Your search keyword '"Akihiko Moriyama"' showing total 98 results

1. Mitochondrial genome of Cipangopaludina japonica (Gastropoda: Viviparidae) with a tRNA gene rearrangement

Author

Kenichiro Nasu, Yuri Yokoyama, Yao Sun, Mieko Suzuki-Matsubara, Tadahiro Teramoto, Akihiko Moriyama, Motohiro Kawase, and Yoshinori Kumazawa

Subjects

river snail, invasive alien species, phylogenetic tree, Genetics, QH426-470

Abstract

The mitochondrial genome of a freshwater snail, Cipangopaludina japonica from Nagoya, Central Japan was nearly completely sequenced. This genome encodes 37 genes as found in most other metazoan species. However, there was a changed order of tRNAGlu and tRNAGly genes, a unique feature that was not found in mitochondrial genomes of closely related river snails. Phylogenetic analysis suggested that C. japonica is more closely related to C. ussuriensis from Amur River than to any other Cipangopaludina species sequenced to date.

Published

2020

2. Morphological and Histochemical Changes in the Uterus Epithelium during Eggshell Formation in Quail

Author

Atsushi Iwasawa, Mohammad A. Rahman, Tushar K. Roy, Akihiko Moriyama, and Norio Yoshizaki

Subjects

avian egg, eggshell matrix, eggshell pore, immunohistochemistry, uterus, Animal culture, SF1-1100

Abstract

The present study was conducted to determine both the site at which the eggshell matrix is produced and the critical period for its production in the oviductal uterus of the Japanese quail, Coturnix japonica. An antiserum was produced against the proteins of the 116-kDa band in electrophoretic profiles of the matrix proteins obtained from eggshells decalcified with EDTA. N-terminal amino acid sequences were very similar to those of chicken ovocleidin-116. Immunofluorescent and immunoelectron microscopic observations revealed that the 116-kDa proteins were synthesized in granular cells of the uterus mucosal epithelia, secreted between 7 and 20 h after the previous oviposition, then integrated into the structure of the eggshell matrix. Scanning electron microscopic observations revealed that 10-μm-wide posts appear on the surface of the mucosal epithelia until 21h, and disappear thereafter. The posts were less prominent in the mucosal epithelium facing the sharp end of an egg than in that facing the equator or blunt end. On the other hand, the number of pores in eggshells at the sharp end was smaller than that at the equator or blunt end. Our results indicate that air canals and/or pores are formed in the eggshell by the retreat of the posts after the establishment of eggshell.

Published

2010

3. VMO-II Mediates the Binding of the Chalaziferous Layer with the Vitelline Membrane in Quail Eggs

Author

Mohammad A. Rahman, Akihiko Moriyama, Atsushi Iwasawa, and Norio Yoshizaki

Subjects

chalaziferous layer, egg envelopes, immunohistochemistry, infundibulum, quail, Animal culture, SF1-1100

Abstract

Electron microscopic observations have revealed an electron density gradient in the chalaziferous layer of avian egg. The density is highest in the innermost sub-layer, which is bound with the vitelline membrane, and is thus traditionally referred to as the vitelline membrane outer layer (VMO). After high-concentration salt treatment, two proteins, VMO-I and VMO-II, are liberated from the egg envelopes of quail (Coturnix japonica), which results in the separation of the chalaziferous layer from the vitelline membrane. VMO-I and VMO-II were purified through gel-filtration and subjected to antisera produced in rabbits. The molecular sizes of these two proteins were estimated to be 9 to 15kDa for VMO-II and 18kDa for VMO-I. Their amino acid sequences were very similar to those of chickens. Immunofluorescent and immunoelectron micrographs showed that VMO-II was produced by the luminal epithelium and VMO-I by both the luminal and glandular epithelia of the infundibulum. Immunogold particles for the labeling of both proteins were distributed throughout the chalaziferous layer, as well as in the chalazae, with a density gradient similar to that mentioned above. In salt-treated envelopes, immunogold labeling was completely absent when stained with anti-VMO-II antiserum and weak with anti-VMO-I antiserum. Immunohistochemical studies revealed that purified VMO-II bound with vitelline membranes of salt-treated envelopes, and ligand blotting tests revealed that ZP1 and ZP3 were the molecules bound by VMO-II; the binding was inhibited by various kinds of sugars. VMO-II might play a role in the binding of the chalaziferous layer with the vitelline membrane, a process that leads to the anchoring of the chalaza cord.

Published

2009

4. DNA barcoding of Japanese click beetles (Coleoptera, Elateridae).

Author

Yuichi Oba, Hitoo Ôhira, Yukio Murase, Akihiko Moriyama, and Yoshinori Kumazawa

Subjects

Medicine, Science

Abstract

Click beetles (Coleoptera: Elateridae) represent one of the largest groups of beetle insects. Some click beetles in larval form, known as wireworms, are destructive agricultural pests. Morphological identification of click beetles is generally difficult and requires taxonomic expertise. This study reports on the DNA barcoding of Japanese click beetles to enable their rapid and accurate identification. We collected and assembled 762 cytochrome oxidase subunit I barcode sequences from 275 species, which cover approximately 75% of the common species found on the Japanese main island, Honshu. This barcode library also contains 20 out of the 21 potential pest species recorded in Japan. Our analysis shows that most morphologically identified species form distinct phylogenetic clusters separated from each other by large molecular distances. This supports the general usefulness of the DNA barcoding approach for quick and reliable identification of Japanese elaterid species for environmental impact assessment, agricultural pest control, and biodiversity analysis. On the other hand, the taxonomic boundary in dozens of species did not agree with the boundary of barcode index numbers (a criterion for sequence-based species delimitation). These findings urge taxonomic reinvestigation of these mismatched taxa.

Published

2015

5. Experiment on the Relation between Color Discriminability and Genetic Polymorphism in the L Cone Using Four Color Primary Display Device.

Author

Johji Tajima, Go Tanaka, Mieko Suzuki, Akihiko Moriyama, and Yasuhiro Yoshida

Published

2013

6. Population Genetic Structure of Little Tern (Sternula albifrons) in Japan Inferred from Nucleotide Sequence Diversities of the Mitochondrial DNA Control Region

Author

Masaharu Hayakawa, Mieko Suzuki-Matsubara, Kazumi Matsubara, Satoshi Kanazawa, Takashi Fujii, Wataru Kitamura, Ryoh Alexander Murofushi, and Akihiko Moriyama

Subjects

Animal Science and Zoology

Published

2022

7. Heterologous expression and functional analysis of the F-box protein Ucc1 from other yeast species in Saccharomyces cerevisiae

Author

Kunio Nakatsukasa, Tomoyuki Kawarasaki, and Akihiko Moriyama

Subjects

biology, Chemistry, F-Box Proteins, Zygosaccharomyces bailii, Saccharomyces cerevisiae, Zygosaccharomyces, Glyoxylate cycle, Bioengineering, biology.organism_classification, Applied Microbiology and Biotechnology, Yeast, Ubiquitin ligase, Fungal Proteins, Citric acid cycle, Biochemistry, Ubiquitin ligase complex, biology.protein, Heterologous expression, Acetic Acid, Biotechnology

Abstract

The ubiquitin-proteasome system plays an important role in metabolic regulation. In a previous study, we reported that, in Saccharomyces cerevisiae, when glucose is available, the SCFUcc1 ubiquitin ligase complex targets citrate synthase 2 (Cit2) for proteasomal degradation, thereby suppressing the glyoxylate cycle, an anabolic pathway that replenishes the TCA cycle with succinate for the activation of gluconeogenesis. However, the roles of Ucc1 in other yeast species remain unclear. Here, we cloned orthologs of the F-box protein Ucc1 from Zygosaccharomyces bailii, an aggressive food spoilage microorganism that is the most acetic acid-tolerant yeast species, and Candida glabrata, an emerging fungal pathogen. These orthologs were expressed in S. cerevisiae, and their activities were tested genetically and biochemically. The results showed that Z. bailii Ucc1 rescued the ucc1Δ phenotype, suggesting the existence of a similar mechanism regulating the glyoxylate cycle in Z. bailii. By contrast, C. glabrata Ucc1 did not complement the ucc1Δ phenotype or exhibit a dominant negative effect on Ucc1. These results suggest the importance of analysing the regulatory mechanisms of glyoxylate cycle in a broad range of yeast species.

Published

2019

8. Structure, molecular evolution, and hydrolytic specificities of largemouth bass pepsins

Author

Yoko Miura, Akihiko Moriyama, Mieko Suzuki-Matsubara, and Takashi Kageyama

Subjects

Fish Proteins, Models, Molecular, 0301 basic medicine, DNA, Complementary, food.ingredient, Swine, Physiology, Molecular Sequence Data, Gene Expression, Sequence alignment, Biology, Molecular cloning, Biochemistry, Protein Structure, Secondary, Substrate Specificity, Evolution, Molecular, 03 medical and health sciences, Bass (fish), fluids and secretions, food, Pepsin, Molecular evolution, Escherichia coli, Animals, Protein Isoforms, Nucleotide, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Molecular Biology, Peptide sequence, Phylogeny, chemistry.chemical_classification, Pepsinogens, Hydrolysis, Pepsin A, Protein Structure, Tertiary, 030104 developmental biology, chemistry, biology.protein, Thermodynamics, Bass, sense organs, Hydrophobic and Hydrophilic Interactions, Sequence Alignment

Abstract

The nucleotide sequences of largemouth bass pepsinogens (PG1, 2 and 3) were determined after molecular cloning of the respective cDNAs. Encoded PG1, 2 and 3 were classified as fish pepsinogens A1, A2 and C, respectively. Molecular evolutionary analyses show that vertebrate pepsinogens are classified into seven monophyletic groups, i.e. pepsinogens A, F, Y (prochymosins), C, B, and fish pepsinogens A and C. Regarding the primary structures, extensive deletion was obvious in S'1 loop residues in fish pepsin A as well as tetrapod pepsin Y. This deletion resulted in a decrease in hydrophobic residues in the S'1 site. Hydrolytic specificities of bass pepsins A1 and A2 were investigated with a pepsin substrate and its variants. Bass pepsins preferred both hydrophobic/aromatic residues and charged residues at the P'1 sites of substrates, showing the dual character of S'1 sites. Thermodynamic analyses of bass pepsin A2 showed that its activation Gibbs energy change (∆G(‡)) was lower than that of porcine pepsin A. Several sites of bass pepsin A2 moiety were found to be under positive selection, and most of them are located on the surface of the molecule, where they are involved in conformational flexibility. The broad S'1 specificity and flexible structure of bass pepsin A2 are thought to cause its high proteolytic activity.

Published

2016

9. Comparison of the primary structures, cytotoxicities, and affinities to phospholipids of five kinds of cytotoxins from the venom of Indian cobra, Naja naja

Author

Akihiko Moriyama, Yoshiyuki Suzuki, Kazumi Matsubara, Mieko Suzuki-Matsubara, and Senarath B. P. Athauda

Subjects

0301 basic medicine, Nonsynonymous substitution, Physiology, Health, Toxicology and Mutagenesis, Naja, Molecular Sequence Data, Poison control, Venom, Biology, Toxicology, complex mixtures, Biochemistry, Mice, 03 medical and health sciences, Cell Line, Tumor, Animals, Humans, Amino Acid Sequence, Elapidae, Peptide sequence, Phospholipids, Elapid Venoms, chemistry.chemical_classification, Base Sequence, 030102 biochemistry & molecular biology, Cytotoxins, Protein primary structure, Cell Biology, General Medicine, biology.organism_classification, Amino acid, chemistry, NIH 3T3 Cells, Indian cobra

Abstract

The molecular mechanism underlying the hemolytic and cytolytic processes of cobra cytotoxins (CTXs) is not yet fully elucidated. To examine this, we analyzed the amino acid sequences, hemolytic and cytotoxic activities, and affinities to phospholipids of the five major CTXs purified from the venom of Indian cobra, Naja naja. CTX2, CTX7, and CTX8 belonged to S-type, and CTX9 and CTX10 to P-type. Comparisons of CTX7 with CTX8 and CTX9 with CTX10 revealed similar primary structures and hemolytic and cytolytic activities. CTX2, whose primary structure was rather different from the others, showed several times weaker hemolytic and cytolytic biological activities than the others. The comparison of CTX2 with CTX7 suggested the importance of Lys30 in loop II for the strong hemolytic and cytolytic activities of S-type CTXs. Cloning of 12 CTX cDNAs from the Naja naja venom cDNA library revealed that 18 out of 23 substitutions found in CTX cDNAs were nonsynonymous. This clearly indicated the accelerated evolution of CTX genes. Multiple sequence alignment of 51 kinds of CTX cDNAs and calculations of nonsynonymous and synonymous substitutions indicated that the codons coding the three loops' regions, which may interact with the hydrophobic tails of phospholipids, have undergone an accelerated evolution. In contrast, the codons coding for amino acid residues considered to participate in the recognition and binding of the hydrophilic head groups of phospholipids, eight Cys residues, and those likely stabilizing β core structure, were all conserved.

Published

2016

10. Pepsinogens and pepsins from largemouth bass, Micropterus salmoides: Purification and characterization with special reference to high proteolytic activities of bass enzymes

Author

Akihiko Moriyama, Takashi Kageyama, and Yoko Miura

Subjects

food.ingredient, Physiology, Molecular Sequence Data, Micropterus, Biochemistry, Bass (fish), chemistry.chemical_compound, fluids and secretions, food, Pepsin, Animals, Amino Acid Sequence, Molecular Biology, chemistry.chemical_classification, Pepsinogens, biology, Stomach, Fast protein liquid chromatography, biology.organism_classification, Pepsin A, Amino acid, Enzyme, chemistry, Sephadex, Proteolysis, biology.protein, Bass, Pepstatin

Abstract

Six pepsinogens were purified from the gastric mucosa of largemouth bass (Micropterus salmoides) by DEAE-Sephacel chromatography, Sephadex G-100 gel filtration, and Mono Q FPLC. The potential specific activities of two major pepsinogens, PG1-1 and PG2-2, against hemoglobin were 51 and 118 units/mg protein, respectively. The activity of pepsin 2-2 was the highest among the pepsins reported to date; this might be linked to the strongly carnivorous diet of the largemouth bass. The molecular masses of PG1-1 and PG2-2 were 39.0 and 41.0 kDa, respectively. The N-terminal amino acid sequences of PG1-1 and PG2-2 were LVQVPLEVGQTAREYLE- and LVRLPLIVGKTARQALLE-, respectively, showing similarities with those of fish type-A pepsinogens. The optimal pHs for hemoglobin-digestive activity of pepsins 1-1 and 2-2 were around 1.5 and 2.0, respectively, though both pepsins retained considerable activity at pHs over 3.5. They showed maximal activity around 50 and 40 °C, respectively. They were inhibited by pepstatin similarly to porcine pepsin A. The cleavage specificities clarified with oxidized insulin B chain were shown to be restricted to a few bonds consisting of hydrophobic/aromatic residues, such as the Leu(15)-Tyr(16), Phe(24)-Phe(25) and Phe(25)-Tyr(26) bonds. When hemoglobin was used as a substrate, the kcat/Km value of bass pepsin 2-2 was 4.6- to 36.8-fold larger than those of other fish pepsins. In the case of substance P, an ideal pepsin substrate mimic, the kcat/Km values were about 200-fold larger than those of porcine pepsin A, supporting the high activity of the bass pepsin.

Published

2015

11. ANALYSIS OF PATIENTS WHO UNDERWENT MODERATE-TO-MASSIVE TRANSFUSION AT A TOKYO METROPOLITAN HOSPITAL

Author

Makoto Kamesaki, Saiko Kurosawa, Kyoko Daibo, Mari Hoshino, Yuki Hazama, Akihiko Moriyama, Emi Yamamoto, Keisuke Ishii, Hiroshi Fujita, Shoko Fujimoto, and Shigeko Nishimura

Subjects

Pediatrics, medicine.medical_specialty, business.industry, General surgery, medicine, business, Massive transfusion

Abstract

近年，大量に輸血を行う際の投与方法が世界的に変化しつつある．当院での輸血の現状を把握するため，2006年1月から2009年6月までの期間に，24時間以内に赤血球濃厚液（以下，RCC）10単位以上の輸血を受けた144例（168回）について後方視的に検討した．このうち，多発外傷患者で来院から24時間以内にRCC 10単位以上の輸血を受けた65例について，さらに詳細に検討した．多発外傷患者の院内死亡率は60％であり，年齢，来院時活性化部分トロンボプラスチン時間，来院時フィブリノゲン分解産物の3つが有意な予後因子であることが判明した．治療に関する解析では，新鮮凍結血漿（以下，FFP）の非投与群の死亡率90％，FFP/RCCの輸血比率0.5以下群で68.4％，0.5より高い群で47.2％であり，輸血比率の重要性が示唆された．当院の大量輸血プロトコール作成について考察を加えた．

Published

2012

12. Cuticle Formation in Quail Eggs

Author

Atsushi Iwasawa, Akihiko Moriyama, Norio Yoshizaki, and Mohammad Anisur Rahman

Subjects

Antiserum, Coturnix japonica, Uterus, Coturnix, Oviducts, Anatomy, Biology, biology.organism_classification, Quail, law.invention, Cell biology, Egg Shell, medicine.anatomical_structure, law, biology.animal, medicine, Animals, Female, Animal Science and Zoology, Cuticle formation, Electron microscope, Eggshell, Ovum, Cuticle (hair)

Abstract

The present study was conducted to determine both the site at which cuticle materials are produced and the critical period for their production in the oviductal uterus of the Japanese quail, Coturnix japonica. An antiserum was produced against the 32-kDa band in electrophoretic profiles of cuticle materials obtained from eggshells decalcified with EDTA. Immunofluorescence and immunoelectron microscopic observations revealed that the 32-kDa protein was synthesized in luminal ciliated epithelial cells of the uterus until 21 h after the previous oviposition (the first phase) and then secreted during the 4 h before the next oviposition (the second phase). Scanning electron microscopic observations revealed that 10-microm-wide posts appear on the surface of the luminal epithella during the first phase, and that they disappear during the second phase. During the second phase, air canals are formed in the eggshell by the retreat of the posts, and a cuticle layer forms on the eggshell. Our results indicate that the cuticle may function as a lubricant that facilitates egg rotation in the uterus.

Published

2009

13. Zinc-binding property of the major yolk protein in the sea urchin − implications of its role as a zinc transporter for gametogenesis

Author

Kazuo Ikeda, Keisuke Yamano, Hiromi Ohta, Tatsuya Unuma, and Akihiko Moriyama

Subjects

medicine.medical_specialty, Gonad, food.ingredient, chemistry.chemical_element, Cell Biology, Zinc, Biology, Biochemistry, Oogenesis, medicine.anatomical_structure, Endocrinology, food, chemistry, Internal medicine, Yolk, biology.animal, medicine, Coelom, Vitellogenesis, Molecular Biology, Sea urchin, Gametogenesis

Abstract

Major yolk protein (MYP), a transferrin superfamily protein that forms yolk granules in sea urchin eggs, is also contained in the coelomic fluid and nutritive phagocytes of the gonad in both sexes. MYP in the coelomic fluid (CFMYP; 180 kDa) has a higher molecular mass than MYP in eggs (EGMYP; 170 kDa). Here we show that MYP has a zinc-binding capacity that is diminished concomitantly with its incorporation from the coelomic fluid into the gonad in the sea urchin Pseudocentrotus depressus. Most of the zinc in the coelomic fluid was bound to CFMYP, whereas zinc in eggs was scarcely bound to EGMYP. Both CFMYP and EGMYP were present in nutritive phagocytes, where CFMYP bound more zinc than EGMYP. Saturation binding assays revealed that CFMYP has more zinc-binding sites than EGMYP. Labeled CFMYP injected into the coelom was incorporated into ovarian and testicular nutritive phagocytes and vitellogenic oocytes, and the molecular mass of part of the incorporated CFMYP shifted to 170 kDa. Considering the fact that the digestive tract is a major production site of MYP, we propose that CFMYP transports zinc, essential for gametogenesis, from the digestive tract to the ovary and testis through the coelomic fluid, after which part of the CFMYP is processed to EGMYP with loss of zinc-binding site(s).

Published

2007

14. Effects of cyclosporine A in hyperzincaemia and hypercalprotectinaemia

Author

Kenji Goto, Kyoko Ban, Tokio Sugiura, Akihiko Moriyama, Shoji Okada, Hajime Togari, and Kouichi Ito

Subjects

business.industry, Pediatrics, Perinatology and Child Health, Medicine, General Medicine, Pharmacology, business

Published

2007

15. Significance of 32-kDa Cathepsin L Secreted from Cancer Cells

Author

Yoko Hashimoto, Chihiro Kondo, Taro Hayakawa, Akihiko Moriyama, Hiroshi Nagata, Nobuhiko Katunuma, and Takashi Kojima

Subjects

Cancer Research, Lung Neoplasms, Cathepsin L, Immunoblotting, Cathepsin D, Biology, Metastasis, Cell Line, Tumor, Neoplasms, Cathepsin L1, medicine, Humans, Neoplasm Invasiveness, Protease Inhibitors, Radiology, Nuclear Medicine and imaging, Zymography, Neoplasm Metastasis, Cathepsin S, Pharmacology, Enzyme Precursors, Tumor Necrosis Factor-alpha, General Medicine, medicine.disease, Cathepsins, Molecular biology, Culture Media, Cysteine Endopeptidases, Oncology, Cell culture, Colonic Neoplasms, Cancer cell, biology.protein

Abstract

It is recognized that many cancer cells secrete cathepsin L to degrade the components of extracellular matrices and basement membranes, thus promoting tumor invasion and metastasis. However, very little information is available concerning the secreted forms of cathepsin L and their possible role in human cancer. We initially demonstrated that approximately 10-fold higher mature cathepsin L activity was secreted in a medium of human fibrosarcoma (HT 1080) cells, compared with their intracellular activity. A 32-kDa major-activity band, together with a 41-kDa faint-activity band, was detected in the medium by our newly developed gelatin zymography. The two forms were further confirmed to be cathepsin L by immunoblot analysis. Both were apparently secreted directly from the cells, as neither was affected when the cells were cultured in the presence of various kinds of proteinase inhibitors. Human tumor necrosis factor-alpha (TNF-alpha) stimulated not only the production of the 32-kDa cathepsin L, but also its secretion. Moreover, the 32-kDa cathepsin L activities in 3 colon and 2 lung cancer tissues were significantly higher than in normal tissues. Based on the foregoing, there are good reasons to speculate that the 32-kDa cathepsin L found in HT 1080 cell medium is involved in cancer invasion and metastasis.

Published

2006

16. Single-chain tissue-type plasminogen activator is a substrate of mouse glandular kallikrein 24

Author

Akihiko Moriyama, Naoharu Takano, Takayuki Takahashi, and Hitoshi Matsui

Subjects

Male, Proteases, Plasmin, extracellular matrix, Blotting, Western, testis, law.invention, Extracellular matrix, Mice, Plasminogen Activators, Sequence Analysis, Protein, law, medicine, Animals, Humans, kallikrein, tPA, mouse spermatogenesis, DNA Primers, chemistry.chemical_classification, biology, Reverse Transcriptase Polymerase Chain Reaction, Leydig Cells, Kallikrein, Blotting, Northern, Immunohistochemistry, Molecular biology, Enzyme, chemistry, proteolytic processing, Recombinant DNA, biology.protein, Kallikreins, Animal Science and Zoology, Antibody, Plasminogen activator, medicine.drug

Abstract

Leydig cells of the adult mouse testis express at a detectable level three distinct glandular (tissue) kallikrein genes: mKlk21, mKlk24, and mKlk27. Recently, the proteins encoded by these genes were characterized using active recombinant proteases, but their roles in the mouse testis remained to be determined. The present study showed that among the proteases, mK24 markedly enhanced the activity of human recombinant single-chain tissue-type plasminogen activator when the two were incubated together. This activation was found to be due to proteolytic conversion of the single-chain enzyme to a two-chain form. The expression of tissue-type plasminogen activator in interstitial Leydig cells was demonstrated by RT-PCR and immunohistochemical analyses. The primary culture medium of adult male testicular Leydig cells contained immunoreactive substances recognized by anti-mK24 antibodies. In addition, the same medium was capable of converting the single-chain plasminogen activator to the two-chain protein. These results suggest that mK24 may play a role in the degradation of extracellular matrix proteins in the interstitial area surrounding the Leydig cells of the adult mouse testis, due not only to its own activity, but also to that of plasmin produced by the single-chain tissue-type plasminogen activator-converting activity of mK24.

Published

2005

17. DNA Replication Checkpoint Control Mediated by the Spindle Checkpoint Protein Mad2p in Fission Yeast

Author

Izumi Sugimoto, Yuko Tonami, Makoto Nakanishi, Akihiko Moriyama, and Hiroshi Murakami

Subjects

DNA Replication, Indoles, Time Factors, Cell cycle checkpoint, Ultraviolet Rays, Green Fluorescent Proteins, Immunoblotting, Mitosis, Cell Cycle Proteins, Eukaryotic DNA replication, Spindle Apparatus, Protein Serine-Threonine Kinases, Biology, Biochemistry, DNA replication factor CDT1, Replication factor C, Control of chromosome duplication, Schizosaccharomyces, Hydroxyurea, Immunoprecipitation, Phosphorylation, DNA, Fungal, Molecular Biology, Temperature, Nuclear Proteins, DNA, Cell Biology, G2-M DNA damage checkpoint, Flow Cytometry, Methyl Methanesulfonate, Culture Media, Cell biology, DNA replication checkpoint, Checkpoint Kinase 2, Phenotype, Mad2 Proteins, Mutation, biology.protein, Tyrosine, Origin recognition complex, Schizosaccharomyces pombe Proteins, Carrier Proteins, Protein Kinases, Mutagens

Abstract

The relationship between the DNA replication and spindle checkpoints of the cell cycle is unclear, given that in most eukaryotes, spindle formation occurs only after DNA replication is complete. Fission yeast rad3 mutant cells, which are deficient in DNA replication checkpoint function, enter, progress through, and exit mitosis even when DNA replication is blocked. In contrast, the entry of cds1 mutant cells into mitosis is delayed by several hours when DNA replication is inhibited. We show here that this delay in mitotic entry in cds1 cells is due in part to activation of the spindle checkpoint protein Mad2p. In the presence of the DNA replication inhibitor hydroxyurea (HU), cds1 mad2 cells entered and progressed through mitosis earlier than did cds1 cells. Overexpression of Mad2p or inactivation of Slp1p, a regulator of the anaphase-promoting complex, also rescued the checkpoint defect of HU-treated rad3 cells. Rad3p was shown to be involved in the physical interaction between Mad2p and Slp1p in the presence of HU. These results suggested that Mad2p and Slp1p act downstream of Rad3p in the DNA replication checkpoint and that Mad2p is required for the DNA replication checkpoint when Cds1p is compromised.

Published

2004

18. Possible involvement of myosin-X in intercellular adhesion: Importance of serial pleckstrin homology regions for intracellular localization

Author

Mamoru Sano, Norio Yoshizaki, Shigeo Masaki, Satoshi Yonezawa, Takenori Takizawa, Akihiko Moriyama, Takashi Kageyama, and Atsuko Hanai

Subjects

Pleckstrin homology domain, Ezrin, Radixin, Myosin, macromolecular substances, Cell Biology, Basolateral plasma membrane, Biology, Lamellipodium, Cytoskeleton, Filopodia, Developmental Biology, Cell biology

Abstract

Subcellular fractionation experiments with mouse hepatocytes, combined with sodium dodecylsulfate (SDS)–polyacrylamide gel electrophoresis (PAGE)–immunoblot analysis using antibodies against two different tail regions of mouse myosin-X demonstrated a 240 kDa molecular mass to be associated with the plasma membrane-rich P2 fraction. The basolateral plasma membrane fraction, but not the brush border fraction, isolated from renal cortices also contained the 240 kDa form of myosin-X. In an attempt to assess relative contributions of possible functional domains in the tail of myosin-X to localization and function, cDNA corresponding to all three pleckstrin homology (PH) domains and different regions (PH1, 2 and 3, and the two subdomains of PH1: PHS1 and PHS2), as well as the myosin tail homology 4 domain (MyTH4) and the band4.1/ezrin/radixin/moesin-like domain (FERM) were separately inserted into the pEGFP vector and expressed in cultured COS-1 cells. As a result, two distinct regions responsible for localization were identified with regard to PH: one covers all three forms that tends to localize to regions of dynamic actin, such as membrane ruffles, lamellipodia and thick cortical actin bundles at the sites of cell–cell adhesion in a Rac- and Cdc42-dependent manner. The other covers PHS1 and PH2 that localizes to filopodia, filopodial puncta and the sites of intercellular adhesion in a Cdc42-dependent manner. Expression of green fluorescent protein (GFP)-MyTH4 fusion protein resulted in formation of phalloidin-positive granules, while GFP-FERM affected the actin cytoskeletal system in a distinctly different way. Taken altogether, the results lend support to the view that myosin-X is involved in cell–cell adhesion-associated signaling-linked membrane and/or cytoskeleton reorganization.

Published

2003

19. Hyperthermic induction of apoptosis in malignant fibrous histiocytoma cells: possible involvement of a p53-independent pathway in the induction of bax gene

Author

Taiji Kato, Akihiko Moriyama, Kohichi H. Kato, Kiyofumi Asai, Masato Yonezawa, Nobuo Matsui, and Takanobu Otsuka

Subjects

Programmed cell death, Hot Temperature, Blotting, Western, Molecular Sequence Data, Cell, Apoptosis, DNA Fragmentation, Biology, medicine.disease_cause, Polymerase Chain Reaction, Gene expression, Tumor Cells, Cultured, medicine, Animals, Point Mutation, Orthopedics and Sports Medicine, RNA, Messenger, Northern blot, Electrophoresis, Agar Gel, Mutation, Base Sequence, Histiocytoma, Benign Fibrous, Blotting, Northern, Genes, p53, Molecular biology, Rats, medicine.anatomical_structure, Cell culture, DNA fragmentation, Surgery

Abstract

We have previously reported the unique heat sensitivity of a cell line of malignant fibrous histiocytoma cells, the MFH-2NR cell line. In the present study, treatment of MFH-2NR cells, at 43 degrees C for 1 h evoked typical apoptosis in these cells, which showed characteristic morphological changes, such as internucleosomal DNA fragmentation (DNA ladders), cell shrinkage, and chromatin condensation. Under these conditions, we examined p53 and bax protein levels, and p53 and bax mRNA expression to assess the potential relationship between these two proteins for the induction of apoptosis. The p53 protein, which is usually detected in trace amounts in normal cells, was highly expressed in untreated MFH-2NR cells, and the level did not increase after heat treatment, whereas the bax protein level increased from 30 min after the treatment. No change in p53 mRNA was found, but a transient increase in bax mRNA, peaking at 30 min, was detected by Northern blotting. DNA sequence analysis of the p53 gene from MFH-2NR cells demonstrated a GGG right arrow GAG homozygous point mutation in codon 242 of exon 6. These results suggest that the expression of bax protein and mRNA was augmented by a p53-independent pathway in the hyperthermia-induced apoptosis of MFH-2NR cells.

Published

2002

20. RETROSPECTIVE STUDY ON BLEEDING SCORE OF UPPER GASTROINTESTINAL TRACT AND TRANSFUSION IN THE TOKYO ER BOKUTOH

Author

Shigeko Nishimura, Saiko Kurosawa, Takao Horiuchi, Yuki Hazama, Hiroshi Fujita, Akihiko Moriyama, Shoko Fujimoto, Kyoko Daibo, and Emi Yamamoto

Subjects

medicine.medical_specialty, business.industry, medicine, Upper gastrointestinal, Retrospective cohort study, business, Surgery

Published

2010

21. Mouse Myosin X: Molecular Architecture and Tissue Expression as Revealed by Northern Blot and in Situ Hybridization Analyses

Author

Satoshi Yonezawa, Takayuki Takahashi, Seizo Koshiba, Atsuko Hanai, Shin-ichi Sonta, Takao Ono, Takashi Kageyama, Atsushi P. Kimura, Akihiko Moriyama, and Shigeo Masaki

Subjects

Male, Talin, Gene isoform, Molecular Sequence Data, Biophysics, macromolecular substances, In situ hybridization, Myosins, Biology, Biochemistry, Mice, Testis, Myosin, medicine, Animals, Humans, Coding region, Tissue Distribution, Amino Acid Sequence, Northern blot, Molecular Biology, In Situ Hybridization, In Situ Hybridization, Fluorescence, Gene Library, Mice, Inbred BALB C, Messenger RNA, Sertoli Cells, Sequence Homology, Amino Acid, Spermatid, Reverse Transcriptase Polymerase Chain Reaction, Blood Proteins, Cell Biology, Blotting, Northern, Phosphoproteins, Molecular biology, Protein Structure, Tertiary, Pleckstrin homology domain, medicine.anatomical_structure, Chromosomes, Human, Pair 5, Signal Transduction

Abstract

The structure of the coding region of mouse myosin X cDNA was determined. The predicted protein sequence indicated an approximately 240 kDa molecular mass with 2062 amino acids. When aligned with the structure predicted for calf myosin X (GenBank Accession No. U55042), extremely highly conserved pleckstrin homology domains and a myosin tail homology 4 domain were apparent in the tail region, suggesting their importance for myosin X's function. Northern blot analysis revealed the existence of a myosin X mRNA, 8.7 kb in size, in various mouse tissues, while a similar size of human type myosin X mRNA was recognized mainly in the testis. In addition to the adult-type transcripts in mice, a smaller embryo-specific mRNA, 4.8 kb in size, was identified in early to late embryonic stages, suggesting the presence of a shorter myosin X isoform in mouse embryos. In situ hybridization experiments with mouse testis revealed that myosin X mRNA was restricted to Sertoli cells at stages VIII–X of the spermatogenesis cycle, suggesting that myosin X is implicated in the supporting cells during the spermatid morphogenesis.

Published

2000

22. Identification of Components of the Intrafollicular Bradykinin-Producing System in the Porcine Ovary1

Author

Iwao Ohkubo, Takayuki Takahashi, Akihiko Moriyama, Takahiro Kihara, and Atsushi P. Kimura

Subjects

chemistry.chemical_classification, High-molecular-weight kininogen, Bradykinin, RNA, Ovary, Cell Biology, General Medicine, Kallikrein, Biology, Follicular fluid, chemistry.chemical_compound, medicine.anatomical_structure, Enzyme, Reproductive Medicine, chemistry, Biochemistry, medicine, Northern blot

Abstract

As a step in elucidating the biological role of plasma kallikrein (PK) present in the follicular fluid of mammalian ovaries, we examined pig ovary fluid to determine its constituent activators and substrates. Using the inactive precursor form of plasma kallikrein (prePK) as a substrate, we purified an enzyme capable of activating this protein. The prePK-activating enzyme was shown to be the active enzyme blood coagulation factor XIIa. We also isolated high molecular weight kininogen (HMW-K) from the same fluid. Incubation of HMW-K with the ovarian follicular fluid PK resulted in the production of the nanopeptide bradykinin (BK). Expression of prePK, blood coagulation factor XII, and HMW-K was examined by Northern blot analysis using ovary and liver poly(A)+ RNA. All these transcripts were found in the liver, but none were found in the ovary. In addition, it was found that BK levels in the fluid derived from the small follicles were approximately 6 times higher than those from medium and large fol...

Published

2000

23. Molecular and Biochemical Characterization of a Serine Proteinase Predominantly Expressed in the Medulla Oblongata and Cerebellar White Matter of Mouse Brain

Author

Motohiro Kaya, Takayuki Takahashi, Ikuya Yoshida, Atsushi P. Kimura, Akihiko Moriyama, Nobuo Takagi, Naoko Yamashiki, and Hitoshi Matsui

Subjects

Transcription, Genetic, medicine.medical_treatment, Molecular Sequence Data, Biology, Biochemistry, Substrate Specificity, Serine, Mice, chemistry.chemical_compound, Lysyl endopeptidase, Cerebellum, Tumor Cells, Cultured, medicine, Animals, Cloning, Molecular, Molecular Biology, Medulla Oblongata, Protease, Base Sequence, Kunitz STI protease inhibitor, cDNA library, Serine Endopeptidases, Leupeptin, Chromosome Mapping, Cell Biology, Molecular biology, Recombinant Proteins, Mice, Inbred C57BL, chemistry, Serine Proteinase Inhibitors, Antipain

Abstract

A full-length cDNA clone of a serine proteinase, mouse brain serine proteinase (mBSP), was isolated from a mouse brain cDNA library. mBSP, which has been recently reported to be expressed in the hair follicles of nude mice, is most similar (88% identical) in sequence to rat myelencephalon-specific protease. The mBSP mRNA was steadily expressed in the brain of adult mice with a transient expression in the early fetal stage during development. The genomic structure of the mouse gene for mBSP was determined. The gene, which is mapped to chromosome 7B4-B5, is about 7.4 kilobases in size and contains 7 exons. Interestingly, the 5'-untranslated region of the mBSP gene was interrupted by two introns. In situ hybridization analyses revealed that mBSP is expressed in the white matter of the cerebellum, medulla oblongata, and capsula interna and capsula interna pars retrolenticularis of mouse brain. Further, mBSP was immunolocalized to the neuroglial cells in the white matter of the cerebellum. Recombinant mBSP was produced in the bacterial expression system and activated by lysyl endopeptidase digestion, and the activated enzyme was purified for characterization. The enzyme showed amidolytic activities preferentially cleaving Arg-X bonds when 4-methylcoumaryl-7-amide-containing peptide substrates were used. Typical serine proteinase inhibitors, such as diisopropyl fluorophosphates, phenylmethanesulfonyl fluoride, soybean trypsin inhibitor, aprotinin, leupeptin, antipain, and benzamidine, strongly inhibited the enzyme activity. The recombinant mBSP effectively hydrolyzed fibronectin and gelatin, but not laminin, collagens I and IV, or elastin. These results suggest that mBSP plays an important role in association with the function of the adult mouse brain.

Published

2000

24. Cloning of a Rat Glia Maturation Factor- (rGMFG) cDNA and Expression of Its mRNA and Protein in Rat Organs

Author

Kiyofumi Asai, Yuichiro Inoue, Toyohiro Tada, Kaori Fujita, Hideki Tsuiki, Yoshiro Wada, Taiji Kato, Manami Yamamoto, Akihiko Moriyama, and Yoko Kawai

Subjects

Glia Maturation Factor, Male, DNA, Complementary, Blotting, Western, Molecular Sequence Data, In situ hybridization, Glia maturation factor, Biology, Biochemistry, Western blot, Pregnancy, Complementary DNA, Testis, Gene expression, Escherichia coli, medicine, Animals, Tissue Distribution, Amino Acid Sequence, RNA, Messenger, Northern blot, Cloning, Molecular, Molecular Biology, Peptide sequence, In Situ Hybridization, Messenger RNA, Base Sequence, Sequence Homology, Amino Acid, medicine.diagnostic_test, Brain, General Medicine, Blotting, Northern, Molecular biology, Rats, Female

Abstract

We isolated a rat glia maturation factor-gamma(rGMFG) cDNA and examined the tissue distribution of GMFG in rat by Northern and Western blot analyses. Sequence analysis of the entire cDNA revealed an open reading frame of 426 nucleotides with a deduced protein of 142 amino acid residues. The deduced amino acid sequence of the putative product is highly homologous (78.9%) to rat glia maturation factor-beta (rGMFB). Northern blot analysis indicated that a 0.9-kb mRNA is predominantly expressed in rat thymus, testis, and spleen. GMFG showed a different tissue distribution from GMFB, being present predominantly in proliferative and differentiative organs.

Published

2000

25. Molecular Cloning of Neonate/Infant-Specific Pepsinogens from Rat Stomach Mucosa and Their Expressional Change during Development

Author

Masao Ichinose, Yuichi Narita, Satoshi Yonezawa, Akihiko Moriyama, Masao Omata, Takashi Kageyama, and Shinko Tsukada-Kato

Subjects

Aging, Pepsinogen C, Molecular Sequence Data, Biophysics, Biology, Molecular cloning, digestive system, Biochemistry, Pepsin, Pepsinogen A, Complementary DNA, Gene expression, Gastric mucosa, medicine, Animals, Humans, Amino Acid Sequence, Northern blot, Cloning, Molecular, Molecular Biology, Gene, Phylogeny, Sequence Homology, Amino Acid, Cell Biology, Chromatography, Ion Exchange, Molecular biology, Recombinant Proteins, digestive system diseases, Rats, medicine.anatomical_structure, Animals, Newborn, Gastric Mucosa, Vertebrates, biology.protein, Macaca, Chymosin, Sequence Alignment

Abstract

To clarify the nature of rat neonate/infant-specific pepsinogens, we carried out their purification and molecular cloning. Prochymosin was found to be the major neonatal pepsinogen. The general proteolytic activity of its active form, chymosin, was, however, lower than those of pepsins A and C which are predominant in adult animals. Molecular cloning of rat prochymosin cDNA was achieved along with cDNA for another neonate-specific pepsinogen, pepsinogen F, although determination of pepsinogen F in neonatal gastric mucosa was unsuccessful, presumably due to its lack of proteolytic activity or different proteolytic specificity. Northern blot analysis confirmed that genes for prochymosin and pepsinogen F are expressed only at neonatal/infant stages and the switching of gene expression to that of pepsinogen C occurred at late infant stages. A phylogenetic tree based on nucleotide sequences showed clearly that pepsinogens fall into four major groups, namely prochymosin and pepsinogen F of the neonate/infant and pepsinogens A and C of adult animals. Although, to date, prochymosin and pepsinogen F were believed to be expressed in only a limited number of mammals, the present results suggest that they might be expressed at the neonatal/infant stage in a variety of mammals.

Published

2000

26. Defective Myosin Genes in Mutant Mice and Human Diseases

Author

Takashi Kageyama, Shin-ichi Sonta, Satoshi Yonezawa, Atsuko Hanai, Shigeo Masaki, Akihiko Moriyama, and Takao Ono

Subjects

Gene isoform, Genetics, Embryology, Mutation, Alternative splicing, Mutant, General Medicine, Biology, medicine.disease_cause, Pediatrics, Perinatology and Child Health, Myosin, medicine, Allele, Gene, Actin, Developmental Biology

Abstract

Myosins are highly divergent actin-based molecular motors. In five of eight classes expressed in mammals, defects in genes have been identified in mutant mice and/or human diseases. A mutated myosin II-7 gene is one of the causes of human familial hypertrophic cardiomyopathy (FHC). The defective myosin Va gene is responsible for Griscelli disease, which is characterized by partial albinism and immunodeficiency, while in its mouse homologue coat color dilution is seen with or without neurological defects. There are three classes of myosins, VI, VII and XV, that are essential in the inner ear function. In humans, mutations in the VIIa gene are associated with three deafness-related diseases, Usher 1B/DFNB2/DFNA11, providing the first example of exhibition of recessive- and dominant-inherited disorders by different mutations in a single myosin gene. There are variations in phenotype between human diseases and their mouse models, which appear to be explicable on the basis of differences in tissue expression patterns of the given myosin between mouse and man. In FHC and Usher 1BDFNB2DFNA11, a wide spectrum of clinical symptoms are observed. Evidence has accumulated suggesting that the more functionally important the mutation site of the molecule, the more serious and severe the symptoms, although involvement of additional factors such as modifier genes and genetic background can not be ruled out. Molecular genetic analyses of a variety of dilute alleles in mice have greatly facilitated our understanding of genotype-phenotype correlations, including information about structurally and functionally important domains of the myosin Va protein and cell-type-specific functions of different isoforms produced by alternative splicing.

Published

1999

27. Development-Dependent Expression of Cathepsins D and E in Various Rat Tissues, with Special Reference to the High Expression of Cathepsin E in Fetal Liver

Author

Akihiko Moriyama, Satoshi Yonezawa, Masao Ichinose, Naohisa Yahagi, Takashi Kageyama, Kazumasa Miki, and Masae Tatematsu

Subjects

Cathepsin, chemistry.chemical_classification, Fetus, Cell, Cathepsin D, Spleen, Cathepsin E, Biology, Andrology, medicine.anatomical_structure, Enzyme, Fetal Stage, chemistry, Immunology, medicine, Animal Science and Zoology

Abstract

The levels of cathepsins D and E in various rat tissues during development were determined with the sensitive assay method we have developed. The level of cathepsin D increased gradually in each tissue during fetal development suggesting the gradual maturation of the lysosomal system in a cell. The level of cathepsin E differed significantly between tissues at various developmental stages. The level in liver increased rapidly from 13-day-gestation fetal stage and decreased gradually at later fetal stages. The level in other tissues such as stomach and spleen began to increase at later fetal stages or the infant stage. Cathepsin E was found in fetal hepatocytes and its gene was hypomethylated when the expression of the gene was elevated. The enzyme was found to be present mainly as a proform suggesting that, after working, an active form is rapidly inactivated.

Published

1998

28. Development-Dependent Expression of Cathepsins D and E in Various Rat Tissues, with Special Reference to the High Expression of Cathepsin E in Fetal Liver

Author

Takashi Kageyama, Masae Tatematsu, Masao Ichinose, Naohisa Yahagi, Kazumasa Miki, Akihiko Moriyama, and Satoshi Yonezawa

Subjects

Animal Science and Zoology

Abstract

The levels of cathepsins D and E in various rat tissues during development were determined with the sensitive assay method we have developed. The level of cathepsin D increased gradually in each tissue during fetal development suggesting the gradual maturation of the lysosomal system in a cell. The level of cathepsin E differed significantly between tissues at various developmental stages. The level in liver increased rapidly from 13-day-gestation fetal stage and decreased gradually at later fetal stages. The level in other tissues such as stomach and spleen began to increase at later fetal stages or the infant stage. Cathepsin E was found in fetal hepatocytes and its gene was hypomethylated when the expression of the gene was elevated. The enzyme was found to be present mainly as a proform suggesting that, after working, an active form is rapidly inactivated.

Published

1998

29. [Untitled]

Author

Tadahisa Miyamoto, Akihiko Moriyama, Takashi Joh, Taiji Kato, Toshihiko Takeuchi, Naotsuka Okayama, and Makoto Itoh

Subjects

Messenger RNA, Forskolin, Physiology, Gastroenterology, Biology, Molecular biology, Guinea pig, Gastric chief cell, chemistry.chemical_compound, chemistry, Cell culture, Ionomycin, Gene expression, Protein kinase C

Abstract

We have investigated the effects of dibutyrylcAMP, forskolin, carbamylcholine chloride (carbachol),ionomycin, and 12-O-tetradecanoylphorbol-13-acetate(TPA) on the expression of guinea pig pepsinogen mRNA in monolayer cultured gastric chief cells.After exposure of the cells to each of these compoundsfor 4 to 24 hr, and at 48 hr after primary culture,total cellular RNA was isolated using acidguanidium-phenol-chloroform and then was reverse transcribed to cDNA.Obtained cDNA was amplified by polymerase chain reaction(PCR) using primers detecting guinea pig pepsinogen mRNAand human β-actin mRNA as an internal standard. The PCR products were separated and quantifiedusing capillary electrophoresis. Dibutyryl cAMP andforskolin significantly increased pepsinogen mRNA, butcarbachol, ionomycin, and TPA failed to increase that. These findings suggested that pepsinogengene expression was up-regulated by intracellular cAMP,but not by intracellular calcium or protein kinase C inguinea pig chief cells.

Published

1998

30. Application of High-Performance Capillary Electrophoresis to Quantification of Products of the Reverse Transcriptase-Polymerase Chain Reaction

Author

Akihiko, Moriyama, Kohei, Matsukawa, Minako, Matsubara, Taiji, Kato, Institute of Natural Sciences, Nagoya City University, Department of Bioregulation, Biomedical Institute, Nagoya City University, Medical School, and Department of Bioregulation, Biomedical Institute, Nagoya

Subjects

PCR, capillary electrophoresis, gliostatin

Abstract

To apply the high-performance capillary electrophoresis (HPCE) to the quantification of RT-PCR products, the conditions for the routine measurement were established as follows: the reaction mixture after RT-PCR (1 μl) was diluted 20-fold with deionized water and introduced into the capillary tube by electrokinetic injection at -10 kV for 40 sec. Electrophoresis was performed at -13 kV for 21 min. DNA was quantified spectrophotometrically at 260 nm during electrophoresis. This method was applied to the quantification of gliostatin mRNA in A 431 cells and compared to the amount of corresponding protein. The amount of gliostatin mRNA was well correlated with that of the protein (r = 0.733), when RT-PCR products derived from β-actin were used as internal standards. The data indicate that HPCE is useful to quantitate mRNA levels in cells.

Published

1997

31. [Untitled]

Author

Akihiko Moriyama, Hiromi Kataoka, Takashi Joh, Taiji Kato, and Kunio Kasugai

Subjects

medicine.medical_specialty, Platelet-derived growth factor, Physiology, Growth factor, medicine.medical_treatment, Basic fibroblast growth factor, Gastroenterology, Biology, In vitro, chemistry.chemical_compound, Endocrinology, chemistry, Epidermal growth factor, Internal medicine, medicine, biology.protein, Thymidine, Platelet-derived growth factor receptor, Transforming growth factor

Abstract

This study was performed to define thebiologically active growth modulators in human gastricjuice. Mitogenic activity was evaluated by theincorporation of [3H]thymidine into 3T3fibroblasts. A negative correlation was observed between pH andmitogenic activity in gastric juice (r = –0.45, P< 0.01). The concentrations of epidermal growthfactor (EGF), transforming growth factor-α and-β1 (TGF-α and -β1), platelet-derived growth factor 1(PDGF), and basic fibroblast growth factor (bFGF) ingastric juice did not explain these changes in mitogenicactivity. Gel filtration identified growth-stimulatingactivity due to small molecule mitogens (less than 13kDa), and growth inhibitory activity only in neutralsamples due to a macromolecular substance (larger than240 kDa) susceptible to trypsin digestion and heat and acid treatments. We conclude thatacidity-dependent changes in mitogenic activity observedin this study are due to appearance of acid-unstable,high-molecular-weight, growth-inhibitorysubstance.

Published

1997

32. Tissue distribution of human gliostatin/platelet-derived endothelial cell growth factor (PD-ECGF) and its drug-induced expression

Author

Kohei Matsukawa, Akihiko Moriyama, Taiji Kato, Yoko Kawai, and Kiyofumi Asai

Subjects

Cell, Expression, Nerve Tissue Proteins, Distribution, Biology, Polymerase Chain Reaction, Enzyme immunoassay, Cell Line, Immunoenzyme Techniques, Receptors, Glucocorticoid, Tumor Cells, Cultured, Extracellular, medicine, Gliostatin, Humans, Cytotoxic T cell, Secretion, Thymidine phosphorylase, Molecular Biology, Thymidine Phosphorylase, Kidney, Platelet-derived endothelial cell growth factor, Cell Biology, Molecular biology, Kinetics, medicine.anatomical_structure, Gene Expression Regulation, Epidermoid carcinoma, Biochemistry, Cell culture, Reverse transcription polymerase chain reaction

Abstract

Human tissue contents of gliostatin/platelet-derived endothelial cell growth factor (PD-ECGF) and its drug-induced expression in tumor cells were currently examined by a sandwich enzyme immunoassay (EIA) system and a reverse transcription-polymerase chain reaction (RT-PCR) method. Gliostatin/PD-ECGF was found to distribute in rather ubiquitous than specific human tissues and organs, with a relatively high levels in the tissues of digestive system (esophagus and rectum), brain, spleen, bladder and lung, but not in gall bladder, aorta, muscle, fat and kidney. Most of examined human tumor cell lines showed 4- or 5-fold higher contents (21.5 ± 3.9 ng/mg protein) than normal tissue contents (4.4 ± 1.1 ng/mg protein) on the average. While gliostatin/PD-ECGF is known to lack a signal sequence, some tumor cells (A431 and MKN74) appeared to release it into the conditioned medium. Expression of gliostatin/PD-ECGF in epidermoid carcinoma cell (A431) and stomach cancer cell (MKN45) was induced by dibutyryl cyclic AMP and phorbol ester, and uniquely in MKN45 by hydrocortisone. In particular, this hydrocortisone specifically caused an increase of the apparent secretion of MKN74 without its cytotoxic effects, suggesting a possible secretion of gliostatin/PD-ECGF in the restricted but not universal cell line. Biological significance on the chemical induction of gliostatin/PD-ECGF in tumor cells and on its extracellular secretion are discussed.

Published

1996

33. Hyperthermia induces apoptosis in malignant fibrous histiocytoma cellsin vitro

Author

Kohichi H. Kato, Hideki Tsuji, Takanobu Otsuka, Taiji Kato, Akihiko Moriyama, Masato Yonezawa, and Nobuo Matsui

Subjects

Cancer Research, Programmed cell death, education.field_of_study, Pathology, medicine.medical_specialty, Necrosis, Cell growth, Cell, Population, Cell cycle, Biology, Molecular biology, medicine.anatomical_structure, Oncology, Terminal deoxynucleotidyl transferase, Apoptosis, medicine, medicine.symptom, education

Abstract

The effect of mild hyperthermia on a cultured rat malignant fibrous histiocytoma (MFH) cell line, MFH-2NR, was investigated. MFH cells in log-phase (growing phase) were heated at 41 degrees-44 degrees C for 1 hr. Hyperthermic treatment at 41 degrees C did not substantially affect cell proliferation and treatment at 44 degrees C caused necrosis. After hypothermic treatment at 42 degrees or 43 degrees C, proliferation of MFH cells was arrested and morphological changes characteristic of apoptosis, cell shrinkage accompanying apoptotic bodies and chromatin condensation, became apparent. Hyperthermia-induced apoptosis was further confirmed by terminal deoxynucleotidyl transferase staining and a ladder pattern on agarose gel electrophoresis. Flow cytometric analysis indicated that the population in the G1 phase of the cell cycle significantly decreased with a concomitant increase in apoptotic cells, indicating that apoptosis might occur mainly in the G1 phase population.

Published

1996

34. Mediation of pepsinogen secretion from guinea pig chief cells by Ca2+/calmodulin-dependent protein kinase II

Author

Makoto Itoh, Tatsuo Suzuki, Toshihiko Takeuchi, Taiji Kato, Akihiko Moriyama, Tadahisa Miyamoto, Takashi Joh, and Naotsuka Okayama

Subjects

Male, endocrine system, medicine.medical_specialty, Calcium ion, intracellular, Calmodulin, Pepsinogen secretion, Guinea Pigs, Monolayer culture, Piperazines, KN-62, chemistry.chemical_compound, 1-(5-Isoquinolinesulfonyl)-2-Methylpiperazine, Internal medicine, medicine, Animals, Secretion, Phosphorylation, Molecular Biology, Cells, Cultured, Forskolin, Pepsinogens, biology, Ionomycin, Autophosphorylation, Calcium/calmodulin-dependent protein kinase II, Cell Biology, Isoquinolines, Immunohistochemistry, Molecular biology, Gastric chief cell, Endocrinology, chemistry, Gastric Mucosa, Calcium-Calmodulin-Dependent Protein Kinases, biology.protein, Carbachol, autophosphorylation, Calcium-Calmodulin-Dependent Protein Kinase Type 2, Intracellular

Abstract

In the presence of Ca2+ bound to calmodulin, Ca2+/calmodulin-dependent protein kinase II (CaMK II) exhibits an intramolecular autophosphorylation and modulates many cell functions. In this study, the role of CaMK II in pepsinogen secretion was investigated in cultured guinea pig chief cells by using a specific CaMK II inhibitor, 1-[N,O-Bis(5-isoquinolinesulfonyl)-N-methyl-l-tyrosyl]-4-phenyl-piperazine (KN-62), and an antibody for the Thr-286-autophosphorylated α subunit of CaMK II which specifically recognized the autophosphorylated form of CaMK II. KN-62 inhibited the pepsinogen secretion stimulated by carbamylcholine chloride, cholecystokinin octapeptide, and ionomycin in a dose-dependent manner without affecting intracellular Ca 2+ concentrations, but had no effect on the secretion by 12-O-tetradecanoyl phorbol-13-acetate (TPA) and forskolin. Heavy staining with the antibody for autophosphorylated CaMK II was observed in the cytoplasm of chief cells treated with carbamylcholine chloride or ionomycin, but only light staining was seen in cells treated with TPA or forskolin. Thus, CaMK II and its autophosphorylation may be a critical step in the intracellular pathway by which Ca2+ causes pepsinogen secretion from guinea pig chief cells.

Published

1995

35. Aberrant production of gliostatin/platelet-derived endothelial cell growth factor in rheumatoid synovium

Author

Takanobu Otsuka, Masanori Takeuchi, Kiyofumi Asai, Akihiko Moriyama, Kohei Matsukawa, Ichiro Isobe, Nobuo Matsui, Takayoshi Hirano, Yaman Z. Eksioglu, Taiji Kato, and Toyohiro Tada

Subjects

Adult, Pathology, medicine.medical_specialty, Platelet-derived growth factor, Angiogenesis, Blotting, Western, Immunology, Immunoglobulins, Arthritis, Nerve Tissue Proteins, Nitric Oxide, Cell Line, Arthritis, Rheumatoid, Neovascularization, Mice, chemistry.chemical_compound, Rheumatology, Osteoarthritis, Synovial Fluid, Tumor Cells, Cultured, medicine, Animals, Humans, Immunology and Allergy, Synovial fluid, Pharmacology (medical), Immunoassay, Platelet-Derived Growth Factor, Thymidine Phosphorylase, business.industry, 3T3 Cells, medicine.disease, Growth Inhibitors, Rats, medicine.anatomical_structure, chemistry, Synovial Cell, Rheumatoid arthritis, Cancer research, Electrophoresis, Polyacrylamide Gel, medicine.symptom, Synovial membrane, business

Abstract

Objective. To purify a protein inhibitor from rheumatoid arthritis (RA) synovial fluids which suppresses the apparent incorporation of 3H-thymidine into fibroblasts and synovial cells, and to define its biochemical features that have clinical relevance to the pathogenesis of RA. Methods. Several standard chromatographic techniques were employed for the purification of the protein. Immunochemical methods with monoclonal antibody were used to quantify and visualize the protein in sera, synovial fluids, and tissues from RA patients. Results. The chemical properties of purified inhibitor from RA synovial fluids confirmed its identity as gliostatin/platelet-derived endothelial cell growth factor (PD-ECGF), a potent angiogenic factor. The gliostatin/ PD-ECGF level in synovial fluid and serum was higher in RA patients than in osteoarthritis controls. Conclusion. These findings strongly suggest that gliostatin/PD-ECGF might play an important role in the aberrant neovascularization of rheumatoid synovium.

Published

1994

36. [Low-titer cold agglutinin disease following Salmonella gastroenteritis]

Author

Ken-Ichiro, Kobayashi, Tamae, Hamaki, Akira, Ohwada, Junji, Tomiyama, Ryoko, Sakuma, Yoko, Mizuta, Akihiko, Moriyama, Emi, Yamamoto, Itsuo, Akiya, and Hiroshi, Fujita

Subjects

Male, Anemia, Hemolytic, Salmonella Infections, Eosine Yellowish-(YS), Humans, Anemia, Hemolytic, Autoimmune, Middle Aged, Gastroenteritis

Abstract

We encountered a patient with cold agglutinin disease (CAD) that worsened after Salmonella gastroenteritis. A 52-year-old male complained pain in the left fingers with cyanosis and was admitted in a local hospital. After treatment for ischemia, he demonstrated diarrhea with fever. Because of progressive anemia, he was referred to our hospital. Salmonella gastroenteritis was diagnosed based on the results of microbiological examination. Severe hemolysis was noted at admission, and Coombs test was positive (IgG-, C3d+). Cold agglutinin titer was elevated (x256). There were no findings of malignancy or infection demonstrating CA. A diagnosis of CAD with Salmonella gastroenteritis was made. Because spherocytosis was noted during admission, we measured the mean channel fluorescence (MCF) of eosin-5-maleimide (EMA) in erythrocytes from patients. MCF of EMA of the patient's erythrocytes was similar to that of normal subjects. Therefore, we concluded that coexisting hereditary spherocytosis was unlikely. We also examined the in vitro hemolytic effect of Salmonella infection on his blood and on blood from normal subjects. Treatment with Salmonella enteritidis isolated from this patient was found to induce hemolysis in the patient's blood, but not in blood from a normal subject. Moreover, treatment with Salmonella increased the titer of cold agglutinin in vitro. These data suggested that Salmonella infection might worsen hemolysis in CAD.

Published

2011

37. Solubilization and reconstitution of high-and low-affinity Na+-dependent neutral l-α-amino acid transporters from rabbit small intestine

Author

Yasuo Kagawa, Akihiko Moriyama, Hajime Hirata, Makoto Sasaki, Tsunao Tetsuka, and Makoto Nakanishi

Subjects

Amino Acid Transport Systems, Imino acid, Proteolipids, Biophysics, Synthetic membrane, Biochemistry, Substrate Specificity, Valinomycin, chemistry.chemical_compound, Intestine, Small, Animals, Amino acid transporter, Alanine, chemistry.chemical_classification, Alanine transport, Chromatography, Microvilli, Sodium, Biological Transport, Cholic Acids, Cell Biology, Membrane transport, Amino acid, Kinetics, Solubility, chemistry, Rabbits, Carrier Proteins

Abstract

High- and low-affinity Na(+)-dependent neutral L-alpha-amino acid transporters were solubilized with 0.25% octaethylene glycol dodecyl ether (C12E8) after removal of the proteins from the brush-border membrane vesicles with 2% CHAPS and 4 M urea. When the CHAPS-insoluble protein was treated with papain before its solubilization with C12E8, a substantial amount of protein was removed without any decrease of the transport activities. The solubilized transporters were reconstituted into proteoliposomes after removal of C12E8 with Bio-Beads SM2. Several parameters proved to be important for optimal reconstitution efficiency: (a) the type of detergent, and (b) the phospholipid/protein and detergent/protein ratio during reconstitution, and (c) the salt concentration during reconstitution. Reconstituted proteoliposomes showed rapid uptake of neutral L-alpha-amino acids but not imino acid, basic or acidic amino acids driven by an electrochemical potential of Na+ (outin). The uptakes under low- and high-substrate condition were further augmented by an artificial membrane potential introduced by K+ diffusion via valinomycin (negative interior). Kinetic analysis revealed that both the brush-border membranes and the solubilized fraction involved two carrier-mediated pathways for alanine transport. The kinetic parameters were determined by curve fitting with a computer to be Kt1 = 0.28 mM (0.21 mM) and Kt2 = 43.2 mM (28.4 mM), respectively (those with brush-border membrane vesicles in parentheses). Studies on the specific activities for transport of individual amino acids under low or high substrate concentration and the cross-inhibitory effects of various amino acids on alanine uptake (low concentration) revealed that these transporters possess broad specificity for neutral L-alpha-amino acids.

Published

1993

38. Molecular diversity in venom proteins of the Russell's viper (Daboia russellii russellii) and the Indian cobra (Naja naja) in Sri Lanka

Author

Mieko, Suzuki, Takeshi, Itoh, B M, Anuruddhe, I K, Bandaranayake, J G, Shirani Ranasinghe, Seranath B P, Athauda, and Akihiko, Moriyama

Subjects

chemistry.chemical_classification, Serine protease, Elapid Venoms, VIPeR, biology, Naja, Proteins, Venom, General Medicine, Viper Venoms, biology.organism_classification, complex mixtures, Isozyme, General Biochemistry, Genetics and Molecular Biology, Amino acid, Serine, Biochemistry, chemistry, Species Specificity, biology.protein, Animals, Indian cobra, Russell's Viper, Elapidae

Abstract

To examine the molecular diversity of the venom proteins of the Russell's viper (Daboia russellii russellii) and the Indian cobra (Naja naja) in Sri Lanka, we isolated 38 venom proteins through a combination of anion exchange chromatography followed by reversed-phase high performance liquid chromatography. From the venom of D. r. russellii we isolated 15 proteins: 5 isozymes of phospholipase A(2) (PLA(2)), 4 serine proteases, 2 C-type lectin-like proteins, 2 L-amino acid oxidases, 1 cysteine-rich secretory protein (CRISP), and 1 metalloproteinase. From the venom of N. naja we isolated 23 proteins: 10 isoforms of cytotoxins (CTX), 7 PLA(2) isozymes, 2 muscarinic toxinlike proteins, 2 CRISPs, 1 nerve growth factor, and 1 new thrombin-like serine protease. Most of these proteins contained new amino acid sequences for each species, indicating molecular diversity in venom proteins. The entire amino acid sequences of PLA(2)3 from D. r. russellii and CTX7 from N. naja were determined. Additionally, the polymorphic amino acid residues of PLA(2)3 were preferentially localized on the potential antigenic sites. While 2 types of PLA(2) (N and S types) were found in D. r. russellii (India) and D. r. siamensis (Java), all the PLA(2)s from D. r. siamensis (Burma) were N type, and those from D. r. russellii (Sri Lanka) were primarily S type.

Published

2010

39. A Novel Glial Growth Inhibitory Factor, Gliostatin, Derived from Neurofibroma

Author

Akihiko Moriyama, Takayoshi Hirano, Shuji Kaneko, Kiyofumi Asai, Ichiro Isobe, Keiko Nakanishi, Taiji Kato, and Yaman Z. Eksioglu

Subjects

Pathology, medicine.medical_specialty, medicine.drug_class, Blotting, Western, Nerve Tissue Proteins, Endogeny, Glial tumor, Biology, Monoclonal antibody, Biochemistry, Mice, Cellular and Molecular Neuroscience, Column chromatography, Western blot, Tumor Cells, Cultured, medicine, Animals, Mice, Inbred BALB C, Thymidine Phosphorylase, Neurofibroma, medicine.diagnostic_test, DNA synthesis, Tissue Extracts, Cell growth, Antibodies, Monoclonal, Molecular biology, Blot, Female

Abstract

Neurofibroma tissue was investigated for the presence of glial growth modulators that would suppress the proliferation of glial cells. A novel endogenous polypeptide inhibitor of proliferation and DNA synthesis in glial cells, gliostatin, was purified from the extracts of neurofibroma by a procedure comprising dye and anion-exchange column chromatography, and HPLC. A monoclonal antibody raised against partially purified gliostatin showed no cross-reactivity with known cytokines, but adsorbed the growth inhibitory activity of gliostatin and immunochemically visualized the putative gliostatin bands on western blot analyses. Although the product showed an apparent M(r) of 100,000 accompanied by an inhibitory activity on gel filtration column chromatography, it migrated at a lower apparent M(r) of 50,000 under the reducing conditions on western blotting, indicating that a homodimeric structure of native gliostatin consisted of 50-kDa subcomponents. Gliostatin was a potent growth inhibitor acting at nanomolar concentrations against all glial tumor cells and glia maturation factor-stimulated astroblasts, but not neuronal cells.

Published

1992

40. Collagen type-I alpha1 chain mRNA is expressed in the follicle cells of the medaka ovary

Author

Katsueki Ogiwara, Akihiko Moriyama, Maya Horiguchi, Chika Fujimori, and Takayuki Takahashi

Subjects

Messenger RNA, medicine.medical_specialty, biology, Oryzias, Proteolytic enzymes, Ovary, biology.organism_classification, Collagen Type I, Cell biology, Extracellular matrix, medicine.anatomical_structure, Endocrinology, Gene Expression Regulation, Ovarian Follicle, Theca, Internal medicine, Complementary DNA, medicine, Animals, Animal Science and Zoology, Female, RNA, Messenger, Ovarian follicle

Abstract

Follicle rupture during ovulation is a well-regulated biological process of extracellular matrix degradation in the vertebrate ovary. Although proteolytic enzymes responsible for the rupture have recently been identified in the medaka, Oryzias latipes , the lack of knowledge about the ovarian expression and distribution of extracellular matrix components in lower vertebrates prevents the understanding of this process's molecular mechanism. To approach the problem, we cloned a cDNA coding for the medaka collagen type-I alpha1 chain and examined its mRNA expression in the fish ovary. The deduced amino acid sequence of the collagen type-I alpha1 chain was homologous to those of the proteins from other vertebrate species. The alpha1 chain mRNA was expressed in various tissues of the adult fish. In the ovary sections of mature female fish, this mRNA was detected in a line surrounding ovarian follicles of all sizes. A comparison with the distribution of gelatinase B mRNA in follicles that had just ovulated indicated that the collagen type-I alpha1 gene is expressed in the theca cells. The current results strongly suggest that collagen type I is synthesized by theca cells and is localized in the same cell layer of the follicles.

Published

2009

41. Gonad-stimulating substance-like molecule from the radial nerve of the sea cucumber

Author

Akihiko Moriyama, Hideki Katow, and Tomoko Katow

Subjects

Embryology, Invertebrate Hormones, Sea Cucumbers, Molecular Sequence Data, Peptide, chemistry.chemical_compound, Protein structure, Complementary DNA, Animals, Amino Acid Sequence, Peptide sequence, chemistry.chemical_classification, Antiserum, Germinal vesicle, biology, Base Sequence, Neuropeptides, biology.organism_classification, Molecular biology, Molecular Weight, chemistry, Biochemistry, Apostichopus japonicus, Radial Nerve, DNA, Developmental Biology

Abstract

Gonad-stimulating substance-like molecule (GSSL) was isolated from the radial nerve of the sea cucumber, Apostichopus japonicus (Aj-GSSL), and its partial DNA and protein sequences were characterized. The smaller part of the molecule that also retains GSSL activity was estimated. Radial nerve extract (RNE) induced germinal vesicle breakdown (GVBD) at 3 mg/ml in 85% of immature ovarian oocytes. Similar intensity of GSSL activity to RNE was seen in a fraction that contained peptides between 3 kDa and 10 kDa (3-10 kDa-fraction) separated by ultrafiltlation membrane. MALDI-TOF MS analysis and silver-stained 18% SDS-PAGE slab gels identified a major peptide at around 4.6 kDa in a 3-10 kDa-fraction, and that was subjected to internal protein sequencing. The resulting 12-amino acid sequence was not found in the BLAST database to date. Immunohistochemistry using antiserum raised against the 12-amino acid peptide located the peptide to granular cells in the hyponeural part of the radial nerve and in the epineural sinus beneath the radial nerve. Sequence data was obtained using degenerate primers designed from the 12-amino acid sequence and 5 and 3 RACEs. These resulted in a 148 bp cDNA that coded a 43-amino acid sequence of H2N-VLSKQAHHHHHEGWSLPGVPAEIDDLAGNIDYNIFKEQREKIK-COOH. The synthetic 43-amino acid Aj-GSSL generated from this sequence induced GVBD in 50% of immature ovarian oocytes at 6 microM. An N-terminal 21-amino acid peptide of the synthetic partial Aj-GSSL (Aj-GSSL-P1) induced GVBD to 80% of immature ovarian oocytes at 12 microM. This indicated that Aj-GSSL-P1 is of sufficient length for GSSL activity.

Published

2009

42. Redox-dependent structural ambivalence of the cytoplasmic domain in the inner ear-specific cadherin 23 isoform

Author

Akihiko Moriyama, Atsuko Hanai, Norihiro Mutoh, Takashi Kageyama, and Satoshi Yonezawa

Subjects

Gene isoform, Cytoplasm, Protein Conformation, Molecular Sequence Data, Biophysics, Cadherin Related Proteins, Biology, Biochemistry, chemistry.chemical_compound, Structure-Activity Relationship, Protein structure, Species Specificity, otorhinolaryngologic diseases, Animals, Humans, Protein Isoforms, Amino Acid Sequence, Molecular Biology, Cadherin, Cell Biology, Glutathione, Transfection, Cadherins, Molecular biology, Transmembrane protein, Protein Structure, Tertiary, chemistry, Ear, Inner, Oxidation-Reduction, Cysteine

Abstract

Cadherin 23 (Cdh23), an essential factor in inner ear mechano-electric transduction, exists in two alternatively spliced forms, Cdh23(+68) and Cdh23(-68), depending on the presence and absence of exon 68. Cdh23(+68) is inner ear-specific. The exon 68-corresponding region confers an alpha-helical configuration upon the cytoplasmic domain (Cy) and includes a cysteine residue, Cys(3240). We demonstrate here that Cy(+68) as well as the transmembrane (TM) plus Cy(+68) region is present in two different forms in transfected cells, reduced and non-reduced, the latter existing in more compact configuration than the former. The observed characteristic of Cy(+68) was completely abolished by Cys(3240)Ala substitution. Treatment of TMCy(+68)-transfected cells with diethyl maleate, a glutathione depleting reagent, resulted in conversion of the non-reduced to the reduced form of TMCy(+68), suggesting glutathione to be a Cys(3240)-binding partner. Multiple alignment of mammalian Cdh23Cy sequences indicated the occurrence of conformation-inducible Cys in Cdh23Cy of mammals, but not lower vertebrates. The implications of Cys-dependent structural ambivalence of Cdh23 in inner ear mechanosensation are discussed.

Published

2007

43. Zinc-binding property of the major yolk protein in the sea urchin - implications of its role as a zinc transporter for gametogenesis

Author

Tatsuya, Unuma, Kazuo, Ikeda, Keisuke, Yamano, Akihiko, Moriyama, and Hiromi, Ohta

Subjects

Protein Transport, Zinc, Sea Urchins, Blotting, Western, Egg Proteins, Chromatography, Gel, Animals, Electrophoresis, Polyacrylamide Gel, Gametogenesis, Protein Binding

Abstract

Major yolk protein (MYP), a transferrin superfamily protein that forms yolk granules in sea urchin eggs, is also contained in the coelomic fluid and nutritive phagocytes of the gonad in both sexes. MYP in the coelomic fluid (CFMYP; 180 kDa) has a higher molecular mass than MYP in eggs (EGMYP; 170 kDa). Here we show that MYP has a zinc-binding capacity that is diminished concomitantly with its incorporation from the coelomic fluid into the gonad in the sea urchin Pseudocentrotus depressus. Most of the zinc in the coelomic fluid was bound to CFMYP, whereas zinc in eggs was scarcely bound to EGMYP. Both CFMYP and EGMYP were present in nutritive phagocytes, where CFMYP bound more zinc than EGMYP. Saturation binding assays revealed that CFMYP has more zinc-binding sites than EGMYP. Labeled CFMYP injected into the coelom was incorporated into ovarian and testicular nutritive phagocytes and vitellogenic oocytes, and the molecular mass of part of the incorporated CFMYP shifted to 170 kDa. Considering the fact that the digestive tract is a major production site of MYP, we propose that CFMYP transports zinc, essential for gametogenesis, from the digestive tract to the ovary and testis through the coelomic fluid, after which part of the CFMYP is processed to EGMYP with loss of zinc-binding site(s).

Published

2007

44. Human B-lymphocytes express alpha2-6-sialylated 6-sulfo-N-acetyllactosamine serving as a preferred ligand for CD22/Siglec-2

Author

Yasunori Kozutsumi, Yuji Matsuzaki, Hiromu Takematsu, Naoko Kimura, Keiko Miyazaki, Yosuke Yasuda, Reiji Kannagi, Akihiko Moriyama, Katsuyuki Ohmori, and Mineko Izawa

Subjects

Glycan, Lymphoid Tissue, Sialic Acid Binding Ig-like Lectin 2, High endothelial venules, Ligands, Biochemistry, Mice, Sulfation, Cell Line, Tumor, Cell Adhesion, Animals, Humans, Molecular Biology, B-Lymphocytes, Mice, Inbred BALB C, biology, CD22, SIGLEC, Antibodies, Monoclonal, Amino Sugars, Cell Biology, Ligand (biochemistry), Cell biology, carbohydrates (lipids), biology.protein, Lymph, Antibody

Abstract

CD22/Siglec-2, an important inhibitory co-receptor on B-lymphocytes, is known to recognize alpha2-6-sialylated glycan as a specific ligand. Here we propose that the alpha2-6-sialylated and 6-GlcNAc-sulfated determinant serves as a preferred ligand for CD22 because the binding of a human B-cell line to CD22 was almost completely abrogated after incubating the cells with NaClO3, an inhibitor of cellular sulfate metabolism, and was also significantly inhibited by a newly generated monoclonal antibody specific to the alpha2-6-sialylated 6-sulfo-N-acetyllactosamine (LacNAc) determinant (KN343, murine IgM). The alpha2-6-sialylated 6-sulfo-LacNAc determinant defined by the antibody was significantly expressed on a majority of normal human peripheral B-lymphocytes as well as follicular B-lymphocytes in peripheral lymph nodes. The determinant was also expressed in endothelial cells of high endothelial venules of secondary lymphoid tissues, including lymph nodes, tonsils, and intestine-associated lymphoid tissues, more strongly than on B-lymphocytes, suggesting a role for CD22 in B-cell interaction with blood vessels and trafficking. These results indicate that the alpha2-6-sialylated 6-sulfo-LacNAc determinant serves as an endogenous ligand for human CD22 and suggest the possibility that 6-GlcNAc sulfation as well as alpha2-6-sialylation may regulate CD22/Siglec-2 functions in humans.

Published

2007

45. Isolation of novel human cDNA (hGMF-γ) homologous to Glia Maturation Factor-β gene

Author

Taiji Kato, Taeko Hotta, Kiyofumi Asai, Kaori Fujita, Minoru Kokubo, Masayuki Morikawa, Akihiko Moriyama, and Manami Yamamoto

Subjects

Glia Maturation Factor, DNA, Complementary, Sequence analysis, Molecular Sequence Data, Biophysics, Nerve Tissue Proteins, Glia maturation factor, Biology, Biochemistry, Fetus, Protein sequencing, Structural Biology, Complementary DNA, Genetics, Humans, Amino Acid Sequence, Northern blot, Cloning, Molecular, Gene, chemistry.chemical_classification, Base Sequence, Sequence Homology, Amino Acid, Brain, Blotting, Northern, Molecular biology, Amino acid, Open reading frame, chemistry, Organ Specificity

Abstract

A novel full-length human cDNA homologous to Glia Maturation Factor-beta (GMF-beta) gene was isolated. Sequence analysis of the entire cDNA revealed an open reading frame of 426 nucleotides with a deduced protein sequence of 142 amino acid residues. The deduced amino acid sequences of its putative product is highly homologous to human GMF-beta (82% identity) and named for GMF-gamma. Northern blot analysis indicated that a message of 0.9 kb long, but not 4.1 kb of GMF-beta, is predominantly expressed in human lung, heart, and placenta.

Published

1998

46. Effects of cyclosporine A in hyperzincaemia and hypercalprotectinaemia

Author

Tokio Sugiura, Kyoko Ban, Hajime Togari, Kouichi Ito, Kenji Goto, Akihiko Moriyama, and Shoji Okada

Subjects

Anemia, Hepatosplenomegaly, Arthritis, Systemic inflammation, Medicine, Humans, Child, Metal Metabolism, Inborn Errors, Inflammation, Metal metabolism, business.industry, Interleukin, General Medicine, medicine.disease, Increased serum zinc, Zinc, Pyoderma, Pediatrics, Perinatology and Child Health, Immunology, Splenomegaly, Cyclosporine, Cytokines, Female, Calprotectin, medicine.symptom, business, Leukocyte L1 Antigen Complex, Immunosuppressive Agents, Metabolism, Inborn Errors, Hepatomegaly

Abstract

Introduction: Hyperzincaemia and hypercalprotectinaemia with systemic inflammation, recurrent infections, hepatosplenomegaly, arthritis, anemia, cutaneous inflammation, and failure to thrive is an extremely rare disease and no therapy is reported. Aim: To evaluated the effects of cyclosporine A in hyperzincaemia and hypercalprotectinaemia in terms of serum cytokine level changes before and after treatment. Methods: A 10-year-old girl was admitted suffering from pyoderma gangrenosum, hepatosplenomegaly, anemia that was unresponsive to iron supplementation, persistent inflammation, arthritis, and increased serum zinc. The level of serum calprotectin was extremely high; therefore, we diagnosed hyperzincaemia and hypercalprotectinaemia and started cyclosporine A treatment. Twelve cytokines in serum were measured before and one year after treatment. Results: Cyclosporine A was very effective. Her skin lesion and joint pain were alleviated and quality of life was markedly improved. C-reactive protein had decreased and anemia had improved. While zinc levels had fallen, calprotectin remained at an extremely high level. Of the cytokines examined, interleukin -6 serum levels had fallen and interleukin -8 showed a marked reduction after treatment. Conclusion: Cyclosporine A is effective for hyperzincaemia and hypercalprotectinaemia. Serum interleukin -8 may be useful in assessing the therapeutic effects of cyclosporine A in hyperzincaemia and hypercalprotectinaemia.

Published

2006

47. Fates of Cdh23/CDH23 with mutations affecting the cytoplasmic region

Author

Mamoru Sano, Yutaka Inaguma, Takashi Kageyama, Satoshi Yonezawa, Yoshihito Tokita, Moriaki Kusakabe, Norio Yoshizaki, Atsuo Nakayama, Shigeo Masaki, Nobuhiko Sakurai, Atsushi Yoshiki, Takayuki Takahashi, Atsuko Hanai, and Akihiko Moriyama

Subjects

Autophagosome, Cytoplasm, Heterozygote, Autolysosome, Recombinant Fusion Proteins, Immunoblotting, Cadherin Related Proteins, Gene Expression, Biology, Mice, otorhinolaryngologic diseases, Genetics, Animals, Genetics (clinical), Cells, Cultured, Cadherin, Homozygote, Membrane Proteins, Transfection, Cadherins, Molecular biology, Transmembrane protein, Mice, Mutant Strains, Transport protein, Protein Transport, Membrane protein, Mutation

Abstract

BUS/Idr mice carrying a mutant waltzer allele (vbus) are characterized by splayed hair bundles in inner ear sensory cells, providing a mouse homolog of USH1D/DFNB12. RT-PCR-based screening for the presence of mutations in mouse Cdh23, the gene responsible for the waltzer phenotype, has identified a G>A mutation in the donor splice site of intron 67 (Cdh23:c.9633+1G>A: GenBank AF308939.1), indicating that two altered Cdh23 molecules having intron-derived COOH-terminal structures could be generated in BUS mouse tissues. Immunochemical analyses with anti-Cdh23 antibodies showed, however, no clear Cdh23-related proteins in vbus/vbus tissues, while the antibodies immunoreacted with approximately 350 kDa proteins in control mice. Immunofluorescent experiments revealed considerable weakening of Cdh23 signals in sensory hair cell stereocilia and Reissner's membrane in the vbus/vbus inner ear, and transmission electron microscopy demonstrated abundant autophagosome/autolysosome vesicles, suggesting aberrant Cdh23:c.9633+1G>A-derived protein-induced acceleration of lysosomal bulk degradation of proteins. In transfection experiments, signal sequence-preceded FLAG-tagged transmembrane plus cytoplasmic regions (TMCy) of tissue-specific Cdh23(+/-68) isoforms were localized to filamentous actin-rich protrusions and the plasma membrane of cultured cells, whereas FLAG-TMCy:c.9633+1G>A proteins were highly insoluble and retained in the cytoplasm. In contrast, FLAG-tagged TMCy:p.Arg3175His and human TMCy:c.9625_9626insC forms were both localized to the plasma membrane in cultured cells, allowing prediction that USH1D-associated CDH23:p.Arg3175His and CDH23:c.9625_9626insC proteins could be transported to the plasma membrane in vivo. The present results thus suggest different fates of CDH23/Cdh23 with mutations affecting the cytoplasmic region.

Published

2005

48. Biochemical characterization of human kallikrein 8 and its possible involvement in the degradation of extracellular matrix proteins

Author

Katsueki Ogiwara, Akihiko Moriyama, Sanath Rajapakse, Naoharu Takano, and Takayuki Takahashi

Subjects

Collagen Type IV, Proteases, Serine Proteinase Inhibitors, medicine.medical_treatment, Recombinant Fusion Proteins, Biophysics, Biology, Arginine, Biochemistry, Substrate Specificity, Structural Biology, Human kallikrein 8, Genetics, medicine, Escherichia coli, Humans, Molecular Biology, Extracellular Matrix Proteins, Enzymatic characterization, Protease, Activator (genetics), Tissue-type plasminogen activator, Prekallikrein, Caseins, Fibrinogen, Cell Biology, Kallikrein, Fibronectins, Fibronectin, Kinetics, Tissue Plasminogen Activator, biology.protein, Gelatin, Female, Kallikreins, Plasminogen activator, KALLIKREIN 8

Abstract

Human kallikrein 8 (KLK8) is a member of the human kallikrein gene family of serine proteases, and its protein, hK8, has recently been suggested to serve as a new ovarian cancer marker. To gain insights into the physiological role of hK8, the active recombinant enzyme was obtained in a pure state for biochemical and enzymatic characterizations. hK8 had trypsin-like activity with a strong preference for Arg over Lys in the P1 position, and its activity was inhibited by typical serine protease inhibitors. The protease degraded casein, fibronectin, gelatin, collagen type IV, fibrinogen, and high-molecular-weight kininogen. hK8 also converted human single-chain tissue-type plasminogen activator (65kDa) to its two-chain form (32 and 33kDa) by specifically cleaving the peptide bond Arg275–Ile276. This conversion resulted in a drastic increase in the activity of the activator toward the fluorogenic substrate Pyr-Gly-Arg-MCA and plasminogen in the absence of fibrin. Our findings suggest that hK8 may be implicated in ECM protein degradation in the area surrounding hK8-producing cells.

Published

2005

49. Cysteine proteases in sea urchin eggs and embryos of Hemicentrotus pulcherrimus

Author

Akihiko Moriyama, K Kato, Yukio Yokota, Y Hibi, A Yoshikawa, Y Hashimoto, and M Marumoto

Subjects

Hemicentrotus, Proteases, biology, Biochemistry, Chemistry, biology.animal, Embryo, biology.organism_classification, Sea urchin, Cysteine

Published

2004

50. Echinoferrin

Author

Yukio Yokota, Akihiko Moriyama, and Tatsuya Unuma

Subjects

food.ingredient, food, biology, Biochemistry, Chemistry, Yolk, biology.animal, Sea urchin

Published

2004