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Featured researches published by Koichi Mamba.


Journal of Molecular Histology | 2003

Distribution, Histochemical and Enzyme Histochemical Characterization of Mast Cells in Dogs

Deni Noviana; Koichi Mamba; Susumu Makimura; Yoichiro Horii

This study describes the distribution, proteoglycan properties and protease activity of mast cells from 15 different dog organs. In beagles and mixed breed dogs, staining with Alcian Blue–Safranin O revealed mast cells in all the organs examined. However, their numbers varied and they demonstrated unique localization patterns within some of these organs. Berberine sulphate fluorescence-positive mast cells were observed in the submucosa, muscularis and serosa of the intestines, as well as the tongue and liver (within the connective tissue). Mast cells within the intestinal mucosa were negative for, or demonstrated weak, berberine sulphate staining. Heterogeneity of mast cells in terms of the proteoglycans contained within their granules was further confirmed by determination of critical electrolyte concentrations (CECs). The CECs of mast cells within the connective tissue of several organs, including the intestines (submucosal and muscularis–serosal layers) were all greater than 1.0 M. The results from CEC experiments together with berberine staining indicate that heparin was contained within their granules. Relative to the CECs of mast cells in other organs, mast cells in the intestinal mucosa exhibited lower CECs, suggesting that the proteoglycans within their granules were of lower charge density and/or molecular weight. Although mast cells were classified into two groups by proteoglycans within the granules, enzyme histochemical analysis in beagles revealed three subtypes of mast cells: chymase (MCC), tryptase (MCT) and dual positive (MCTC) cells. There was no correlation between the proteoglycan content and enzyme properties of the mast cell granules.


Histochemical Journal | 2001

Distribution and enzyme histochemical characterisation of mast cells in cats.

Deni Noviana; Fumi Kono; Yuko Nagakui; Hidemi Shimizu; Koichi Mamba; Susumu Makimura; Yoichiro Horii

Mast cells from 15 different cat organs were examined in terms of distribution and protease activity. The number of mast cells in each site was found to vary when visualised by metachromatic staining using Alcian Blue. Enzyme histochemical analysis revealed the existence of two subtypes of mast cells. These were categorised based on protease content, i.e. whether the mast cells contained chymase or tryptase. Tryptase-positive mast cells were clearly identifiable in every organ examined, whereas chymase-containing mast cells were predominantly observed in the ear (skin), tongue, spleen, and submucosa of the stomach and rectum. The chymase-reactive cells were not detected in the heart, or in the muscularis or serosa of the duodenum, jejunum, ileum or rectum. In addition, we suggest the existence of another subtype of mast cell containing both chymase and tryptase and localised within the ear (skin), tongue, spleen and submucosa of the rectum.


Laboratory Animals | 2004

Diurnal variation and age-related changes of bone turnover markers in female Göttingen minipigs

Hideki Tsutsumi; K. Katagiri; M. Morimoto; T. Nasu; M. Tanigawa; Koichi Mamba

We investigated diurnal variation and age-related changes in bone turnover markers in female Göttingen minipigs. Ten females, 6–9 months of age, were used for confirmation of diurnal variation. Blood was collected at 3 h intervals for 24 h, and bone-specific alkaline phosphatase and intact osteocalcin (OC) levels were determined by enzyme immunoassay and radioimmunoassay, respectively. Urine was collected at 3 h intervals for 24 h using a tray attached to the bottom of the cage. The levels of N-terminal telopeptide of type I collagen (NTX) were determined by enzyme immunoassay. Pyridinoline and deoxypyridinoline were measured by high performance liquid chromatography. OC and NTX exhibited diurnal variation (Kruskal–Wallis test, P < 0.05), with the highest and lowest levels at 18:00 h (76.7 ± 26.2 ng/ml) and 06:00 h (44.3 ± 10.3 ng/ml), and at 03:00–05:59 h (550.4 ± 82.4 nmol/μmol Cr) and 12:00–14:59 h (297.8 ± 152.5 nmol/μmol Cr), respectively. In the study of age-related changes, blood and urine samples from 66 females (age range, 3–76 months) were examined to determine the bone turnover markers. All markers showed high correlations with age (0.569 < R 2 < 0.818). High levels of bone turnover markers were observed in young animals, decreasing with age (Kruskal–Wallis test, P < 0.01). The diurnal variation and age-related changes revealed in the present study will be useful in studies of bone diseases using female Göttingen minipigs.


Journal of Molecular Histology | 2007

Gene expression and immunohistochemical localization of megalin in the anterior pituitary gland of helmeted guinea fowl (Numida meleagris)

Claudius Luziga; Masaru Usui; Horii Yoichiro; Rudovick R. Kazwala; Yoshimi Yamamoto; Koichi Mamba

Megalin/the low density lipoprotein receptor-related protein-2 (LRP-2) is expressed in a variety of epithelia and mediates endocytosis of numerous substances. Megalin is also shown to bind clusterin with high affinity. In the pituitary gland, clusterin is localized in endocrine cells, folliculostellate (FS) cells and colloids. The present study examines the expression pattern of megalin within the gland and assesses its cellular localization to that of clusterin so as to deduce their functional implications in colloidal accumulation as relevant in vivo. Quantity of megalin mRNA expression in pituitary and other endocrine tissues was quantified by real-time PCR using SYBR-green I detective system. High levels were detected in kidneys and pituitary. In situ hybridization showed megalin mRNA in FS cells. Megalin protein detected by immunohistochemistry was also observed in FS cells. Immunoelectron microscopy clearly showed the localization of megalin in peripheral region of colloid-containing follicles and on vesicular structures in FS cells. Immunolabeling was also found to be associated with membranes of vacuoles in apoptotic endocrine cells and cell remnants engulfed by FS cells. Double immunofluorescence labeling was performed to determine whether megalin and clusterin in the anterior pituitary were present within the same cell. Simultaneous localization was detected in almost all FS cells surrounding colloids and in several foci of FS cells surrounding endocrine cells. These findings suggest that megalin may drive ingestion of clusterin complexes with products of digested apoptotic endocrine cells in FS cells, and thereby providing a potential mechanism for a receptor mediated uptake of degenerating endocrine cells and secretion of colloid.


Journal of Veterinary Medical Science | 1996

Establishment and Characterization of a New Canine B-Cell Leukemia Cell Line.

Munekazu Nakaichi; Yasuho Taura; Masashi Kanki; Koichi Mamba; Yasuyuki Momoi; Hajime Tsujimoto; Sanenori Nakama


Experimental Animals | 2004

Standardized Data and Relationship between Bone Growth and Bone Metabolism in Female Göttingen Minipigs

Hideki Tsutsumi; Koichi Katagiri; Satoshi Takeda; Tetsuo Nasu; Sinichi Igarashi; Manabu Tanigawa; Koichi Mamba


Tohoku Journal of Experimental Medicine | 2005

Fibrin Stimulates the Proliferation of Human Keratinocytes through the Autocrine Mechanism of Transforming Growth Factor-α and Epidermal Growth Factor Receptor

Misa Yamamoto; Hiroko Yanaga; Hiromichi Nishina; Shoji Watabe; Koichi Mamba


Journal of Veterinary Medical Science | 2006

Characterization and distribution of an arginine vasotocin receptor in mouse.

Masaru Usui; Hitoshi Aoshima; Yoshimi Yamamoto; Claudius Luziga; Koichi Mamba


Zoological Science | 2002

NUCLEOTIDE SEQUENCE DETERMINATION AND EXPRESSION OF BOVINE MITOCHONDRIAL ATP-DEPENDENT PROTEASE(Biochemistry)(Proceedings of the Seventy-Third Annual Meeting of the Zoological Society of Japan)

Shoji Watabe; Misa Yamamoto; Masayuki Hara; Yoshimi Yamamoto; Koichi Mamba; Tomoko Hiroi


Journal of Veterinary Medical Science | 1995

Flow Cytometric Analysis and Immunohistochemistry of Delayed-Type Hypersensitivity Responses in Mice Immunized with Rat Hepatocytes

Shigeyuki Tanabe; Yasuho Taura; Shuichi Furusawa; Yoshikazu Hirota; Michinori Tanaka; Makoto Yokosuka; Kazumasa Kondo; Koichi Mamba; Munekazu Nakaichi; Sanenori Nakama

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Deni Noviana

Bogor Agricultural University

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