mdx mice. Thus, further studies including the functional role of OAs would be required to understand the pathomechanism of merosin-deficient CMD.

Published

2003

27. Expression of aquaporin 3 and its localization in normal skeletal myofibres

Author

Yoshihiro, Wakayama, Takahiro, Jimi, Masahiko, Inoue, Hiroko, Kojima, Seiji, Shibuya, Makoto, Murahashi, Hajime, Hara, and Hiroaki, Oniki

Subjects

Aquaporin 3, Reverse Transcriptase Polymerase Chain Reaction, Immunoblotting, Antibodies, Monoclonal, Humans, Aquaporins, Microscopy, Immunoelectron, Muscle, Skeletal, Immunohistochemistry

Abstract

The question whether aquaporin 3 (AQP3) is expressed in normal human skeletal muscle at mRNA and protein levels has been examined, since AQP3 has been reported to be coexpressed with AQP4 in various kinds of tissues other than skeletal muscle. The gel electrophoresis of the reverse transcription polymerase chain reaction (RT-PCR) product of total RNA samples extracted from normal human muscle specimens by using the oligonucleotide primers for AQP3 contained a band of 629 base pairs which corresponded to the base pair length between two primers of AQP3. The nucleotide sequence of this RT-PCR product coincided with that of AQP3. At the protein level, immunoblot, immunohistochemical and immunoelectron microscopical studies were done by using rabbit antibody against the synthetic peptide of the cytoplasmic domain of the human AQP3 molecule. Immunoblot analysis showed that rabbit antibody against the human AQP3 reacted with a protein of approximately 30 kDa molecular weight in extracts of normal human skeletal muscles. The immunoreaction for the anti-AQP3 antibody with normal human muscle was noted at the myofibre surface. Immunogold labelling electron microscopy revealed that the gold particles indicating the presence of AQP3 molecules were located mainly at the inside surface of muscle plasma membrane.

Published

2003

28. Expression and localization of aquaporin 7 in normal skeletal myofiber

Author

Seiji Shibuya, Takahiro Jimi, Masahiko Inoue, Yoshihiro Wakayama, Hiroko Kojima, Hiroaki Oniki, and Hajime Hara

Subjects

Gel electrophoresis, Messenger RNA, Histology, Muscle Fibers, Skeletal, Skeletal muscle, RNA, Gene Expression, Cell Biology, Biology, Aquaporins, Molecular biology, Immunohistochemistry, Antibodies, Pathology and Forensic Medicine, Mice, medicine.anatomical_structure, Immunoblot Analysis, Gene expression, medicine, Myocyte, Animals, Humans, RNA, Messenger

Abstract

We examined whether AQP7 molecules are expressed in the normal skeletal muscle at mRNA and protein levels. Gel electrophoresis of the reverse transcription-polymerase chain reaction (RT-PCR) product of total RNA samples of normal human or mouse muscles by using oligonucleotide primers for human or mouse AQP7 showed a band of 328 or 369 basepairs, which corresponded to the basepair length between two primers of AQP7. The nucleotide sequence of these RT-PCR products coincided with those of human and mouse AQP7. Immunoblot, immunohistochemical and immunoelectron-microscopic studies of the protein were done by using the rabbit antibody against the synthetic peptide of the N-terminal cytoplasmic domain of the human AQP7 molecule. Immunoblot analysis showed that the rabbit antibody against human AQP7 reacted with a protein of approximately 30 kDa molecular weight in extracts of normal human and mouse skeletal muscles, and normal mouse liver. Immunohistochemistry with our anti-AQP7 antibody showed an immunoreaction at the myofiber surface of type 1 and type 2 fibers in human muscles and of type 2 fibers in mouse muscles.

Published

2003

29. [Available laboratory tests of neurological diseases involving autoimmune]

Author

Seiji, Shibuya and Yoshihiro, Wakayama

Subjects

Autoimmune Diseases of the Nervous System, Multiple Sclerosis, Myasthenia Gravis, Humans, Immunotherapy, Guillain-Barre Syndrome, Biomarkers, Dermatomyositis, Polymyositis

Published

2003

30. [ACE inhibitors and its usefulness in the prevention of aspiration pneumonia in chronic cerebrovascular disease patients with asymptomatic swallowing dysfunction]

Author

Seiji, Shibuya, Makoto, Murahashi, Masahiko, Inoue, Takahiro, Jimi, and Yoshihiro, Wakayama

Subjects

Male, Cerebrovascular Disorders, Chronic Disease, Humans, Pharynx, Angiotensin-Converting Enzyme Inhibitors, Female, Deglutition Disorders, Pneumonia, Aspiration, Tomography, X-Ray Computed, Aged

Abstract

The double contrast pharyngogram by use of computed radiography (DCP-CR) has been found to be useful in detection of asymptomatic swallowing dysfunction. Following the DCP-CR examination, we investigated the incidence of aspiration pneumonia in 143 patients with chronic cerebrovascular disease (CVD) for 3 years and the effects of ACE inhibitors on the prevention of pneumonia. Aspiration pneumonia occurred in 29 out of 143 patients, and more frequently in the elderly chronic CVD patients with multiple brain lesions. Aspiration pneumonia was confirmed in 26 out of 85 patients (30.6%) with abnormal barium adhesion to the pharyngeal wall on the double contrast pharyngogram image by DCP-CR; whereas pneumonia occurred in 3 out of 58 patients (5.2%) with normal findings of DCP-CR pharyngogram. Among chronic CVD patients with abnormal findings of DCP-CR pharyngogram, the incidence of aspiration pneumonia was significantly lower in the patients treated with ACE inhibitors than in those treated with other antihypertensive agents or without antihypertensive agents (chi 2 value = 7.163, p0.05). Accordingly, ACE inhibitors may prevent the aspiration pneumonia and reduce the incidence of aspiration pneumonia in the chronic CVD patients with abnormal DCP-CR pharyngogram images.

Published

2002

31. Ultrastructural localization of aquaporin 4 and alpha1-syntrophin in the vascular feet of brain astrocytes

Author

Seiji Shibuya, Masahiko Inoue, Hiroaki Oniki, Makoto Murahashi, Yoshihiro Wakayama, and Jian Wu Liu

Subjects

PDZ domain, Immunoblotting, Aquaporin, Muscle Proteins, Biology, Aquaporins, General Biochemistry, Genetics and Molecular Biology, Mice, medicine, Animals, Tissue Distribution, Syntrophin, Aquaporin 4, Sarcolemma, Calcium-Binding Proteins, Cell Membrane, Colocalization, Brain, Membrane Proteins, General Medicine, Immunogold labelling, Immunohistochemistry, Cell biology, Mice, Inbred C57BL, Microscopy, Electron, medicine.anatomical_structure, Astrocytes, sense organs, Astrocyte

Abstract

Aquaporin 4 (AQP4) is a recently discovered membrane bound water-selective channel and has been described at the light microscopic level to be predominantly expressed in the astrocytes of the brain, especially at the perivascular astrocyte endfoot processes. Alpha1-syntrophin, a member of dystrophin-associated protein, has also been reported at the light microscopic to be expressed level in the same site of astrocytes as AQP4 and interacts with other molecules through its PDZ domain. AQP4 expression has been reported to be absent at the sarcolemma and the perivascular astrocyte endfoot processes of alpha1-syntrophin knockout mice. Based on these observations, the molecular association between AQP4 and alpha1-syntrophin could be speculated. To test this hypothesis, we investigated the ultrasturctural localization of AQP4 and alpha1-syntrophin in the brain astrocytes by using double immunogold labeled electron microscopy. The results showed that AQP4 and alpha1-syntrophin colocalized frequently at the astrocyte membrane, especially at the perivascular astrocyte endfoot processes and suggested the presence of linkage between AQP4 and alpha1-syntrophin at the astrocyte plasma membrane.

Published

2002

32. Localization of sarcoglycan, neuronal nitric oxide synthase, beta-dystroglycan, and dystrophin molecules in normal skeletal myofiber: triple immunogold labeling electron microscopy

Author

Hiroaki Oniki, Masahiko Inoue, Seiji Shibuya, Hiroko Kojima, Makoto Murahashi, and Yoshihiro Wakayama

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, Histology, Immunoelectron microscopy, Immunoblotting, Molecular Sequence Data, Nitric Oxide Synthase Type I, Dystrophin, Sarcoglycans, Utrophin, Myocyte, Animals, Humans, Amino Acid Sequence, Dystroglycans, Microscopy, Immunoelectron, Muscle, Skeletal, Instrumentation, chemistry.chemical_classification, Membrane Glycoproteins, Sheep, biology, Immunogold labelling, musculoskeletal system, Molecular biology, Immunohistochemistry, Cell biology, Medical Laboratory Technology, Sarcoglycan, Cytoskeletal Proteins, chemistry, biology.protein, Rabbits, Anatomy, Nitric Oxide Synthase, Glycoprotein, tissues

Abstract

In order to investigate the mode of existence of the sarcoglycan complex, neuronal nitric oxide synthase (nNOS), β-dystroglycan, and dystrophin in the normal skeletal myofiber, we examined the ultrastructural localization and mutual spatial relationship of nNOS, β-dystroglycan, dystrophin, and the individual components of the sarcoglycan complex by using triple immunogold labeling electron microscopy. Each molecule of α-, β-, γ- and δ-sarcoglycans is located intracellularly or extracellularly near the muscle plasma membrane mostly in accordance with the sarcoglycan antigenic sites against which the antibodies were generated. The association of different two and/or three sarcoglycan molecules out of α-, β-, γ- and δ-sarcoglycan molecules was frequently observed. Each molecule of nNOS, β-dystroglycan, and dystrophin was ultrastructurally noted along the cell surface of normal skeletal myofibers. Moreover, the close relation of a sarcoglycan molecule with β-dystroglycan and dystrophin, and the association of nNOS with dystrophin were also confirmed ultrastructurally. Thus, this study demonstrated that the constituting molecules of the sarcoglycan complex, nNOS, β-dystroglycan, and dystrophin existed in the form of a cluster at the normal muscle plasma membrane. The association of nNOS with dystrophin and its associated glycoproteins may form a macromolecular signaling complex at the muscle plasma membrane. Microsc. Res. Tech. 55:154–163, 2001. © 2001 Wiley-Liss, Inc.

Published

2001

33. Muscle plasma membrane changes in dystrophin gene exon 52 knockout mouse

Author

Hiroaki Oniki, Tetsuya Matsuzaki, Hiroko Kojima, Seiji Shibuya, Yoshihiro Wakayama, Makoto Murahashi, and Ikuya Nonaka

Subjects

mdx mouse, Protein subunit, Pathology and Forensic Medicine, Dystrophin, Exon, Mice, Sarcolemma, Species Specificity, Caveolae, Utrophin, Animals, Freeze Fracturing, Muscle, Skeletal, Mice, Knockout, Chemistry, Cell Membrane, Gene Abnormality, Cell Biology, musculoskeletal system, Molecular biology, Immunohistochemistry, Mice, Inbred C57BL, Disease Models, Animal, Microscopy, Electron, Knockout mouse, Mice, Inbred mdx

Abstract

Changes in muscle plasma membranes in mice lacking exon 52 of the dystrophin gene (mdx52 mouse) were studied using the freeze-fracture technique. The extensor digitorum longus (EDL) muscle plasma membrane of the mdx52 mouse at 8 weeks of age showed significantly increased caveola density (p < 0.05 by two-tailed t-test) and significantly decreased densities of intramembranous particles (IMPs), orthogonal arrays (OAs) and orthogonal array subunit particles (OASPs) (p < 0.05 by two-tailed t-test, p < 0.01 by Wilcoxon rank-sum test, p < 0.05 by two-tailed t-test, respectively) on the protoplasmic face when compared with those of control EDL muscles. These changes are more similar to those seen in DMD than those in the mdx mouse at the same age as reported previously. Thus, the gene abnormality in the different exon of the mouse dystrophin gene seems to induce somewhat different changes in the muscle plasma membrane.

Published

2001

34. Aquaporin 4: lack of mRNA expression in the rat regenerating muscle fiber under denervation

Author

Yoshihiro Wakayama, Masahiko Inoue, Takahiro Jimi, Yoko Matsuzaki, Seiji Shibuya, Makoto Murahashi, Norie Uemura, and Hajime Hara

Subjects

Male, Muscle Fibers, Skeletal, Aquaporin, Biology, Aquaporins, Gene expression, medicine, Animals, Regeneration, RNA, Messenger, Muscular dystrophy, Rats, Wistar, Muscle, Skeletal, Denervation, Aquaporin 4, Messenger RNA, urogenital system, General Neuroscience, Water-Electrolyte Balance, medicine.disease, Molecular biology, Muscle Denervation, Rats, Immunohistochemistry, Immunostaining

Abstract

The recently identified water channel aquaporin 4 is a major component of the orthogonal arrays observed with freeze-fracture electron microscopy. We examined the expression of aquaporin 4 mRNA and protein in rat regenerating muscle under innervated and denervated conditions. We found decreased sarcolemmal immunostaining of aquaporin 4 in denervated regenerating muscle as opposed to innervated muscle. Quantitative reverse transcription-polymerase chain reaction revealed that aquaporin 4 mRNA was expressed in the innervated regenerating muscle; whereas it was not expressed in denervated muscle. Thus, lack of aquaporin 4 protein may be due to lack of aquaporin 4 mRNA in the denervated regenerating muscle. We conclude that the nerve supply influences expression of aquaporin 4 at the mRNA level in regenerating muscle.

Published

2000

35. Expression of selectin families and their ligand sialyl Lewis X in the muscles of inflammatory myopathies: an immunohistochemical study

Author

Takahiro Jimi, Seiji Shibuya, Sumimasa Yamashita, Yoshihiro Wakayama, Makoto Murahashi, Takuya Kobayashi, Masahiko Inoue, and Nobuko Misugi

Subjects

Pathology, medicine.medical_specialty, P-selectin, Lewis X Antigen, Oligosaccharides, Inflammation, Pathogenesis, chemistry.chemical_compound, Reference Values, E-selectin, Internal Medicine, medicine, Humans, Sialyl Lewis X Antigen, biology, Myositis, business.industry, Cell adhesion molecule, Binding protein, General Medicine, Neuromuscular Diseases, Up-Regulation, P-Selectin, Sialyl-Lewis X, chemistry, biology.protein, medicine.symptom, business, E-Selectin, Cell Adhesion Molecules, Selectin

Abstract

Object Adhesion molecules are suggested to play important roles in the pathogenesis of inflammatory diseases. We examined the expression of adhesion molecules in the muscles of human inflammatory myopathies. Methods We immunohistochemically studied the expression and distribution of two molecules in the selectin family (E- and P-selectin) and their common ligand sialyl Lewis X in 18 inflammatory myopathies, 13 disease controls, and 16 normal controls. Results In inflammatory myopathies, E- and P-selectin were upregulated on the surface of blood vessels, especially on the endothelial cells of the venules. Sialyl Lewis X was upregulated in the blood vessels, infiltrating leukocytes, and the surface of some atrophic myofibers. Some control muscles also showed weakly positive staining with these molecules, however, expression of these molecules was most striking in the muscles of inflammatory myopathies. Conclusion The results suggested that these molecules are upregulated in inflammatory myopathies and might play a role in the pathogenesis of inflammatory myopathies.(Internal Medicine 38: 632-635, 1999)

Published

1999

36. Immunocytochemical studies of aquaporin 4 in the skeletal muscle of mdx mouse

Author

Takahiro Jimi, Hiroaki Oniki, Masahiko Inoue, Yoshihiro Wakayama, Seiji Shibuya, Jian Wu Liu, and Hiroko Kojima

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, mdx mouse, Pathology, medicine.medical_specialty, Aquaporin, Biology, Aquaporins, Mice, medicine, Myocyte, Animals, Freeze Fracturing, Muscle, Skeletal, Aquaporin 4, Skeletal muscle, Immunogold labelling, Muscular Dystrophy, Animal, Water-Electrolyte Balance, musculoskeletal system, Molecular biology, Mice, Inbred C57BL, Microscopy, Electron, medicine.anatomical_structure, Neurology, biology.protein, Mice, Inbred mdx, Neurology (clinical), Rabbits, Dystrophin, Immunostaining

Abstract

Immunostainability of anti aquaporin 4 antiserum was investigated in the muscles of dystrophin deficient mdx mice. Western blot analysis showed that the rabbit antiserum against aquaporin 4 reacted with a 28 kDa protein in extracts of normal mouse quadriceps femoris muscles but did not react with the protein in extracts of quadriceps femoris muscles of mdx mice. Immunoperoxidase staining of the muscles from normal and mdx mice revealed the positive immunoreaction at the myofiber surface of normal mice and the negative, or the faint and discontinuous immunostaining at the surface of mdx myofibers. Immunogold electron microscopy disclosed the localization of aquaporin 4 molecules at the myofiber plasma membranes of normal mice and the localization was consistent with that of orthogonal array particles in the protoplasmic face of normal muscle plasma membrane seen in freeze fracture replicas. This study demonstrated that the density of aquaporin 4 molecules was decreased in the muscle plasma membranes of mdx mice, resulting in the faulty function of mdx myofibers.

Published

1999

37. Ultrastructural localization of alpha-, beta- and gamma-sarcoglycan and their mutual relation, and their relation to dystrophin, beta-dystroglycan and beta-spectrin in normal skeletal myofiber

Author

Hiroaki Oniki, Yoshihiro Wakayama, Hajime Hara, Masahiko Inoue, Takahiro Jimi, Seiji Shibuya, Hiroko Kojima, and Makoto Murahashi

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, Immunoelectron microscopy, Blotting, Western, Biology, Pathology and Forensic Medicine, Dystrophin, Cellular and Molecular Neuroscience, Immunolabeling, Mice, Sarcoglycans, Utrophin, Myocyte, Animals, Humans, Spectrin, Dystroglycans, Microscopy, Immunoelectron, Muscle, Skeletal, Membrane Glycoproteins, musculoskeletal system, Molecular biology, Immunohistochemistry, Cell biology, Mice, Inbred C57BL, Sarcoglycan, Cytoskeletal Proteins, Polyclonal antibodies, biology.protein, Neurology (clinical)

Abstract

Ultrastructural localization of alpha-, beta- and gamma-sarcoglycan and their mutual relation, and their relation to dystrophin, beta-dystroglycan and beta-spectrin were investigated in normal skeletal myofibers. Single-immunogold labeling electron microscopy showed that the signals of rabbit and sheep polyclonal antibodies against the synthetic peptide of the cytoplasmic domain of alpha-, beta or gamma-sarcoglycan were present along the inside surface of muscle plasma membrane and at the sarcoplasmic side of plasma membrane invaginations and vesicular structures in subsarcolemmal areas. These localizations were similar to that of dystrophin, beta-dystroglycan and beta-spectrin. Double-immunogold labeling disclosed the close association of alpha-, beta- and gamma-sarcoglycan each other and alpha-, beta-, gamma-sarcoglycan with dystrophin or beta-dystroglycan, and this was confirmed by statistical analysis. Monoclonal antibody against the extracellular domain of alpha-sarcoglycan was used with above-mentioned polyclonal anti-beta- and -gamma-sarcoglycan antibodies for triple-immunogold labeling, in which signals of alpha-sarcoglycan localized at the outer surface of muscle plasmalemma and those of beta- and gamma-sarcoglycans were present at the inside surface of plasma membrane. The triple immunolabeling showed an occasional closely associated presence of the three signals for alpha-, beta-and gamma-sarcoglycans, and a more frequent association for two signals out of alpha-, beta- and gamma-sarcoglycans. This study demonstrated that alpha-, beta- and gamma-sarcoglycan are closely located to one another and to dystrophin and beta-dystroglycan at the muscle plasma membrane.

Published

1999

38. Ultrastructural localization of alpha 1-syntrophin and neuronal nitric oxide synthase in normal skeletal myofiber, and their relation to each other and to dystrophin

Author

Seiji Shibuya, Hiroko Kojima, Hiroaki Oniki, Takahiro Jimi, Makoto Murahashi, Yoshihiro Wakayama, and Masahiko Inoue

Subjects

Immunoelectron microscopy, Sarcoplasm, Blotting, Western, Molecular Sequence Data, Muscle Fibers, Skeletal, Muscle Proteins, Pathology and Forensic Medicine, Dystrophin, Cellular and Molecular Neuroscience, Immunolabeling, medicine, Myocyte, Humans, Amino Acid Sequence, Microscopy, Immunoelectron, Muscle, Skeletal, Syntrophin, Neurons, biology, Calcium-Binding Proteins, Skeletal muscle, Membrane Proteins, musculoskeletal system, Molecular biology, Immunohistochemistry, Nitric oxide synthase, medicine.anatomical_structure, biology.protein, Neurology (clinical), Nitric Oxide Synthase

Abstract

We investigated the ultrastructural localization of alpha 1-syntrophin and neuronal nitric oxide synthase (nNOS) in normal human skeletal myofibers and analyzed their relation to each other and to dystrophin using single and double immunogold-labeling electron microscopy. Single immunolabeling showed antibodies to alpha 1-syntrophin and nNOS on the inner surface of the muscle plasma membrane, the sarcoplasmic side of plasma membrane invaginations, and the sarcoplasm near mitochondria of subsarcolemmal areas. The epitopes of alpha 1-syntrophin and nNOS tended to be present in clusters. Double immunolabeling revealed that epitope combinations of alpha 1-syntrophin-dystrophin, alpha 1-syntrophin-nNOS, and nNOS-dystrophin occurred more frequently in doublet form than did other epitope combinations, such as alpha 1-syntrophin-beta- spectrin and nNOS-beta-spectrin. These increased frequencies were noted both at the muscle plasma membrane undercoat and near mitochondria of subsarcolemmal areas. A significantly higher percentage of doublets comprised antibodies against alpha 1-syntrophin and dystrophin (28.5 +/- 1.5%, group mean +/- SE) than those against alpha 1-syntrophin and beta-spectrin (9.2 +/- 0.8%, P0.01). Furthermore, nNOS formed doublets significantly more frequently with dystrophin (25.2 +/- 3.3%) and alpha 1-syntrophin (26.0 +/- 4.1%) than with beta-spectrin (13.9 +/- 2.3%; P0.05). These data support the association of dystrophin, alpha 1-syntrophin, and nNOS at the inner surface of the muscle plasma membrane and near mitochondria of subsarcolemmal areas of normal human skeletal myofibers.

Published

1997

39. Immunogold and freeze etch electron microscopic studies of merosin localization in basal lamina of human skeletal muscle fibers

Author

Makoto Murahashi, Hiroaki Oniki, Hiroko Kojima, Takahiro Jimi, Yoshihiro Wakayama, and Seiji Shibuya

Subjects

Basement membrane, Pathology, medicine.medical_specialty, Lamina reticularis, Freeze Etching, Immunogold labelling, Biology, Lamina lucida, Immunohistochemistry, Basement Membrane, Pathology and Forensic Medicine, Cellular and Molecular Neuroscience, Microscopy, Electron, medicine.anatomical_structure, Anchoring fibrils, Ultrastructure, medicine, Biophysics, Humans, Lamina densa, Basal lamina, Neurology (clinical), Laminin, Muscle, Skeletal

Abstract

Merosin is a basement-membrane-associated protein found in striated muscle, peripheral nerve and placenta, the deficiency of which causes the muscle wasting condition in C57BL/6J-dy/dy, so-called dy/dy mouse. Moreover, merosin is the binding protein of 156 kDa alpha-dystroglycan which binds dystrophin by way of 43 kDa beta-dystroglycan. Therefore, merosin is an important component of the basal lamina of normal skeletal myofibers. We investigated the ultrastructural localization of merosin antibody in normal human skeletal myofibers by using immunogold electron microscopy and freeze etch electron microscopy. The ultrastructure of the basal lamina showed the presence of the lamina lucida, lamina densa and lamina reticularis. The lamina lucida appeared electron translucent with the exception of fuzzy fibrils. The immunogold electron microscopy disclosed that the merosin was present at the innermost layer (lamina lucida) of the basal lamina of normal human skeletal myofibers. With freeze etch replica electron microscopy, short cross-bridge fine fibrils were noted in the lamina lucida, connecting the basal lamina to the outer leaflet of the muscle plasma membrane. They measured 3-13 nm in diameter, 20-90 nm in length and were distributed with a spacing of 30-40 nm. The immunogold particles showing the presence of the merosin epitope were associated with these connecting structures.

Published

1997

40. Immunoelectron Microscopic Localization of C-Terminus of 43-kDa Dystrophin-Associated Glycoprotein in Normal Human Skeletal Myofibers

Author

Seiji Shibuya, Yoshiko Nakamura, Atsushi Takeda, Takahiro Jimi, Yoshihiro Wakayama, and Hiroaki Oniki

Subjects

Sarcoplasm, law.invention, law, Humans, Dystroglycans, Microscopy, Immunoelectron, Muscle, Skeletal, Instrumentation, chemistry.chemical_classification, Membrane Glycoproteins, biology, urogenital system, Chemistry, Immunogold labelling, musculoskeletal system, Immunohistochemistry, Cell biology, Cytoskeletal Proteins, Membrane, Ultrastructure, biology.protein, lipids (amino acids, peptides, and proteins), Electron microscope, Antibody, Dystrophin, Glycoprotein

Abstract

Ultrastructural localization of the C-terminus of a 43-kDa dystrophin-associated glycoprotein (43-DAG) and its relation to dystrophin were investigated in normal human skeletal myofibers by using single and double immunogold labelling methods. The C-terminal end of 43-DAG antibody was localized ultrastructurally at the inside surface of muscle plasma membrane and the sarcoplasmic side of the plasma membrane invaginations. Double immunolabelling electron microscopy disclosed that signals of the C-terminal end of 43-DAG and dystrophin were often associated with each other and formed a doublet at the inside surface of plasma membranes in normal human skeletal myofibers.

Published

1994

41. Size and localization of dystrophin molecule: immunoelectron microscopic and freeze etching studies of muscle plasma membranes of murine skeletal myofibers

Author

Seiji Shibuya, Yoshihiro Wakayama, Hiroaki Oniki, Takahiro Jimi, and Atsushi Takeda

Subjects

Sarcoplasm, Blotting, Western, Molecular Sequence Data, Biology, Antibodies, Pathology and Forensic Medicine, law.invention, Dystrophin, Cellular and Molecular Neuroscience, Mice, Mice, Neurologic Mutants, law, Molecule, Animals, Amino Acid Sequence, Microscopy, Immunoelectron, Actin, Freeze Etching, Muscles, Cell Membrane, Muscular Dystrophy, Animal, Peptide Fragments, Mice, Inbred C57BL, Membrane, Biochemistry, Transmission electron microscopy, Biophysics, Ultrastructure, biology.protein, Neurology (clinical), Rabbits, Electron microscope

Abstract

The ultrastructure and mode of existence of the dystrophin molecule and its relations to actin filaments were examined in murine skeletal myofibers. Electron microscopy of freeze-etched replicas of gold-labelled dystrophin molecules in quick-freeze, deep-etch, rotary-shadow preparations revealed rod-like structures 108.2 +/- 16.3 nm long and 3.1 +/- 1.5 nm thick. Some dystrophin molecules appeared to link their ends to form anastomosing networks; others were separate from each other. The dystrophin molecules were parallel or nearly parallel to the inner surface of the muscle plasma membrane. Double immuno-labelling transmission electron microscopy using N- and C-terminal dystrophin antibodies showed that the group mean distances of the N- and C-terminal signals from the muscle plasma membrane were 52.7 +/- 8.1 nm and 45.9 +/- 11.3 nm, respectively, which were not significantly different. Histograms of the distribution of the N- and C-terminal distances from the muscle plasma membrane had similar patterns with peaks 10-20 nm from the membrane. This was consistent with the findings of the mode of existence of dystrophin molecules seen in freeze-etched replicas. Finally, the dystrophin molecules were linked with the most peripheral sarcoplasmic actin like filaments, end to side as well as end to end.

Published

1993

42. High levels of nervous system-specific proteins in cerebrospinal fluid in patients with early stage Creutzfeldt-Jakob disease

Author

Takahiro Jimi, Youichi Takahashi, Tomiko Asano, Kenji Kosaka, Kanefusa Kato, Hiroumi Nakata, Seiji Shibuya, Teruaki Tomaru, and Yoshihiro Wakayama

Subjects

Nervous system, Pathology, medicine.medical_specialty, G protein, Clinical Biochemistry, Enolase, Alpha (ethology), Nerve Tissue Proteins, Biology, Biochemistry, Isozyme, Creutzfeldt-Jakob Syndrome, Cerebrospinal fluid, GTP-Binding Proteins, mental disorders, medicine, Humans, Creatine Kinase, G alpha subunit, Biochemistry (medical), S100 Proteins, Brain, General Medicine, nervous system diseases, Isoenzymes, medicine.anatomical_structure, Phosphopyruvate Hydratase, biology.protein, Creatine kinase

Abstract

Concentrations of several proteins that are characteristic of the nervous system were time-sequentially analyzed by radio- and enzyme-immunoassay in the cerebrospinal fluid (CSF) of patients with Creutzfeldt-Jakob disease (CJD). We found abnormally high levels of several proteins, such as neuron-specific enolase (NSE), S-100b protein, brain-type isozyme of creatine kinase (CK-BB) and alpha subunit of GTP binding protein G0 (G0 alpha) in the early stage of the disease. Generally, these protein levels were far higher in CJD patients than in normal controls and other neurological patients in the early stage before the typical clinical manifestations were evident. These levels increased to maxima when the disease activity was most prominent and returned to normal or mildly elevated levels in the terminal stage. The results imply that these protein levels can serve as biochemical markers for the presence of an active destructive process in CJD brain and provide us with a useful indicator for early diagnosis of CJD.

Published

1992

43. Antibody-decorated Dystrophin Molecule of Murine Skeletal Myofiber as Seen by Freeze-etching Electron Microscopy

Author

Yoshihiro Wakayama and Seiji Shibuya

Subjects

musculoskeletal diseases, Duchenne muscular dystrophy, Immunoelectron microscopy, macromolecular substances, Antibodies, Dystrophin, Mice, Utrophin, medicine, Animals, Myocyte, Microscopy, Immunoelectron, Cytoskeleton, Instrumentation, Actin, biology, Freeze Etching, Muscles, Cell Membrane, medicine.disease, Molecular biology, Actins, Cell biology, Mice, Inbred C57BL, biology.protein, Myofibril

Abstract

Dystrophin is the protein product of Duchenne muscular dystrophy gene which is defective in this genetic disorder. Here we identified ultrastructurally the dystrophin molecule from the various cytoskeletons at the cytoplasmic surface of murine myofiber plasma membrane by using quick-freeze, deep-etch, rotary-shadow replica of anti-dystrophin antibody-decorated muscle samples. The molecule was really cytoskeleton and incorporated in the meshwork of the plasma membrane-associated cytoskeletons. The molecule appeared to connect directly and/or through another cytoskeletal molecule with actin filament.

Published

1991

44. Gold-labelled dystrophin molecule in muscle plasmalemma of mdx control mice as seen by electron microscopy of deep etching replica

Author

Yoshihiro Wakayama and Seiji Shibuya

Subjects

musculoskeletal diseases, congenital, hereditary, and neonatal diseases and abnormalities, Pathology, medicine.medical_specialty, Duchenne muscular dystrophy, Pathology and Forensic Medicine, law.invention, Dystrophin, Cellular and Molecular Neuroscience, Mice, Mice, Neurologic Mutants, law, Reference Values, medicine, Molecule, Animals, Microscopy, Immunoelectron, biology, Chemistry, Freeze Etching, Muscles, Cell Membrane, Skeletal muscle, Immunogold labelling, Muscular Dystrophy, Animal, musculoskeletal system, medicine.disease, Mice, Inbred C57BL, Microscopy, Electron, Membrane, medicine.anatomical_structure, Cytoplasm, biology.protein, Biophysics, Neurology (clinical), Gold, Electron microscope

Abstract

The Duchenne muscular dystrophy product 'dystrophin' has been shown to be located at the inner surface of normal muscle plasma membrane. This study was undertaken to visualize the shape of dystrophin molecules and their topographical distribution at the inner surface of murine skeletal muscle plasma membrane. The immunogold electron microscopy of plastic-embedded quadriceps femoris muscles of six mdx mice and six control mice showed the presence of gold particles along the muscle plasma membrane undercoat of all muscle samples from the control mice without any antibody reaction in the mdx mice muscles. The gold-labelled muscles of six mdx and six control mice were quickly frozen by liquid helium in a rapid-freeze apparatus. High magnification electron microscopy of the quick-freeze, deep-etch, rotary-shadow replicas of the gold-labelled muscles demonstrated the presence of dystrophin molecules associated with gold particles at the cytoplasmic surface of mdx control mice. The dystrophin molecules displayed a variety of shapes, such as rods with a reduction in diameter from one end to the other end and/or with the enlargement of their end(s). These dystrophin molecules were incorporated in the meshwork of muscle plasma membrane-associated cytoskeletons.

Published

1991

45. Immunoreactivity of antibodies raised against synthetic peptide fragments predicted from mid portions of dystrophin cDNA

Author

Shota Miyake, Nobuko Misugi, Atsushi Takeda, Toshiyuki Kumagai, Takahiro Jimi, Yoshihiro Wakayama, and Seiji Shibuya

Subjects

Adult, Duchenne muscular dystrophy, Blotting, Western, Molecular Sequence Data, Muscle Proteins, Myotonic dystrophy, Antibodies, Muscular Dystrophies, Dystrophin, Mice, Nemaline myopathy, Muscular Diseases, medicine, Animals, Humans, Amino Acid Sequence, Amyotrophic lateral sclerosis, Child, Antiserum, biology, Base Sequence, Muscles, Dystrophy, DNA, medicine.disease, Molecular biology, Immunohistochemistry, Peptide Fragments, Mice, Inbred C57BL, Neurology, biology.protein, Neurology (clinical), Immunostaining

Abstract

We synthesized 3 peptide fragments predicted by residues 2354–2368 (peptide I), 2310–2324 (peptide II) and 2255–2269 (peptide III) on the mid-portion of the human dystrophin cDNA map where the most frequent intragenic deletions occurred in Duchenne muscular dystrophy. Rabbit antibodies against these peptides were raised and cryosections of 47 biopsied muscles were studied immunohistochemically. The 47 biopsied muscles included the quadriceps femoris muscles of 8 Duchenne muscular dystrophy patients, 8 child and 5 adult normal controls, 1 facioscapulohumeral dystrophy, 2 limb girdle dystrophy, 3 myotonic dystrophy, 3 polymyositis, 1 mitochondrial myopathy, 1 nemaline myopathy, 3 amyotrophic lateral sclerosis and the extensor digitorum longus muscles of 6 mdx mice (C57BL/10ScSn-mdx) and 6 normal control mice (C57BL/10ScSn). The peptide I antiserum continuously stained the myofiber surface membranes in 8 child and 5 adult normal control muscles, and in 14 other muscles from various neuromuscular diseases, but failed to stain the surface membranes in normal control mice. The surface membranes of 8 Duchenne muscles were not stained by the peptide I antiserum except for a few myofibers. Although the ELISA titers of peptide I, II and III antibodies were high, immunostaining by peptide II antiserum showed no reaction in the myofibers of any of the biopsied muscles, and immunostaining by peptide III antiserum revealed faint reactions on the myofiber surface membranes of all biopsied muscles, including the mdx control mouse muscles except for the Duchenne and mdx myofibers.

Published

1990

46. Observations on the muscle plasma membrane-associated cytoskeletons of mdx mice by quick-freeze, deep-etch, rotary-shadow replica method

Author

Seiji Shibuya and Yoshihiro Wakayama

Subjects

musculoskeletal diseases, Pathology, medicine.medical_specialty, Immunoelectron microscopy, Duchenne muscular dystrophy, Muscle Proteins, Biology, Pathology and Forensic Medicine, law.invention, Dystrophin, Cellular and Molecular Neuroscience, Mice, law, medicine, Animals, Cytoskeleton, Microscopy, Immunoelectron, Sarcolemma, Freeze Etching, Muscles, Cell Membrane, Muscular Dystrophy, Animal, musculoskeletal system, medicine.disease, Mice, Inbred C57BL, Cytoplasm, Biophysics, Ultrastructure, biology.protein, Neurology (clinical), Electron microscope, tissues

Abstract

The Duchenne muscular dystrophy gene product "dystrophin" is a sarcolemma-associated cytoskeleton which is present just inside the sarcolemma. We investigated the ultrastructure and the relationship of this cytoskeleton to the muscle plasma membrane by immunoelectron microscopy and freeze-etch electron microscopy of liquid helium-frozen fresh muscles. The immunoelectron microscopy of the extensor digitorum longus muscles of six mdx mice and six control mice showed the location of anti-dystrophin antibody along the muscle plasma membrane undercoat of all the muscle samples from the control mice without any antibody reaction in the mdx mice muscles. Fresh extensor digitorum longus muscles of seven mdx and six control mice were quick-frozen in liquid helium in the rapid-freeze device. High-magnification electron microscopy of the deep-etch, rotary-shadow replicas of the frozen muscles showed the network formation and attachment of individual rod-shaped cytoskeletons of variable size to the cytoplasmic surface of the muscle plasma membrane in both mdx mice and control mice. The length of cytoskeletons attached to the muscle plasma membranes was measured and mean length +/- SE in mdx mice and control mice were 98 +/- 4 nm and 101 +/- 3 nm, respectively. Although these values were not statistically different (P greater than 0.1), the distribution frequency of 130-150 nm muscle plasma membrane-associated cytoskeletons was 7.9% in mdx mice versus 14.5% in control mice. Since the predicted length of dystrophin is 125-150 nm, the 130- to 150-nm plasma membrane-associated cytoskeletons of mdx control mice may include dystrophin.

Published

1990

47. Subject Index Vol. 184, 2006

Author

Kazunobu Sasaki, Ana Karina M.V. Cardoso, Mako Tosaka, Gaëlle Chopin Stukart-Parsons, Hannes Kutta, Takayuki Asahara, Ayako Nagahashi, Yoko Matsuzaki, M. Gordjestani, Seiji Shibuya, Jin Choon Lee, Jinxi Wang, Lygia da Veiga Pereira, Lars Martin Jakt, Jochen G. Hofstaetter, Melanie Meersch, Fúlvio Borges Miguel, Hae Jin Jeong, Hiroo Iwata, Silvia Maria Gomes Massironi, Hajime Hara, Norbert Pallua, Hirokazu Hirata, Dennis von Heimburg, Alexandre Kerkis, Soo Geun Wang, Hiroko Kojima, Kayoko Inoue, Buddy D. Ratner, Jacob D. Woolman, Hiroaki Oniki, Jeffrey R. Avansino, F. Mohamed, Hwal Woong Kim, L. Dermaut, Fabiana Paim Rosa, Humberto F. Cerruti, Melvin J. Glimcher, Yuji Sonoda, David C. Chen, Philipp Steven, V. Filippa, W. De Leersnijder, Elcio Marcantonio, Aryon A. Barbosa, Yoshinobu Murakami, Sheng Pan, Marcos Farina, Arnold I. Caplan, Jin Sup Jung, F. Bosman, Gloria Dulce de Almeida Soares, Karsten Hemmrich, Yoshiaki Miyamoto, Takahiro Jimi, Matthias Stelzner, Friedrich Paulsen, Vatche G. Agopian, Irina Kerkis, Yoshihiro Wakayama, Masahiko Inoue, Shin Kawamata, D. Dozortsev, Joji Takahashi, Yoshiki Sawa, Robert R. Lorenz, L. De Ridder, Byung Joo Lee, P. De Waele, Jun Yan, Vicki D. Hoagland, and Yong Chan Bae

Subjects

Histology, Index (economics), Statistics, Subject (documents), Anatomy, Mathematics

Published

2006

48. Reduced Aquaporin 4 Expression in the Muscle Plasma Membrane of Patients With Duchenne Muscular Dystrophy

Author

Toshiyuki Kumagai, Takahiro Jimi, Masahiko Inoue, Hajime Hara, Seiji Shibuya, Hiroko Kojima, Makoto Murahashi, Yoshihiro Wakayama, and Sumimasa Yamashita

Subjects

Male, musculoskeletal diseases, Duchenne muscular dystrophy, Immunoblotting, Aquaporins, Arts and Humanities (miscellaneous), Reference Values, Gene expression, medicine, Humans, Myocyte, RNA, Messenger, Muscular dystrophy, Child, Muscle, Skeletal, Aquaporin 4, Messenger RNA, Genome, Staining and Labeling, biology, Reverse Transcriptase Polymerase Chain Reaction, Cell Membrane, Infant, DNA, Neuromuscular Diseases, medicine.disease, Immunohistochemistry, Molecular biology, Muscular Dystrophy, Duchenne, Reverse transcription polymerase chain reaction, genomic DNA, Child, Preschool, biology.protein, sense organs, Neurology (clinical), Dystrophin, Protein Processing, Post-Translational

Abstract

Background In Duchenne muscular dystrophy (DMD), previous freeze-fracture electron microscopic studies demonstrated that muscle plasma membrane contained markedly decreased numbers of orthogonal arrays. Recent investigations showed that orthogonal arrays were composed of aquaporin 4 (AQP4) molecules, a member of the water channel protein family. Objectives To study whether the immunostainability of anti-AQP4 antibody is reduced in muscles of patients with DMD and whether, if it is reduced, the problem is at the genomic DNA, messenger RNA (mRNA), or posttranscriptional level. Patients and methods We analyzed the muscle and blood samples from 6 boys with DMD, 6 normal control subjects, and 12 patients with neuromuscular diseases at the protein, genomic DNA, and mRNA levels. At the protein level, immunohistochemical staining and immunoblot analysis were performed. At the genomic DNA and mRNA levels, the polymerase chain reaction and reverse transcription polymerase chain reaction, respectively, were used to screen for mutations in the AQP4 gene. Results At the protein level, immunohistochemical staining of our originally generated rabbit anti-AQP4 antibody in DMD muscles was markedly reduced. Most of the DMD myofibers showed negative staining with sporadic partially positive fibers at their myofiber surface, whereas the control muscles displayed continuous myofiber surface staining. Immunoblot analysis showed that the content of AQP4 in DMD muscles was remarkably decreased. Amplification of leukocyte genomic DNA by polymerase chain reaction showed that the patients with DMD had genomic DNA of the AQP4 molecule. Quantitative reverse transcription polymerase chain reaction demonstrated that DMD skeletal muscles contained markedly decreased AQP4 mRNA compared with controls. Conclusion The reduction in AQP4 in DMD muscles results from decreased levels of AQP4 mRNA in DMD myofibers.

Published

2002

49. THE EXPRESSION OF AQUAPORIN 4 mRNA IN EXPERIMENTAL REGENERATING MUSCLE

Author

Yoshihiro Wakayama, Takahiro Jimi, Seiji Shibuya, and Makoto Murahashi

Subjects

Cellular and Molecular Neuroscience, Messenger RNA, Aquaporin 4, Neurology, Chemistry, Neurology (clinical), General Medicine, Pathology and Forensic Medicine, Cell biology

Published

1999

50. Benign adult-onset focal myositis confined to the calf muscles

Author

Seiji Shibuya, Yoshihiro Wakayama, and Makoto Murahashi

Subjects

Cellular and Molecular Neuroscience, Pathology, medicine.medical_specialty, Physiology, business.industry, Physiology (medical), Focal myositis, medicine, Neurology (clinical), business, Calf muscles

Published

1998