Your search keyword '"Sakon M"' showing total 13 results

1. ULTRASOUND-MEDIATED NONVIRAL EX VIVO GENE TRANSFER INTO LIVER GRAFT

Author

Gotoh, K, primary, Umeshita, K, additional, Endoh, M, additional, Lu, Z, additional, Marubashi, S, additional, Miyamoto, A, additional, Nagano, H, additional, Dono, K, additional, Nakamori, S, additional, Sakon, M, additional, Kaneda, Y, additional, Uchiyama, Y, additional, and Monden, M, additional

Published

2004

2. DIC COMBINED CT-ANGIOGRAPHY FOR DONOR’S PREOPERATIVE ASSESSMENT IN LRLTX

Author

Kubota, M, primary, Dono, K, additional, Hashimoto, K, additional, Marubashi, S, additional, Miyamoto, A, additional, Nakata, Y, additional, Hori, M, additional, Nagano, H, additional, Nakamori, S, additional, Umeshita, K, additional, Murakami, H, additional, Sakon, M, additional, Nakamura, M, additional, and Monden, M, additional

Published

2004

3. LIVER CONTROLS ALLOIMMUNE RESPONSE FOLLOWING DONOR SPLEEN CELLS INJECTION I

Author

OKUYAMA, M., primary, NAGANO, H., additional, SAKON, M., additional, HE, L., additional, SHIMIZU, J., additional, TAKEDA, Y., additional, DONO, K., additional, UMESHITA, K., additional, NAKAMORI, S., additional, GOTOH, M., additional, and MONDEN, M., additional

Published

1999

4. PROTECTION OF ISLET ALLOGRAFTS TRANSPLANTED TOGETHER WITH FAS LIGAND EXPRESSING TESTICULAR ALLOGRAFTS

Author

TAKEDA, Y., primary, GOTOH, M., additional, NISHIHARA, M., additional, OHTA, Y., additional, OTA, H., additional, GROCHOWIECKI, T., additional, DONO, K., additional, KIMURA, F., additional, NAGANO, H., additional, UMESHITA, K., additional, MATSUURA, N., additional, SAKON, M., additional, MIYASAKA, M., additional, and MONDEN, M., additional

Published

1998

5. Participation of the liver in generation of a vigorous anti-donor response after inoculation of donor spleen cells

Author

He, L., Gotoh, M., Dono, K., Nagano, H., Ota, H., M., ..LN.-Ohta, Y., Okuyama, Shimizu, ..LN.-J., Grochowiecki, T., Sakon, M., and Monden, M.

Published

1999

6. Living-related liver transplantation with renoportal anastomosis for a patient with large spontaneous splenorenal collateral.

Author

Miyamoto A, Kato T, Dono K, Umeshita K, Kawabata R, Hayashi S, Kubota M, Kobayashi S, Nagano H, Nakamori S, Sakon M, and Monden M

Subjects

Adult, Female, Humans, Anastomosis, Surgical methods, Collateral Circulation, Kidney blood supply, Liver Transplantation methods, Living Donors, Portal Vein surgery, Renal Veins surgery, Spleen blood supply

Abstract

Background: A large splenorenal collateral must be interrupted during liver transplantation to secure adequate portal perfusion. However, this process increases the complexity of the operative procedure and may cause hazardous bleeding. Recently, renoportal anastomosis in portal reconstruction was reported in cadaveric liver transplantation for patients with surgically created splenorenal shunts. We used this technique in a living-related liver transplantation., Methods: A 29-year-old female with a large spontaneous splenorenal collateral and a portal venous thrombus underwent a living-related liver transplantation. At surgery, the left renal vein was divided and the distal stump was anastomosed to the portal vein of the graft without interrupting collaterals., Results: Adequate portal venous blood flow was maintained throughout the postoperative course. The patient was discharged 9 weeks after transplantation and remains well., Conclusion: The renoportal anastomosis could be used for portal reconstruction in living-related liver transplantation for patients with a large splenorenal collateral. It provides adequate portal perfusion without interrupting collateral circulation.

Published

2003

7. The inhibitory effect of prostaglandin E1 on oxidative stress-induced hepatocyte injury evaluated by calpain-mu activation.

Author

Kishimoto S, Sakon M, Umeshita K, Miyoshi H, Taniguchi K, Meng W, Nagano H, Dono K, Ariyosi H, Nakamori S, Kawasaki T, Gotoh M, Monden M, and Imajoh-Ohmi S

Subjects

Animals, Calcium metabolism, Cell Membrane drug effects, Enzyme Activation drug effects, Enzyme Activation physiology, Intracellular Membranes metabolism, Isoenzymes metabolism, Liver drug effects, Male, Osmolar Concentration, Protein Kinase C metabolism, Protein Kinase C-alpha, Rats, Rats, Wistar, Alprostadil pharmacology, Calpain metabolism, Liver metabolism, Liver pathology, Oxidative Stress physiology

Abstract

Background: Prostaglandin E1 (PGE1) is known to inhibit ischemia-reperfusion injury of the liver. The calcium-dependent neutral proteinase, calpain-mu, is involved in oxidative stress-induced hepatocyte injury. We investigated the mechanisms of cytoprotection by PGE1, focusing on the elevation of intracellular calcium ([Ca2+]i), activation of calpain-mu, and calpain-mu-mediated activation of protein kinase C-alpha (PKC-alpha)., Methods: Cultured hepatocytes were treated with various amounts of PGE1 (0, 0.1, 1.0, 10, and 100 ng/ml) for 30 min and subsequently with 0.5 mM tert-butyl hydroperoxide (TBHP). Cell injury was evaluated by the release of lactate dehydrogenase. Plasma membrane bleb formation was examined by phase contrast microscopy. Activation of calpain-mu and limited degradation of PKC-alpha was evaluated by Western blotting using antibodies that specifically recognize the amino-terminal regions of calpain-mu and PKC-alpha. [Ca2+]i was measured by confocal microscopy using Fluo-3AM., Results: LDH release from cells treated with 10 ng/ml PGE1 was significantly lower than from untreated cells (135 +/- 12 vs. 258 +/- 18 IU/L, respectively; P < 0.05). Morphologically, many blebs were observed in untreated cells, but very few were seen in those treated with 10 ng/ml PGE1. Western blotting revealed that the amount of activated calpain-mu and [Ca2+]i increased up to 1,300 nM at 35 min after the addition of TBHP (0.5 mmol/L) in control experiments (without PGE1). PGE1 (10 ng/ml) delayed the rise in [Ca2+]i for about 30 min, but did not suppress it completely. PKC-alpha decreased in experiments using PGE1 (10 ng/ml)., Conclusion: PGE1 exerts its cytoprotective effect in TBHP-induced hepatocyte injury partly by inhibiting Ca2+-calpain-mu-mediated mechanisms.

Published

2000

8. Induction of unresponsiveness to islet xenograft by MMC treatment of graft and blockage of LFA-1/ICAM-1 pathway.

Author

Grochowiecki T, Gotoh M, Dono K, Takeda Y, Sakon M, Yagita H, Okumura K, Miyasaka M, and Monden M

Subjects

Animals, Diabetes Mellitus, Experimental surgery, Drug Therapy, Combination, Graft Survival drug effects, Male, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Rats, Rats, Inbred Strains, Antibodies, Monoclonal therapeutic use, Intercellular Adhesion Molecule-1 immunology, Islets of Langerhans Transplantation immunology, Lymphocyte Function-Associated Antigen-1 immunology, Mitomycin therapeutic use, Transplantation, Heterologous immunology

Abstract

Background: Induction of unresponsiveness to graft is one of major interest in xenotransplantation. Two different modalities [direct graft treatment by mitomycin C (MMC) and blockage of the lymphocyte function-associated antigen-1/intracellular adhesion molecule-1 (LFA-1/ICAM-1) pathway in recipients by species-specific mAbs] were tested for their ability to produce unresponsiveness to secondary islet xenografts., Methods: Collagenase-digested WS (RT1k) rat islets, purified by Ficoll density gradient, were incubated for 30 min with MMC 10 microg/ml, cultured for 20 hr, and transplanted into the renal subcapsular space of streptozotocin-induced diabetic C57BL/6 (H-2b) mice. Recipient mice were divided into experimental groups according to anti-rat ICAM-1 and/or anti-mouse LFA-1 mAb treatment and transplantation of MMC-treated or nontreated islets., Results: MMC pretreatment alone prolonged graft survival, with a mean survival time (MST) of 23.0+/-7.4 days, compared with that of cultured islets (12.4+/-2.7 days; P<0.01). MMC treatment of islets significantly augmented graft survival, compared with that of crude islet grafts under treatment with anti-donor ICAM-1 mAb (MST: >41.3+/-30 vs. 16.6+/-5.4 days, P<0.01), anti-recipient LFA-mAb (MST: >70.3+/-28.9 vs. 30.4+/-10.4 days, P<0.001), or both mAbs (MST: >88.1+/-24.1 vs. 23+/-7.4 days, P<0.0001). One of six, four of nine, and six of eight animals accepted MMC-treated islet xenografts over 100 days after treatment with anti-rat ICAM-1, anti-mouse LFA-1, or both mAbs treatments, respectively, whereas none of the animals accepted nontreated islets under the same treatment. When the mice bearing long-term functioning xenografts were challenged with the secondary graft from the original donor strain, the animals previously treated with anti-recipient LFA-1 and anti-donor ICAM-1 mAbs were more prone to accept it than animals given anti-recipient LFA-1 mAb alone (MST: 55.8+/-25.7 vs. 15+/-2.4 respectively; P<0.001), although they rejected the third-party xenograft and allograft acutely., Conclusions: In the xenogeneic islet transplantation model, MMC graft pretreatment and blockage of the ICAM-1/LFA-1 pathway constitute a potent protocol for inducing unresponsiveness to islet xenografts.

Published

2000

9. Pretreatment of crude pancreatic islets with mitomycin C prolongs graft survival time in xenogeneic rat-to-mouse model.

Author

Grtochowiecki T, Gotoh M, Dono K, Takeda Y, Nishihara M, Ohta Y, Ota H, Ohzato H, Okuyama M, Shimizu J, Kimura F, He L, Nagano H, Nakamori S, Umeshita K, Sakon M, and Monden M

Subjects

Animals, Cell Division, Glucose metabolism, Graft Survival drug effects, Islets of Langerhans Transplantation immunology, Lymph Nodes cytology, Male, Mice, Premedication, Rats, Islets of Langerhans drug effects, Mitomycin pharmacology, Transplantation, Heterologous immunology

Abstract

Background: Rejection of pancreatic islet grafts is still a serious problem. We evaluated the effect of mitomycin C (MMC) on the survival of crude islets grafts after xenogeneic islet transplantation., Methods: WS (RT1k) rat islets pretreated with various concentrations of MMC (0, 1, 3.2, 10, 32, 50, 100, 320, and 1,000 microg/ml) were transplanted into C57BL/6 mice with streptozotocin-induced diabetes. In vivo graft function was assessed by a daily measurement of nonfasting blood glucose concentration in each animal. We also examined the separate effect of MMC on purified islets and contaminants present in the crude islet preparation., Results: MMC at doses of 10, 32, 50, and 100 microg/ml resulted in a significant prolongation of the mean graft survival time from a control of 12.4+/-2.5 days to 23+/-7.4, 17.5+/-5.4, 25.5+/-14.7, and 26.7+/-8.9 days, respectively. Deterioration of glucose metabolism was noted when the dose exceeded 32 microg/ml, whereas at 320 microg/ ml, MMC failed to restore normoglycemia. Prolongation of survival time of crude islets was the result of its effect on islets and contaminant components of the crude islet preparation. In vitro study showed that MMC treatment at a higher concentration than 10 microg/ml reduces the stimulatory as well as proliferative capacity of lymph node cells., Conclusions: Pretreatment of pancreatic islets with MMC at 10 microg/ml prolongs xenograft survival without deterioration of in vivo graft function. This novel treatment modality represents a new strategy for the modulation of immunity of islets and contaminants in crude islet preparations.

Published

1999

10. Injection of mitomycin-C-treated spleen cells induces donor-specific unresponsiveness to cardiac allografts in rats.

Author

Tanigawa T, Gotoh M, Nagano H, Ota H, Fukuzaki T, Sakon M, and Monden M

Subjects

Adoptive Transfer, Animals, Hypersensitivity, Delayed immunology, Male, Preoperative Care, Rats, Rats, Inbred BUF, Rats, Inbred Lew, Spleen transplantation, Transplantation, Homologous, Heart Transplantation immunology, Mitomycin pharmacology, Spleen drug effects

Abstract

Background: In this study, preoperative mitomycin-C- (MMC) treated donor-specific transfusion (DST) was examined for its ability to induce unresponsiveness to cardiac allografts in rats., Methods: DA (RT1a) rats were used as donors, BUF (RT1b) or WS (RT1k) rats as recipients, and Lew (RT1l) rats as third party donors. BUF or WS rats were given i.v. injection of DA spleen cells (SPCs) suspension (5x10(7)/l ml) with or without MMC treatment 10 days before cardiac transplantation. Delayed-type hypersensitivity and complement-dependent cytotoxicity assays were carried out in these animals separately to examine in vivo immunosuppressive effect. Suppressor assay was also examined to determine in vitro immunosuppressive effects in allogeneic mixed leukocyte culture., Results: In the full allogeneic DA-to-BUF rat strain combination, preoperative i.v. administration of MMC-treated donor SPCs led to a significant prolongation of graft survival over the control (110+/-66 versus 7.2+/-0.8 days: P<0.01), although administration of nontreated donor SPCs did not (9.3+/-1.0 days). This beneficial effect of MMC treatment was also seen in the DA-to-WS rat combination (31+/-16 days versus donor-specific transfusion alone; 11+/-1.5 days or untreated control; 12+/-1.5 days; P<0.05). However, injection of third party DA SPCs in the Lew-to-BUF combination induced no significant prolongation of cardiac allograft survival compared with the untreated control (11+/-0.6 versus 11+/-2.0 days; NS), indicating that this prolongation effect was induced in an antigen-specific manner. The immunosuppressive effect was also secured for both delayed-type hypersensitivity response and anti-donor cytotoxic antibody production. Moreover, addition of MMC-treated SPCs to mixed lymphocyte culture led to antigen-specific suppression., Conclusions: Preoperative i.v. injection of MMC-treated donor SPCs is promising for inducing unresponsiveness in rat cardiac allograft model.

Published

1999

11. Microchimerism in thymus is associated with up-regulated T helper type 1 cytokine transcription during cardiac allograft rejection in rats.

Author

Ota H, Gotoh M, Ohzato H, He L, Tanigawa T, Nagano H, Dono K, Takeda Y, Okuyama M, Shimizu J, Umeshita K, Nakamori S, Sakon M, Nishisho I, and Monden M

Subjects

Animals, Cell Transplantation, Erythrocyte Transfusion, Male, Polymerase Chain Reaction, RNA, Messenger metabolism, Rats, Rats, Inbred Strains, Rats, Wistar, Spleen metabolism, Spleen pathology, Th1 Cells metabolism, Th2 Cells metabolism, Thymus Gland cytology, Thymus Gland metabolism, Thymus Gland pathology, Chimera physiology, Cytokines genetics, Graft Rejection genetics, Heart Transplantation, T-Lymphocytes, Helper-Inducer physiology, Thymus Gland physiology, Transcription, Genetic physiology

Abstract

Background: Intrathymic microchimerism (MC) is thought to be responsible for inducing allograft tolerance. However, the role of MC in the thymus gland after transplantation, particularly in the rejection response, is unknown. We investigated serial changes in intrathymic cytokine production associated with MC and allograft rejection., Methods: Donor-specific cell injection (DSI) and heterotopic heart transplantation (HTx) were performed in the fully allogeneic combination using DA rats (RT1a) as donors and WS rats (RT1k)as recipients. MC was checked by polymerase chain reaction (PCR) using a donor RT1.Bbeta domain 1 region sequence-specific primers. Reverse transcription (RT)-PCR analysis of cytokine (interleukin [IL]-2, interferon-gamma, IL-4, and IL-10) profiles of the thymus was performed in animals given DSI, HTx, or DSI/HTx., Results: DSI alone resulted in an immediate development of MC, detected by PCR, in various organs including the thymus, spleen, liver, and blood, of most rats, lasting for over 2 months. However, DSI-induced MC selectively disappeared in the thymus on day 7 after grafting, several days before the rejection of cardiac allograft. RT-PCR analysis of cytokine profiles showed that the levels of Th1 (IL-2 and interferon-gamma) cytokines transcribed in the thymus were higher than in the spleen. MC reappeared in the thymus on day 21 after grafting, but was not associated with elevation of Th1 cytokine transcription when allograft was replaced by fibrosis., Conclusions: Intrathymic MC does not always confer unresponsiveness to alloantigen, but can be eliminated after anti-donor response.

Published

1999

12. Direct antigen presentation through binding of donor intercellular adhesion molecule-1 to recipient lymphocyte function-associated antigen-1 molecules in xenograft rejection.

Author

Ohta Y, Gotoh M, Ohzato H, Fukuzaki T, Nishihara M, Dono K, Umeshita K, Sakon M, Yagita H, Okumura K, Tanaka T, Kawashima H, Miyasaka M, and Monden M

Subjects

Animals, Antibodies, Monoclonal pharmacology, Graft Survival immunology, Intercellular Adhesion Molecule-1 immunology, Intercellular Adhesion Molecule-1 isolation & purification, Lymphocyte Activation, Lymphocyte Culture Test, Mixed, Lymphocyte Function-Associated Antigen-1 immunology, Male, Mice, Mice, Inbred C57BL, Rats, Rats, Wistar, Time Factors, Antigen-Presenting Cells immunology, Graft Rejection immunology, Intercellular Adhesion Molecule-1 physiology, Islets of Langerhans Transplantation immunology, Lymphocyte Function-Associated Antigen-1 physiology, T-Lymphocytes immunology, Transplantation, Heterologous immunology

Abstract

Cellular interactions that lead to graft rejection were examined in a rat-to-mouse xenogeneic combination using species-specific monoclonal antibodies (mAbs) against donor and recipient intercellular adhesion molecule-1 (ICAM-1) and lymphocyte function-associated antigen-1 (LFA-1) molecules, respectively. Although both mAbs displayed moderate blocking activity in an in vitro mixed lymphocyte response assay, strong suppression was observed when anti-donor (rat) ICAM-1 mAb was combined with anti-recipient (mouse) LFA-1 mAb. Likewise, significant prolongation of islet xenograft survival was observed with these mAbs. Thus, 0.05 mg of anti-mouse LFA-1 mAb and anti-rat ICAM-1 mAb given on days 0 and 1 produced significant prolongation of graft survival over the control (51+/-20 days vs. 10+/-3 days, P<0.0001), but not when anti-mouse ICAM-1 mAb was combined with anti-mouse LFA-1 mAb (13+/-3 days). In this species combination, mouse T cells were able to proliferate in the presence of rat antigen-presenting cells (APCs) in a cell number-dependent manner, but not in the presence of mouse APCs. The binding assay showed that LFA-1 molecules on mouse T cells can bind immobilized rat ICAM-1 molecules. These results suggest that rat ICAM-1 molecules on APCs can interact with mouse LFA-1 molecules on T cells across a species barrier and that this binding generates the consequent immune responses leading to rejection. mAb treatment against these adhesion molecules of recipient as well as donor is crucial for preventing rejection in a xenogeneic transplantation model.

Published

1998

13. Awareness of donor alloantigens in antiadhesion therapy induces antigen-specific unresponsiveness to islet allografts.

Author

Nishihara M, Gotoh M, Ohzato H, Ohta Y, Luo Z, Dono K, Umeshita K, Sakon M, Monden M, Yagita H, Okumura K, and Miyasaka M

Subjects

Animals, Immunosuppression Therapy methods, Lymphocyte Culture Test, Mixed, Male, Mice, Mice, Inbred BALB C, Mice, Inbred C3H, Mice, Inbred C57BL, Reoperation, Time Factors, Transplantation, Homologous, Antibodies, Monoclonal therapeutic use, Graft Survival immunology, Intercellular Adhesion Molecule-1 immunology, Islets of Langerhans Transplantation immunology, Isoantigens analysis, Lymphocyte Function-Associated Antigen-1 immunology

Abstract

Background: Antiadhesion therapy using monoclonal antibodies (mAbs) to adhesion molecules in vivo has been shown to produce significant prolongation of graft survival in various transplantation models. However, it remains unclear whether antiadhesion therapy operates by merely blocking adhesion between antigen-presenting cells and T cells physically and/or by blocking costimulatory signals while preserving signals mediated through T-cell receptors in vivo. We examined antigen-specific T-cell responses during and after antiadhesion therapy., Methods: BALB/c islets were transplanted into the renal subcapsular space of streptozotocin-induced diabetic C57BL/6 mice given anti-lymphocyte function-associated antigen (LFA)-1 and/or anti-intercellular adhesion molecule-1 mAb treatment. The animals bearing surviving islet allografts were challenged with BALB/c or third-party islets on day 7 or more than 100 days after transplantation., Results: Islet allografts were acutely rejected in untreated animals, with a mean survival time (MST) of 19+/-8 days. Administration of anti-LFA-1 mAb induced significant prolongation of graft survival with a mean survival time of 72+/-33 days, and half of the allografts showed indefinite survival. The animals given anti-LFA-1 mAb alone 7 days before transplantation showed acute rejection of BALB/c islets, whereas a significant number of animals given anti-LFA-1 mAb and the BALB/c islet allograft simultaneously accepted secondary BALB/c islets, but rejected third-party islets. Likewise, most of the animals bearing long-term functioning BALB/c allografts for more than 100 days accepted secondary BALB/c islets, but rejected C3H islets acutely. Interestingly, the spleen cells from these animals transferred unresponsiveness to BALB/c islets into the 2.5-Gy x-irradiated recipients, whereas those from naive animals induced acute rejection., Conclusions: These results indicate that anti-LFA-1 mAb treatment prevents T-cell activation leading to rejection, but results in a T-cell receptor engagement leading to antigen-specific unresponsiveness maintained by transferrable suppressor cells.

Published

1997