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6. Accurate determination of volume and evaporation rate of micron-size liquid particle.

Author

Yamada, T., Sasagawa, N., and Sakai, K.

Subjects
*EVAPORATION (Chemistry), *NUCLEAR liquid drop model, *LIQUIDS, *NOZZLES, *GRAVITY
Abstract

We developed a noncontact method to measure the liquid droplet size of about 10 μm diameter within accuracy of 0.1 μm. A droplet ejected by an inkjet nozzle is induced into the glass windshield and falls due to the gravity against the viscosity of the atmosphere. The droplet is illuminated by a laser passing along the center of the glass windshield and the droplet diameter is determined from the falling velocity by the video analysis with the knowledge about the density of the droplet, and the viscosity of the atmosphere. The real time measurement of the droplet size through the rapid evaporation process thus becomes possible. The evaporation rate from the pure water droplet determined by the present method was found be more than 200 times larger than that from the surface with macroscopic spatial scale. [ABSTRACT FROM AUTHOR]

Published
2010
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7. Clinical Nephrology - Lab methods and other markers

Author

Kleophas, W., primary, Bieber, B., additional, Robinson, B., additional, Duttlinger, J., additional, Fliser, D., additional, Lonneman, G., additional, Rump, L., additional, Pisoni, R., additional, Port, F., additional, Reichel, H., additional, Daniela, R., additional, Ciocalteu, A., additional, Checherita, I. A., additional, Peride, I., additional, Spataru, D. M., additional, Niculae, A., additional, Laetitia, K., additional, Amna, K., additional, Laurence, D., additional, Aoumeur, H.-A., additional, Flamant, M., additional, Haymann, J.-P., additional, Letavernier, E., additional, Vidal-Petiot, E., additional, Boffa, J.-J., additional, Vrtovsnik, F., additional, Bianco, F., additional, Pessolano, G., additional, Carraro, M., additional, Panzetta, G. O., additional, Ebert, N., additional, Gaedeke, J., additional, Jakob, O., additional, Kuhlmann, M., additional, Martus, P., additional, Van der Giet, M., additional, Scha  ner, E., additional, Khan, I., additional, Law, Y., additional, Turgutalp, K., additional, Ozhan, O., additional, Gok Oguz, E., additional, Kiykim, A., additional, Donadio, C., additional, Hatmi, Z. N., additional, Mahdavi-Mazdeh, M., additional, Morales, E., additional, Gutierrez-Millet, V., additional, Rojas-Rivera, J., additional, Huerta, A., additional, Gutierrez, E., additional, Gutierrez-Solis, E., additional, Polanco, N., additional, Caro, J., additional, Gonza z, E., additional, Praga, M., additional, Marco Mayayo, M., additional, Valdivielso, J., additional, Marti  z, M., additional, Fernaez Giraez, E., additional, Obrador, G., additional, Olvera, N., additional, Ortiz de la Pe, D., additional, Gutie ez, V., additional, Villa, A., additional, Redal-Baigorri, B., additional, Sombolos, K., additional, Tsakiris, D., additional, Boletis, J., additional, Vlahakos, D., additional, Siamopoulos, K., additional, Vargiemezis, V., additional, Nikolaidis, P., additional, Iatrou, C., additional, Dafnis, E., additional, Argyropoulos, C., additional, Xynos, K., additional, Schock-Kusch, D., additional, Shulhevich, Y., additional, Geraci, S., additional, Hesser, J., additional, Stsepankou, D., additional, Neudecker, S., additional, Koenig, S., additional, Hoecklin, F., additional, Pill, J., additional, Gretz, N., additional, Schweda, F., additional, Schreiber, A., additional, Kudo, K., additional, Konta, T., additional, Choi, S. O., additional, Kim, J. S., additional, Kim, M. K., additional, Yang, J. W., additional, Han, B. G., additional, Delanaye, P., additional, Cavalier, E., additional, Masson, I., additional, Mehdi, M., additional, Nicolas, M., additional, Lambermont, B., additional, Dubois, B., additional, Damas, P., additional, Krzesinski, J.-M., additional, Morel, J., additional, Lautrette, A., additional, Christophe, M., additional, Gagneux-Brunon, A., additional, Anne, F., additional, Fre (C)ric, L., additional, Bevc, S., additional, Ekart, R., additional, Hojs, R., additional, Gorenjak, M., additional, Puklavec, L., additional, Hashimoto, N., additional, Suzuki, A., additional, Mitsumoto, K., additional, Shimizu, M., additional, Niihata, K., additional, Kawabata, A., additional, Sakaguchi, Y., additional, Hayashi, T., additional, Shoji, T., additional, Okada, N., additional, Tsubakihara, Y., additional, Hamano, T., additional, Nakano, C., additional, Fujii, N., additional, Obi, Y., additional, Mikami, S., additional, Inoue, K., additional, Matsui, I., additional, Isaka, Y., additional, Rakugi, H., additional, Edvardsson, V., additional, Siguron, B., additional, Thorsteinsdottir, M., additional, Palsson, R., additional, Matsumoto, J., additional, Miyazaki, N., additional, Murata, I., additional, Yoshida, G., additional, Morishita, K., additional, Ushikoshi, H., additional, Nishigaki, K., additional, Ogura, S., additional, Minatoguchi, S., additional, Werneke, U., additional, Ott, M., additional, Salander-Renberg, E., additional, Taylor, D., additional, Stegmayr, B., additional, Surel, S., additional, Wenzlova, M., additional, Silva Junior, G., additional, Vieira, A. P., additional, Couto Bem, A., additional, Alves, M., additional, Torres, A., additional, Meneses, G., additional, Martins, A., additional, Liborio, A., additional, Daher, E., additional, Gluhovschi, G., additional, Modilca, M., additional, Daminescu, L., additional, Gluhovschi, C., additional, Velciov, S., additional, Petrica, L., additional, Gadalean, F., additional, Balgradean, C., additional, Schmeiser, H. H., additional, Kolesnyk, M., additional, Stepanova, N., additional, Surzhko, L., additional, Stashevska, N., additional, Filiopoulos, V., additional, Hadjiyannakos, D., additional, Arvanitis, D., additional, Panagiotopoulos, K., additional, Vlassopoulos, D., additional, Kaesler, N., additional, Schettgen, T., additional, Magdeleyns, E., additional, Brandenburg, V., additional, Vermeer, C., additional, Floege, J., additional, Kr, T., additional, Randone, O., additional, Ferraresi, M., additional, Aroasio, E., additional, Depascale, A., additional, Scognamiglio, S., additional, Consiglio, V., additional, Piccoli, G. B., additional, Jensen, L. V., additional, Lizakowski, S., additional, Rutkowski, P., additional, Tylicki, L., additional, Renke, M., additional, Sulikowska, B., additional, Donderski, R., additional, Bednarski, R., additional, Heleniak, Z., additional, Przybylska, M., additional, Manitius, J., additional, Rutkowski, B., additional, Bobrova, L., additional, Kozlovskaya, N., additional, Kanayama, K., additional, Hasegawa, M., additional, Kitagawa, F., additional, Ishii, J., additional, Yuzawa, Y., additional, Tanaka, K., additional, Sakai, K., additional, Hara, S., additional, Suzuki, Y., additional, Tanaka, Y., additional, Aikawa, A., additional, Hinoshita, F., additional, Hamano, N., additional, Sasaki, E., additional, Kato, A., additional, Katsuki, T., additional, Katsuma, A., additional, Imai, E., additional, Shibata, M., additional, Tada, M., additional, Shimbo, T., additional, Kikuchi, Y., additional, Oka, S., additional, Muramatsu, T., additional, Yanagisawa, N., additional, Fukutake, K., additional, Yamamoto, Y., additional, Ajisawa, A., additional, Tsuchiya, K., additional, Nitta, K., additional, Ando, M., additional, Liang, X., additional, Wang, P., additional, Liu, Z., additional, Zhao, Z., additional, Luyckx, V., additional, Bowker, S., additional, Miekle, A., additional, Toth, E., additional, Heguilen, R., additional, Malvar, A., additional, Hermes, R., additional, Cohen, L., additional, Muguerza, G., additional, Lococo, B., additional, Bernasconi, A., additional, Loboda, O., additional, Dudar, I., additional, Krot, V., additional, Alekseeva, V., additional, Ichinose, M., additional, Sasagawa, N., additional, Toyama, K., additional, Saito, A., additional, Kayamori, Y., additional, Kang, D., additional, Kim, H. W., additional, Yoshioka, K., additional, Hara, M., additional, Ohashi, K., additional, Maksudova, A., additional, Khalfina, T., additional, Cuoghi, A., additional, Bellei, E., additional, Caiazzo, M., additional, Bergamini, S., additional, Palladino, G., additional, Monari, E., additional, Tomasi, A., additional, Loiacono, E., additional, Camilla, R., additional, Dapr, V., additional, Morando, L., additional, Gallo, R., additional, Peruzzi, L., additional, Conrieri, M., additional, Bianciotto, M., additional, Bosetti, F. M., additional, Coppo, R., additional, DI Lullo, L., additional, Floccari, F., additional, Rivera, R., additional, Granata, A., additional, Faiola, R., additional, Feliziani, C., additional, Villani, A., additional, Malaguti, M., additional, Santoboni, A., additional, Kyriaki, K., additional, Droulias, J., additional, Bogdanova, M., additional, Rameev, V. V., additional, Simonyan, A. H., additional, Kozlovskaya, L. V., additional, Altiparmak, M. R., additional, Trabulus, S., additional, Akalin, N., additional, Yalin, A. S., additional, Esenkaya, A., additional, Yalin, S. F., additional, Serdengeae(C), K., additional, Arita, D., additional, Cunha, T., additional, Perez, J., additional, Sakata, M., additional, Arita, L., additional, Nogueira, M., additional, Jara, Z., additional, Souza, N., additional, Casarini, D., additional, Metzger, M., additional, Vallet, M., additional, Karras, A., additional, Froissart, M., additional, Stengel, B., additional, Houillier, P., additional, Paul, K., additional, Kretzschmar, D., additional, Yilmaz, A., additional, Ba hlein, B., additional, Titze, S., additional, Figulla, H.-R., additional, Wolf, G., additional, Busch, M., additional, Korotchaeva, Y., additional, Gordovskaya, N., additional, Kozlovskaya, L., additional, Ng, K. P., additional, Sharma, P., additional, Stringer, S., additional, Jesky, M., additional, Dutton, M., additional, Ferro, C., additional, Cockwell, P., additional, Moon, S. J., additional, Lee, S. C., additional, Yoon, S. Y., additional, Lee, J. E., additional, Han, S. J., additional, Anna, B., additional, Kirsch, T., additional, Svjetlana, L., additional, Joon-Keun, P., additional, Jan, B., additional, Johanna, K., additional, Haller, H., additional, Haubitz, M., additional, Smirnov, A., additional, Kayukov, I., additional, Rafrafi, N., additional, Degtereva, O., additional, Dobronravov, V., additional, Koch, M., additional, Stefan, H., additional, Dika, G., additional, Antoine, M.-H., additional, Husson, C., additional, Kos, J., additional, Milic, M., additional, Fucek, M., additional, Cvoriocec, D., additional, Bourgeade, M.-F., additional, Nortier, J. L., additional, Jelakovic, B., additional, Nawal, E. H., additional, Naoufal, M., additional, Nabila, M., additional, Fadwa, E. M., additional, Salma, E. K., additional, Nisrine, B., additional, Mohamed, Z., additional, Guislaine, M., additional, Mohamed Gharbi, B., additional, Benyounes, R., additional, Sotila, G. G., additional, Sorin, R., additional, Irina Magdalena, D., additional, Roxana, C., additional, Claudia, R., additional, Correa Barcellos, F., additional, Hallal, P. H., additional, Bohlke, M., additional, Boscolo Del Vechio, F., additional, Reges, A., additional, Santos, I., additional, Mielke, G., additional, Fortes, M., additional, Antunez, B., additional, Laganovic, M., additional, Vukovic Lela, I., additional, Karanovic, S., additional, Seric, J., additional, Premuic, V., additional, Fitrek, M., additional, Fodor, L., additional, Meljkovic Vrkic, T., additional, Bansal, V., additional, Hoppensteadt, D., additional, and Fareed, J., additional

Published
2012
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21. Delamination of Acuseal early cannulation arteriovenous graft months after implantation.

Author

Suemitsu K, Shiraki T, Miyamoto M, Sasagawa N, Nakamura T, and Izumi M

Subjects
Blood Vessel Prosthesis, Catheterization, Humans, Prosthesis Design, Renal Dialysis, Time Factors, Treatment Outcome, Vascular Patency, Arteriovenous Shunt, Surgical adverse effects, Blood Vessel Prosthesis Implantation adverse effects
Abstract

Arteriovenous fistula is recommended, but arteriovenous graft is acceptable when a fistula is not possible. Acuseal is an early cannulation graft with a trilayer structure. Although primary patency rates of Acuseal appear to be similar to those of other standard grafts, few studies have investigated long-term results and complications. In our series, delamination of the wall structure occurred in 5.1% (6/115) by 21 months after Acuseal implantation. The causes could be divided into cannulation-related and cannulation-unrelated. Here, we describe the six cases in which delamination of the wall structure occurred in the medium term after Acuseal implantation.

Published
2021
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22. Protein C and protein S deficiencies may be related to survival among hemodialysis patients.

Author

Ichinose M, Sasagawa N, Chiba T, Toyama K, Kayamori Y, and Kang D

Subjects
Aged, Female, Follow-Up Studies, Humans, Kidney Failure, Chronic blood, Male, Middle Aged, Protein C Deficiency blood, Protein S Deficiency blood, Protein S Deficiency therapy, Renal Dialysis trends, Survival Rate trends, Kidney Failure, Chronic mortality, Kidney Failure, Chronic therapy, Protein C Deficiency mortality, Protein S Deficiency mortality, Renal Dialysis mortality
Abstract

Background: Thrombophilia due to protein C (PC) and protein S (PS) deficiencies is highly prevalent among patients with stage 5 chronic kidney disease and is reported to arise due to extracorporeal circulation during hemodialysis (HD). This study aimed to evaluate the relationship between HD treatment and thrombophilia., Methods: A total of 114 Japanese patients on maintenance HD (62 men, 52 women) were followed during 2008-2011. Their survival rates were compared against the duration of HD. Prior to each HD, coagulation/fibrinolysis parameters and PC and PS activities were measured using standard techniques. The patients were divided into two groups: Group 1, with PC and/or PS deficiencies (n = 32), and Group 2, without PC and PS deficiencies (n = 82). The influence of such deficiencies and duration of dialysis on survival was examined. Time-to-event analysis was applied using Kaplan-Meier estimates, and the log-rank test was proposed to test the equivalence of relative survival data. Hazard ratios and 95% confidence intervals (CI) were calculated., Results: Of the 114 patients, 37 died (Group 1, 22; Group 2, 15). The hazard ratio (95% CI) was higher (p = 0.004) in Group 1 than Group 2. Gene analyses of PC and PS were performed in 14 patients from Group 1. No mutations in either protein were observed. We analyzed the causes of death in both groups; however, the estimated thrombophilia-related incidence of death could not be determined due to small sample size of HD patients., Conclusions: Our results suggest that PC and PS deficiencies may be related to survival in HD patients. However, this finding warrants additional research.

Published
2019
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23. A freeze-and-thaw method to reuse agarose gels for DNA electrophoresis.

Author

Sasagawa N

Subjects
Buffers, Ethidium chemistry, Gels chemistry, Recycling, Water chemistry, DNA isolation & purification, Electrophoresis, Agar Gel methods, Freezing, Sepharose chemistry
Abstract

A novel protocol to reuse agarose following agarose gel electrophoresis was established in this study. By repeated freeze-and-thaw of the agarose gel, ethidium bromide and other buffer components in the gel were safely removed from the gel without generation of any toxic fume. The agarose recovered using this method can be used for further electrophoretic experiments without any issues.

Published
2018
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24. Duplex ultrasound for the prediction of vascular events associated with arteriovenous fistulas in hemodialysis patients.

Author

Ishii T, Suzuki Y, Nakayama T, Ohmori M, Masai S, Sasagawa N, and Ohyama K

Subjects
Aged, Area Under Curve, Blood Flow Velocity, Brachial Artery diagnostic imaging, Brachial Artery physiopathology, Disease-Free Survival, Female, Graft Occlusion, Vascular etiology, Graft Occlusion, Vascular physiopathology, Graft Occlusion, Vascular therapy, Humans, Kaplan-Meier Estimate, Kidney Diseases diagnosis, Male, Middle Aged, Multivariate Analysis, Predictive Value of Tests, Proportional Hazards Models, ROC Curve, Regional Blood Flow, Reoperation, Risk Factors, Thrombosis etiology, Thrombosis physiopathology, Thrombosis therapy, Time Factors, Treatment Outcome, Vascular Patency, Arteriovenous Shunt, Surgical adverse effects, Brachial Artery surgery, Graft Occlusion, Vascular diagnostic imaging, Kidney Diseases therapy, Renal Dialysis, Thrombosis diagnostic imaging, Ultrasonography, Doppler, Duplex
Abstract

Objective: To determine if duplex ultrasound (US) for arteriovenous fistulas (AVFs) can predict vascular events (VEs; thrombosis and stenosis)., Methods: Duplex US was performed for vascular access evaluation in 2557 maintenance hemodialysis (HD) patients between October 1, 2013 and March 31, 2016. Of these patients, 2184 patients were finally included in this study. AVF dysfunction was assessed using the brachial artery blood flow volume (Qa; mL/min), arterial blood flow resistance index (RI), and residual diameter of the fistula vein (RD; mm). Proximal, midpoint, and distal aspects of the fistulas were measured. The baseline measurements were the US assessments, and the endpoint was VEs requiring vascular access intervention therapy or vascular surgery. Associations of US findings and VEs were assessed with receiver operating characteristic curve analysis, log-rank analysis, and multivariate Cox hazard models., Results: The mean Qa was 772.8 ± 441.4 mL/min; RI, 0.56 ± 0.1; and RD, 2.37 ± 1.0 mm. The optimal Qa cut-off point was calculated as 581.5 mL/min, RI cut-off as 0.56, and RD cut-off as 1.85 mm. VEs were more frequent in patients with a Qa <581.5 mL/min than in those with a Qa >581.5 mL/min (p<0.001). In multivariate analysis, Qa, ferritin, transferrin saturation, and warfarin use were significantly associated with VEs., Conclusions: US evaluation of AVFs in HD patients is a simple method to predict the risks of thrombosis and fistula dysfunction. Qa, ferritin, transferrin saturation, and warfarin use might be associated with VEs.

Published
2016
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25. Sall1 transiently marks undifferentiated heart precursors and regulates their fate.

Author

Morita Y, Andersen P, Hotta A, Tsukahara Y, Sasagawa N, Hayashida N, Koga C, Nishikawa M, Saga Y, Evans SM, Koshiba-Takeuchi K, Nishinakamura R, Yoshida Y, Kwon C, and Takeuchi JK

Subjects
Animals, Gene Expression Regulation, Developmental, Heart Ventricles metabolism, Humans, Mice, Myocardium metabolism, Transcription Factors biosynthesis, Transcription Factors metabolism, Cell Differentiation genetics, Heart Ventricles growth & development, Stem Cells metabolism, Transcription Factors genetics
Abstract

Cardiac progenitor cells (CPCs) are a crucial source of cells in cardiac development and regeneration. However, reported CPCs are heterogeneous, and no gene has been identified to transiently mark undifferentiated CPCs throughout heart development. Here we show that Spalt-like gene 1 (Sall1), a zing-finger transcription factor, is expressed in undifferentiated CPCs giving rise to both left and right ventricles. Sall1 was transiently expressed in precardiac mesoderm contributing to the first heart field (left ventricle precursors) but not in the field itself. Similarly, Sall1 expression was maintained in the second heart field (outflow tract/right ventricle precursors) but not in cardiac cells. In vitro, high levels of Sall1 at mesodermal stages enhanced cardiomyogenesis, whereas its continued expression suppressed cardiac differentiation. Our study demonstrates that Sall1 marks CPCs in an undifferentiated state and regulates cardiac differentiation. These findings provide fundamental insights into CPC maintenance, which can be instrumental for CPC-based regenerative medicine., (Copyright © 2016 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published
2016
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26. Is bypass graft technique effective in arteriovenous graft?

Author

Noguchi T, Miyamoto M, Kataoka K, Sato K, Nihei H, Takeda I, Inoue K, Sasagawa N, and Chiba T

Subjects
Aged, Angioplasty, Balloon, Arteriovenous Shunt, Surgical instrumentation, Blood Vessel Prosthesis, Blood Vessel Prosthesis Implantation instrumentation, Female, Graft Occlusion, Vascular diagnosis, Graft Occlusion, Vascular etiology, Graft Occlusion, Vascular physiopathology, Humans, Kaplan-Meier Estimate, Male, Prosthesis Design, Reoperation, Retrospective Studies, Risk Factors, Thrombosis diagnosis, Thrombosis etiology, Thrombosis physiopathology, Time Factors, Treatment Outcome, Vascular Patency, Arteriovenous Shunt, Surgical adverse effects, Blood Vessel Prosthesis Implantation adverse effects, Graft Occlusion, Vascular surgery, Renal Dialysis adverse effects, Thrombectomy adverse effects, Thrombosis surgery
Abstract

Background: Arteriovenous graft (AVG) requires percutaneous transluminal angioplasty (PTA) to maintain its patency; however, bypass graft technique is often chosen in cases requiring PTA again within 3 months. We retrospectively examined whether bypass graft technique is effective for AVG., Methods: The sample patient population consisted of 50 patients who underwent bypass graft technique on the venous side of the AVG between April 2012 and March 2014. The primary and assisted patencies of the technique were calculated, and compared by the type and length of the bypass graft. Kaplan-Meier method and log-rank test were used for the calculation and comparison of the patency, respectively. p&lt;0.05 was considered statistically significant., Results: The reasons for surgery were thrombotic occlusion (27 cases), frequent PTA (15 cases) and others (8 cases). Frequent PTA was conducted within 3 months in 22 of 27 thrombotic occlusion cases (making 37/50, or 74%). Moreover, thrombectomy was required in 34 cases (68%). The 1-year primary and 1-year assisted patencies of the technique were 6.5% and 72.6%, respectively. When the endpoint was frequent PTA within 3 months after the technique, 1-year primary patency was 45.9%., Conclusions: The 1-year primary patency of the technique was poor, and patency was hard to maintain without the assistance of PTA. Given that frequent PTA was conducted in 74% of patients, it may be a cause for the poor patency. Many cases required thrombectomies, which have the disadvantage of being more invasive than PTA. We concluded that bypass graft technique is not valuable for cases that received frequent PTA.

Published
2015
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27. A high-salinity solution with calcium chloride enables RNase-free, easy plasmid isolation within 55 minutes.

Author

Sasagawa N, Koebis M, Yonemura Y, Mitsuhashi H, and Ishiura S

Subjects
Calcium Chloride chemistry, Plasmids chemistry, Plasmids isolation & purification, Ribonucleases chemistry, Sodium Chloride chemistry
Abstract

We dramatically improved a plasmid-isolation protocol based on the popular alkaline-sodium dodecyl sulfate plasmid isolation method. Our modified method provides significant time and cost savings. We used a modified solution during the neutralization step, which allowed us to skip several subsequent handling steps, saving a great amount of time. The plasmids purified by this method were of high quality, and the optical density ratio 260 and 280 was approximately 1.8. Plasmid DNA isolated by our method was of sufficient quality to perform subsequent restriction enzyme cuts and other downstream experiments, including budding yeast transformation, cultured cell transfection, and Caenorhabditis elegans injection experiments.

Published
2013

28. Complete remission of human parvovirus b19 associated symptoms by loxoprofen in patients with atopic predispositions.

Author

Kazama I, Sasagawa N, and Nakajima T

Abstract

Two cases of women in their thirties with past histories of atopic dermatitis and allergic rhinitis developed a low grade fever, followed by a butterfly-shaped erythema, swelling of their fingers, and polyarthralgia. Despite such symptoms that overlap with those of systemic lupus erythematosus (SLE), the diagnostic criteria for SLE were not fulfilled. Due to positive results for human parvovirus B19 (HPV-B19) IgM antibodies in the serum, diagnoses of HPV-B19 infection were made in both cases. Although acetaminophen failed to improve their deteriorating symptoms, a nonsteroidal anti-inflammatory drug (NSAID), loxoprofen, completely removed the symptoms immediately after the administration. In those cases, since the patients were predisposed to atopic disorders, an increased immunological response based on the lymphocyte hypersensitivity was likely to be involved in the pathogenesis. The immunomodulatory property of NSAID was thought to repress such lymphocyte activity and thus provided a rapid and sustained remission of the disease.

Published
2012
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29. Alternative splicing of myomesin 1 gene is aberrantly regulated in myotonic dystrophy type 1.

Author

Koebis M, Ohsawa N, Kino Y, Sasagawa N, Nishino I, and Ishiura S

Subjects
Base Sequence, CELF1 Protein, Connectin, Consensus Sequence, Exons, HEK293 Cells, Humans, Molecular Sequence Data, Muscle, Skeletal metabolism, Mutation genetics, Myotonic Dystrophy metabolism, RNA Splice Sites, RNA-Binding Proteins metabolism, Alternative Splicing genetics, Gene Expression Regulation, Muscle Proteins genetics, Myotonic Dystrophy genetics
Abstract

Myotonic dystrophy type 1 (DM1) is a multisystemic disease caused by a CTG repeat expansion in the 3'-UTR of dystrophia myotonica-protein kinase. Aberrant regulation of alternative splicing is a characteristic feature of DM. Dozens of genes have been found to be abnormally spliced; however, few reported splicing abnormalities explain the phenotypes of DM1 patients. Thus, we hypothesized that other, unknown abnormal splicing events exist. Here, by using exon array, we identified aberrant inclusion of myomesin 1 (MYOM1) exon 17a as a novel splicing abnormality in DM1 muscle. A cellular splicing assay with a MYOM1 minigene revealed that not only MBNL1-3 but also CELF1 and 2 decreased the inclusion of MYOM1 exon 17a in HEK293T cells. Expression of expanded CUG repeat impeded MBNL1 activity but did not affect CELF1 activity on the splicing of MYOM1 minigene. Our results suggest that the downregulation of MBNL proteins should lead to the abnormal splicing of MYOM1 exon 17a in DM1 muscle., (© 2011 The Authors. Journal compilation © 2011 by the Molecular Biology Society of Japan/Blackwell Publishing Ltd.)

Published
2011
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30. Transgenic rice expressing amyloid β-peptide for oral immunization.

Author

Yoshida T, Kimura E, Koike S, Nojima J, Futai E, Sasagawa N, Watanabe Y, and Ishiura S

Subjects
Agrobacterium tumefaciens genetics, Amyloid beta-Peptides genetics, Amyloid beta-Peptides immunology, Animals, Antibodies blood, Enzyme-Linked Immunosorbent Assay, Mice, Peptide Fragments genetics, Peptide Fragments immunology, Transformation, Bacterial, Vaccines, Edible therapeutic use, Alzheimer Disease immunology, Amyloid beta-Peptides therapeutic use, Immunotherapy, Active methods, Oryza genetics, Peptide Fragments therapeutic use, Plants, Genetically Modified metabolism
Abstract

Various vaccine therapies for Alzheimer's disease (AD) have been investigated. Here we report transgenic rice expressing amyloid β-peptide (Aβ). The Aβ42 gene fused with a green fluorescent protein gene was introduced into rice using the Agrobacterium method. When transgenic brown rice expressing Aβ was orally administered to mice, serum anti-Aβ antibody titers were elevated. The same results were observed when mice were fed boiled, transgenic brown rice. The results indicate that an edible vaccine against AD using rice may be feasible. A vaccine derived from rice would be far cheaper than existing medical vaccines., (© Ivyspring International Publisher.)

Published
2011
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31. Production of anti-amyloid β antibodies in mice fed rice expressing amyloid β.

Author

Nojima J, Ishii-Katsuno R, Futai E, Sasagawa N, Watanabe Y, Yoshida T, and Ishiura S

Subjects
Administration, Oral, Alzheimer Disease immunology, Alzheimer Disease prevention & control, Alzheimer Disease therapy, Amyloid beta-Peptides chemistry, Amyloid beta-Peptides genetics, Animals, Antibody Specificity immunology, Epitope Mapping, Female, Gene Expression, Male, Mice, Plants, Genetically Modified genetics, Th2 Cells immunology, Vaccines, Edible administration & dosage, Vaccines, Edible chemistry, Vaccines, Edible genetics, Amyloid beta-Peptides administration & dosage, Amyloid beta-Peptides immunology, Antibodies immunology, Oryza genetics, Vaccines, Edible immunology
Abstract

The main signs of Alzheimer's disease (AD) are cognitive impairment and senile plaques composed of amyloid beta (Aβ) observed in patients' brains. Therefore, therapy for AD focuses on the removal of Aβ. We developed an "edible vaccine" that employs intestinal immunity with little to no side effects. Rice was utilized as an edible vaccine. It expressed GFP-Aβ42. Aβ rice was administered orally to wild-type (WT) mice causing production of anti-Aβ antibodies. Since Aβ rice was mixed with the cholera toxin B subunit (CTB), antibody against the rice seed protein was also produced. Then, mice were caused to develop immune tolerance against the rice seed protein by oral administration of Aβ rice mixed with CTB. The results indicated that only anti-Aβ antibodies were produced.

Published
2011
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32. Reduction of amyloid beta-peptide accumulation in Tg2576 transgenic mice by oral vaccination.

Author

Ishii-Katsuno R, Nakajima A, Katsuno T, Nojima J, Futai E, Sasagawa N, Yoshida T, Watanabe Y, and Ishiura S

Subjects
Administration, Oral, Amyloid beta-Peptides biosynthesis, Animals, Antibodies metabolism, Brain metabolism, Capsicum genetics, Capsicum metabolism, Immunoglobulin G biosynthesis, Mice, Mice, Transgenic, Plant Leaves genetics, Plant Leaves metabolism, Vaccination, Alzheimer Disease prevention & control, Alzheimer Vaccines administration & dosage, Alzheimer Vaccines immunology, Amyloid beta-Peptides administration & dosage, Amyloid beta-Peptides immunology
Abstract

Alzheimer's disease (AD) is pathologically characterized by the presence of extracellular senile plaques and intracellular neurofibrillary tangles. Amyloid beta-peptide (Abeta) is the main component of senile plaques, and the pathological load of Abeta in the brain has been shown to be a marker of the severity of AD. Abeta is produced from the amyloid precursor protein by membrane proteases and is known to aggregate. Recently, immune-mediated cerebral clearance of Abeta has been studied extensively as potential therapeutic strategy. In previous studies that used a purified Abeta challenge in a mouse model of AD, symptomatic improvement was reported. However, a clinical Alzheimer's vaccine trial in the United States was stopped because of severe side effects. Immunization with the strong adjuvant used in these trials might have activated an inflammatory Th1 response. In this study, to establish a novel, safer, lower-cost therapy for AD, we tested an oral vaccination in a wild-type and a transgenic mouse model of AD administered via green pepper leaves expressing GFP-Abeta. Anti-Abeta antibodies were effectively induced after oral immunization. We examined the immunological effects in detail and identified no inflammatory reactions. Furthermore, we demonstrated a reduction of Abeta in the immunized AD-model mice. These results suggest this edible vehicle for Abeta vaccination has a potential clinical application in the treatment of AD., (Copyright 2010 Elsevier Inc. All rights reserved.)

Published
2010
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33. ADAM19 autolysis is activated by LPS and promotes non-classical secretion of cysteine-rich protein 2.

Author

Tanabe C, Hotoda N, Sasagawa N, Futai E, Komano H, and Ishiura S

Subjects
ADAM Proteins chemistry, ADAM Proteins genetics, Animals, COS Cells, Cell Line, Tumor, Chlorocebus aethiops, Enzyme Activation, Humans, LIM Domain Proteins, Protein Structure, Tertiary, Two-Hybrid System Techniques, ADAM Proteins biosynthesis, Adaptor Proteins, Signal Transducing metabolism, Lipopolysaccharides metabolism
Abstract

ADAM family proteins are type I transmembrane, zinc-dependent metalloproteases. This family has multiple conserved domains, including a signal peptide, a pro-domain, a metalloprotease domain, a disintegrin (DI) domain, a cysteine-rich (Cys) domain, an EGF-like domain, a transmembrane domain, and a cytoplasmic domain. The Cys and DI domains may play active roles in regulating proteolytic activity or substrate specificity. ADAM19 has an autolytic processing activity within its Cys domain, and the processing is necessary for its proteolytic activity. To identify a new physiological function of ADAM19, we screened for associating proteins by using the extracellular domain of ADAM19 in a yeast two-hybrid system. Cysteine-rich protein 2 (CRIP2) showed an association with ADAM19 through its DI and Cys domains. Sequence analysis revealed that CRIP2 is a secretable protein without a classical signal. CRIP2 secretion was increased by overexpression of ADAM19 and decreased by suppression of ADAM19 expression. Moreover, CRIP2 secretion increased in parallel with the autolytic processing of ADAM19 stimulated by lipopolysaccharide. These findings suggest that ADAM19 autolysis is activated by lipopolysaccharide and that ADAM19 promotes the secretion of CRIP2., ((c) 2010 Elsevier Inc. All rights reserved.)

Published
2010
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34. MBNL and CELF proteins regulate alternative splicing of the skeletal muscle chloride channel CLCN1.

Author

Kino Y, Washizu C, Oma Y, Onishi H, Nezu Y, Sasagawa N, Nukina N, and Ishiura S

Subjects
Animals, CELF Proteins, Chloride Channels metabolism, DNA Repeat Expansion, Exons, Humans, Mice, Muscle, Skeletal metabolism, RNA Splice Sites, RNA, Messenger metabolism, RNA-Binding Proteins antagonists & inhibitors, Alternative Splicing, Chloride Channels genetics, RNA-Binding Proteins metabolism
Abstract

The expression and function of the skeletal muscle chloride channel CLCN1/ClC-1 is regulated by alternative splicing. Inclusion of the CLCN1 exon 7A is aberrantly elevated in myotonic dystrophy (DM), a genetic disorder caused by the expansion of a CTG or CCTG repeat. Increased exon 7A inclusion leads to a reduction in CLCN1 function, which can be causative of myotonia. Two RNA-binding protein families--muscleblind-like (MBNL) and CUG-BP and ETR-3-like factor (CELF) proteins--are thought to mediate the splicing misregulation in DM. Here, we have identified multiple factors that regulate the alternative splicing of a mouse Clcn1 minigene. The inclusion of exon 7A was repressed by MBNL proteins while promoted by an expanded CUG repeat or CELF4, but not by CUG-BP. Mutation analyses suggested that exon 7A and its flanking region mediate the effect of MBNL1, whereas another distinct region in intron 6 mediates that of CELF4. An exonic splicing enhancer essential for the inclusion of exon 7A was identified at the 5' end of this exon, which might be inhibited by MBNL1. Collectively, these results provide a mechanistic model for the regulation of Clcn1 splicing, and reveal novel regulatory properties of MBNL and CELF proteins.

Published
2009
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35. Biochemical analysis of oligomerization of expanded polyalanine repeat proteins.

Author

Nojima J, Oma Y, Futai E, Sasagawa N, Kuroda R, Turk B, and Ishiura S

Subjects
Alanine genetics, Alanine metabolism, Analysis of Variance, Animals, Bacterial Proteins genetics, Bacterial Proteins metabolism, COS Cells, Chlorocebus aethiops, Cricetinae, Humans, Luminescent Proteins genetics, Luminescent Proteins metabolism, Peptides metabolism, Protein Conformation, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Transfection methods, Trypsin pharmacology, Two-Hybrid System Techniques, Peptides chemistry, Repetitive Sequences, Amino Acid genetics
Abstract

Many human proteins contain amino acid repeats that can form homopolymeric amino acid (HPAA) tracts. HPAA tract proteins that contain polyalanine sequences promote diseases, including oculopharyngeal muscular dystrophy. The pathological properties of these proteins develop when the repeats match or exceed approximately 20 residues. We analyzed the oligomerization of yellow fluorescent protein (YFP) and GST fusion proteins containing >20 alanine repeats by using sucrose density gradient centrifugation. YFP and GST fusion proteins having 23 polyalanine residues sedimented readily in sucrose density gradients, suggesting instability and oligomerization of proteins with an excess of 20 alanine repeats. Moreover, GST fusion proteins were resistant to trypsin digestion after oligomerization. Oligomerized artificial proteins with long polyalanine repeats may be suitable models for studying polyalanine-related diseases., (Copyright 2009 Wiley-Liss, Inc.)

Published
2009
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36. Polyalanine tracts directly induce the release of cytochrome c, independently of the mitochondrial permeability transition pore, leading to apoptosis.

Author

Toriumi K, Oma Y, Mimoto A, Futai E, Sasagawa N, Turk B, and Ishiura S

Subjects
Animals, COS Cells ultrastructure, Caspase 3 metabolism, Chlorocebus aethiops, Enzyme Activation, Humans, Mice, Mitochondria, Liver enzymology, Mitochondria, Liver metabolism, Mitochondrial Permeability Transition Pore, Apoptosis physiology, Cytochromes c metabolism, Mitochondria enzymology, Mitochondria metabolism, Mitochondrial Membrane Transport Proteins metabolism, Peptides metabolism, Peptides pharmacology
Abstract

In recent years, several novel types of disorder caused by the expansion of triplet repeats in specific genes have been characterized; in the "polyalanine diseases", these expanded repeats result in proteins with aberrantly elongated polyalanine tracts. In this study, we fused expanded polyalanine tracts to yellow fluorescent protein to examine their physical interaction with mitochondria. Tracts containing more than 23 alanine repeats were found to physically associate with mitochondria, strongly suggesting that an interaction between polyalanine tracts and mitochondria is a contributing factor in the pathology of polyalanine diseases. Furthermore, in in vitro experiments, polyalanine tracts induced release of cytochrome c from mitochondria and caspase-3 activation, independently of the mitochondrial permeability transition pore. These results suggest that oligomerized polyalanine tracts might induce the rupture of the mitochondrial membrane, the subsequent release of cytochrome c, and apoptosis. This novel mechanism for polyalanine tract cytotoxicity might be common to the pathogenesis of all polyalanine diseases. Further investigation of this mechanism might aid the development of therapies for these diseases.

Published
2009
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37. Identification of Caenorhabditis elegans K02H8.1 (CeMBL), a functional ortholog of mammalian MBNL proteins.

Author

Sasagawa N, Ohno E, Kino Y, Watanabe Y, and Ishiura S

Subjects
Animals, Caenorhabditis elegans, Caenorhabditis elegans Proteins metabolism, Conserved Sequence, Drosophila, Drosophila Proteins, Gene Expression, Green Fluorescent Proteins metabolism, Male, Muscles metabolism, Mutation, Neurons metabolism, Nuclear Proteins, Pharynx growth & development, Pharynx metabolism, Promoter Regions, Genetic, Protein Isoforms, RNA metabolism, RNA-Binding Proteins metabolism, Seminal Vesicles growth & development, Seminal Vesicles metabolism, Two-Hybrid System Techniques, Zinc Fingers, Caenorhabditis elegans Proteins genetics, RNA-Binding Proteins genetics
Abstract

The genome of the nematode Caenorhabditis elegans possesses an orthologous sequence to the Drosophila muscleblind (mbl) and mammalian muscleblind-like genes (MBNLs). This ortholog, K02H8.1, which has a high degree of homology (about 50%) to human MBNLs, encodes two zinc finger domains, as does the sequence of the Drosophila mbl gene. This distinguishes it from human MBNLs, which encode four zinc finger domains. In this study, we cloned six major isoforms of K02H8.1 using cDNA generated from C. elegans total RNA. All six of the cloned isoforms had an SL1 leader sequence at the 5'-position. Interestingly, one of the isoforms lacked a zinc finger domain-encoding sequence. To understand better the function of K02H8.1, we performed yeast three-hybrid experiments to characterize the binding of K02H8.1 to bait RNAs. K02H8.1 exhibited strong binding affinity for CUG and CCUG repeats, and the binding affinity was very similar to that of MBNLs. In addition, promoter analysis was performed using promoter-green fluorescent protein (GFP) fusion constructs. The expression of GFP driven by the K02H8.1 promoter was absent in muscle; however, significant GFP expression was detected in the neurons around the pharynx.

Published
2009
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38. 1,3-Capryloyl-2-arachidonoyl glycerol activates alpha-secretase activity and suppresses Abeta40 secretion in A172 cells.

Author

Tanabe C, Ebina M, Asai M, Futai E, Sasagawa N, Katano K, Fukami H, and Ishiura S

Subjects
Alzheimer Disease drug therapy, Alzheimer Disease enzymology, Amyloid Precursor Protein Secretases metabolism, Amyloid beta-Peptides metabolism, Brain enzymology, Brain physiopathology, Cell Line, Cell Line, Tumor, Down-Regulation drug effects, Down-Regulation physiology, Enzyme Activation drug effects, Enzyme Activation physiology, Fatty Acids, Unsaturated metabolism, Humans, Neurons enzymology, Neurons metabolism, Peptide Fragments metabolism, Amyloid Precursor Protein Secretases drug effects, Amyloid beta-Peptides antagonists & inhibitors, Brain drug effects, Caprylates pharmacology, Fatty Acids, Unsaturated pharmacology, Neurons drug effects, Peptide Fragments antagonists & inhibitors, Triglycerides pharmacology
Abstract

Alzheimer's disease (AD) is characterized by the deposition of amyloid beta-peptide (Abeta), derived from amyloid precursor protein (APP). Membrane states, such as lipid components or membrane fluidity, are important for enzymes related to APP processing in meeting their substrates efficiently. We analyzed the effects of triglycerides combined with polyunsaturated fatty acids (PUFAs) and/or caprylic acids on APP proteolysis. Our results showed that 1,3-capryloyl-2-arachidonoyl glycerol (8A8) moderately increased alpha-secretase activity (18%) in A172 cells. beta-Secretase activity was not statistically significantly changed in HEK293 cells stably expressing BACE1. However, Abeta40 secretion decreased by 22%. Thus, we conclude that 8A8 is a useful lipid compound for activating alpha-secretase activity and suppressing Abeta40 secretion.

Published
2009
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39. Inhibition by KMI-574 leads to dislocalization of BACE1 from lipid rafts.

Author

Ebina M, Futai E, Tanabe C, Sasagawa N, Kiso Y, and Ishiura S

Subjects
Amyloid Precursor Protein Secretases chemistry, Amyloid Precursor Protein Secretases drug effects, Aspartic Acid Endopeptidases chemistry, Aspartic Acid Endopeptidases drug effects, Blotting, Western, Cell Line, Enzyme Activation physiology, Humans, Protein Conformation drug effects, Protein Transport drug effects, Transfection, Amyloid Precursor Protein Secretases metabolism, Aspartic Acid Endopeptidases metabolism, Enzyme Inhibitors pharmacology, Membrane Microdomains enzymology, Protein Transport physiology
Abstract

BACE1 initiates processing of the amyloid precursor protein (APP) in the production of amyloid beta (Abeta) peptide. After beta-cleavage by BACE1, the C-terminal stub of the APP fragment is further processed by the gamma-secretase complex to produce Abeta. Because APP, Abeta, the gamma-secretase complex, and BACE1 are found in lipid raft membranes, Abeta production is widely accepted to occur in lipid rafts. However, whether BACE1 is activated within the rafts is unclear. To analyze the relationship between the activity and the localization of BACE1, we used a new BACE1 inhibitor, KMI-574, and separated raft membranes on sucrose density gradients. In the presence of KMI-574, the localization of BACE1 shifted from the rafts to nonraft membranes in HEK293 cells. We also analyzed the proteolytically inactive mutants, D93A, D289A, and D93A/D289A, of BACE1. These mutants also moved from rafts to nonrafts, and the D93A/D289A double-mutant localized exclusively to nonraft membranes. The mutants were defective in maturation by glynosylation and formed hyperoligomers, suggesting that the BACE1 oligomers could not exit from the ER and be transported to the Golgi apparatus. Our findings suggest that the activated conformation of BACE1 is important for protein transport and localization to lipid rafts., (2008 Wiley-Liss, Inc.)

Published
2009
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40. Dysbindin-1, a schizophrenia-related protein, functionally interacts with the DNA- dependent protein kinase complex in an isoform-dependent manner.

Author

Oyama S, Yamakawa H, Sasagawa N, Hosoi Y, Futai E, and Ishiura S

Subjects
Carrier Proteins genetics, Carrier Proteins physiology, Cell Nucleus, Central Nervous System, Dysbindin, Dystrophin-Associated Proteins, Humans, Phosphorylation, Polymorphism, Single Nucleotide, Protein Isoforms metabolism, Carrier Proteins metabolism, DNA-Activated Protein Kinase metabolism, Schizophrenia etiology
Abstract

DTNBP1 has been recognized as a schizophrenia susceptible gene, and its protein product, dysbindin-1, is down-regulated in the brains of schizophrenic patients. However, little is known about the physiological role of dysbindin-1 in the central nervous system. We hypothesized that disruption of dysbindin-1 with unidentified proteins could contribute to pathogenesis and the symptoms of schizophrenia. GST pull-down from human neuroblastoma lysates showed an association of dysbindin-1 with the DNA-dependent protein kinase (DNA-PK) complex. The DNA-PK complex interacts only with splice isoforms A and B, but not with C. We found that isoforms A and B localized in nucleus, where the kinase complex exist, whereas the isoform C was found exclusively in cytosol. Furthermore, results of phosphorylation assay suggest that the DNA-PK complex phosphorylated dysbindin-1 isoforms A and B in cells. These observations suggest that DNA-PK regulates the dysbindin-1 isoforms A and B by phosphorylation in nucleus. Isoform C does not contain exons from 1 to 6. Since schizophrenia-related single nucleotide polymorphisms (SNPs) occur in these introns between exon 1 and exon 6, we suggest that these SNPs might affect splicing of DTNBP1, which leads to impairment of the functional interaction between dysbindin-1 and DNA-PK in schizophrenic patients.

Published
2009
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41. MBNL1 associates with YB-1 in cytoplasmic stress granules.

Author

Onishi H, Kino Y, Morita T, Futai E, Sasagawa N, and Ishiura S

Subjects
DEAD-box RNA Helicases genetics, DNA, Complementary genetics, DNA-Binding Proteins genetics, Gene Amplification, Humans, Nuclear Proteins genetics, Poly(A)-Binding Proteins, Polyribosomes metabolism, RNA-Binding Proteins metabolism, Recombinant Proteins metabolism, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, T-Cell Intracellular Antigen-1, Y-Box-Binding Protein 1, Cytoplasmic Granules physiology, DNA-Binding Proteins metabolism, Muscle, Skeletal physiology, Nuclear Proteins metabolism, RNA-Binding Proteins genetics
Abstract

The muscleblind-like (MBNL) protein family is thought to be involved in the molecular mechanism of myotonic dystrophy (DM). Although it has been shown to have splicing activity, a broader function in cellular RNA metabolism has been implicated. In this study, we attempted to find the binding proteins of MBNL1 in order to elucidate its physiological function. First, we performed a GST pull-down assay using GST-MBNL1-6xHis as bait. Several proteins were identified, including YB-1, a multifunctional DNA/RNA-binding protein, and DDX1, a DEAD box RNA helicase. MBNL1 formed an RNP complex with YB-1 and DDX1 in binding assays. YB-1 also showed a weak but significant effect on alpha-actinin splice site selection. Interestingly, in response to stress, MBNL1 moved to cytoplasmic stress granules, where it colocalized with YB-1, which was previously reported to be a component of stress granules. We found that DDX1 also colocalized with MBNL1 at stress granules. These results provide new insight into the dynamics of MBNL1 in response to stress, and they suggest a role for MBNL1 in mRNA metabolism in the cytoplasm., (2008 Wiley-Liss, Inc.)

Published
2008
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42. Expression of polyalanine stretches induces mitochondrial dysfunction.

Author

Toriumi K, Oma Y, Kino Y, Futai E, Sasagawa N, and Ishiura S

Subjects
Animals, Bacterial Proteins, COS Cells ultrastructure, Carrier Proteins, Chlorocebus aethiops, Cytochromes c metabolism, Flow Cytometry methods, Glutathione Transferase metabolism, Luminescent Proteins, Mass Spectrometry methods, Membrane Potential, Mitochondrial physiology, Mitochondria ultrastructure, Peptides genetics, Subcellular Fractions metabolism, Succinate Dehydrogenase metabolism, Transfection, Trinucleotide Repeat Expansion genetics, Mitochondria metabolism, Peptides metabolism, Trinucleotide Repeat Expansion physiology
Abstract

In recent years, several novel types of disorders have been characterized, including what have been termed polyalanine diseases, in which patients have expanded triplet repeats in specific genes, resulting in the translation of aberrantly elongated polyalanine stretches. In this study, we showed that yellow fluorescent protein (YFP)-fused elongated polyalanine stretches localized exclusively to the cytoplasm and formed aggregates. Additionally, the polyalanine stretches themselves were toxic. We sought to identify proteins that bound directly to the polyalanine stretches, as factors that might be involved in triggering cell death. Many mitochondrial proteins were identified as polyalanine-binding proteins. We showed that one of the identified proteins, succinate dehydrogenase subunit A, was decreased in the mitochondria of cells expressing polyalanine stretches; as a result, succinate oxidative activity was decreased. Furthermore, the polyalanine stretches also associated directly with mitochondria. This suggests that polya-lanine stretches might directly induce cell death. Additionally, the mitochondrial membrane potential was reduced in cells expressing polyalanine stretches. We propose a novel mechanism by which polyalanine stretches may cause cytotoxicity through mitochondrial dysfunction. This may be a common mechanism underlying the pathogenesis of all polyalanine diseases.

Published
2008
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43. Csk-homologous kinase interacts with SHPS-1 and enhances neurite outgrowth of PC12 cells.

Author

Mitsuhashi H, Futai E, Sasagawa N, Hayashi Y, Nishino I, and Ishiura S

Subjects
Animals, Bacterial Proteins biosynthesis, Cells, Cultured, Cerebral Cortex cytology, Chlorocebus aethiops, Cloning, Molecular, Embryo, Mammalian, Gene Expression physiology, Glutathione Transferase physiology, Humans, Luminescent Proteins biosynthesis, Mutation physiology, Neurons cytology, Phosphorylation, Proto-Oncogene Proteins pp60(c-src) genetics, Rats, Transfection, Two-Hybrid System Techniques, Tyrosine metabolism, src Homology Domains physiology, Neurites physiology, PC12 Cells cytology, Proto-Oncogene Proteins pp60(c-src) metabolism, Receptors, Immunologic metabolism
Abstract

SHPS-1 is an immunoglobulin superfamily protein with four immunoreceptor tyrosine-based inhibitory motifs (ITIMs) in its cytoplasmic region. Various neurotrophic factors induce the tyrosine phosphorylation of SHPS-1 and the association of SHPS-1 with the protein tyrosine phosphatase SHP-2. Using a yeast two-hybrid screen, we identified a protein tyrosine kinase, Csk-homologous kinase (CHK), as an SHPS-1-interacting protein. Immunoprecipitation and pull-down assays using glutathione S-transferase (GST) fusion proteins containing the Src homology 2 (SH2) domain of CHK revealed that CHK associates with tyrosine-phosphorylated SHPS-1 via its SH2 domain. HIS3 assay in a yeast two-hybrid system using the tyrosine-to-phenylalanine mutants of SHPS-1 indicated that the first and second ITIMs of SHPS-1 are required to bind CHK. Over-expression of wild-type CHK, but not a kinase-inactive CHK mutant, enhanced the phosphorylation of SHPS-1 and its subsequent association with SHP-2. CHK phosphorylated each of four tyrosines in the cytoplasmic region of SHPS-1 in vitro. Co-expression of SHPS-1 and CHK enhanced neurite outgrowth in PC12 cells. Thus, CHK phosphorylates and associates with SHPS-1 and is involved in neural differentiation via SHP-2 activation.

Published
2008
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44. Quantitative analysis of CUG-BP1 binding to RNA repeats.

Author

Mori D, Sasagawa N, Kino Y, and Ishiura S

Subjects
CELF1 Protein, DNA Mutational Analysis, Humans, Kinetics, Nucleotides metabolism, Protein Binding, RNA-Binding Proteins isolation & purification, Surface Plasmon Resonance, Two-Hybrid System Techniques, RNA metabolism, RNA-Binding Proteins metabolism, Repetitive Sequences, Nucleic Acid genetics
Abstract

CUG-binding protein 1 (CUG-BP1) is a member of the CUG-BP1 and ETR-3-like factors (CELF) family of RNA-binding proteins, and is involved in myotonic dystrophy type 1 (DM1). Several mRNA targets of CUG-BP1 have been identified, including the insulin receptor, muscle chloride channel, and cardiac troponin T. On the other hand, CUG-BP1 has only a weak affinity for CUG repeats. We conducted quantitative-binding assays to assess CUG-BP1 affinities for several repeat RNAs by surface plasmon resonance (SPR). Although we detected interactions between CUG-BP1 and CUG repeats, other UG-rich sequences actually showed stronger interactions. Binding constants of CUG-BP1 for RNAs indicated that the affinity for UG repeats was far stronger than for CUG repeats. We also found that N-terminal deletion mutant of CUG-BP1 has UG repeat-binding activity in a yeast three-hybrid system, although C-terminal deletion mutant does not. Our data indicates that CUG-BP1 specifically recognized UG repeats, probably through cooperative binding of RNA recognition motifs at both ends of the protein. This is the first report of a binding constant for CUG-BP1 calculated in vitro.

Published
2008
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45. Methylmercury activates ASK1/JNK signaling pathways, leading to apoptosis due to both mitochondria- and endoplasmic reticulum (ER)-generated processes in myogenic cell lines.

Author

Usuki F, Fujita E, and Sasagawa N

Subjects
Animals, Antioxidants pharmacology, Caspases metabolism, Cell Line, Transformed, Chromans pharmacology, Dose-Response Relationship, Drug, Enzyme Activation drug effects, Mice, Mutation physiology, Myotonin-Protein Kinase, Protein Serine-Threonine Kinases genetics, Reactive Oxygen Species metabolism, Time Factors, Transfection methods, Trinucleotide Repeat Expansion genetics, Up-Regulation drug effects, Apoptosis drug effects, Endoplasmic Reticulum drug effects, MAP Kinase Kinase Kinase 5 physiology, Methylmercury Compounds toxicity, Mitochondria drug effects, Myoblasts drug effects, Myoblasts physiology, Myoblasts ultrastructure, Signal Transduction drug effects
Abstract

Cellular stress responses following exposure to methylmercury (MeHg) were investigated using myogenic cell lines that showed different susceptibilities to MeHg. The susceptible cell line showed apoptosis within 24h after exposure to low levels of MeHg. The activation of caspase 12, 9, and 3 was detected in the apoptotic cells at 14-16 h after MeHg exposure, suggesting that MeHg causes apoptosis via both mitochondria- and endoplasmic reticulum (ER)-generated processes. An early increase in the level of intracellular reactive oxygen species (ROS) was quantitatively recognized since 2-3h after exposure to MeHg in both MeHg-susceptible and non-susceptible cell lines; however, the increase was lower in the latter cell line. The phosphorylation of apoptosis signal-regulating kinase 1 (ASK1) was also recognized in both cell lines, with the increase in intracellular ROS. However, the activation of stress-activated protein kinase/c-Jun N-terminal kinase (SAPK/JNK) pathways was observed only in the MeHg-susceptible cell line. In contrast, the non-susceptible cell line exhibited activation of the cell survival ERK pathway. Up-regulation of metallothioneine I and Hic-5 mRNAs encoding proteins induced by oxidative stress was recognized during the early stage of MeHg cytotoxicity in the MeHg-susceptible cell line. Quantitative real-time PCR and western blot analyses confirmed that ER stress is a late event during MeHg cytotoxicity. Coaddition of the antioxidant Trolox dramatically suppressed the increase in the level of ROS, activation of caspases and, finally, apoptosis. However, later treatment with Trolox attenuated its protective effect against MeHg cytotoxicity. The results indicate that failure to protect cells against the early oxidative stress triggers ER stress and apoptosis processes. Combined treatment with protective factors against oxidative and ER stresses is necessary, especially in the later stages of MeHg cytotoxicity.

Published
2008
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46. Identification of an estrogenic hormone receptor in Caenorhabditis elegans.

Author

Mimoto A, Fujii M, Usami M, Shimamura M, Hirabayashi N, Kaneko T, Sasagawa N, and Ishiura S

Subjects
Animals, Caenorhabditis elegans, Caenorhabditis elegans Proteins metabolism, Estrogens metabolism, Estrogens, Conjugated (USP) metabolism, Receptors, Cytoplasmic and Nuclear metabolism, Receptors, Estrogen metabolism
Abstract

Changes in both behavior and gene expression occur in Caenorhabditis elegans following exposure to sex hormones such as estrogen and progesterone, and to bisphenol A (BPA), an estrogenic endocrine-disrupting compound. However, only one steroid hormone receptor has been identified. Of the 284 known nuclear hormone receptors (NHRs) in C. elegans, we selected nhr-14, nhr-69, and nhr-121 for analysis as potential estrogenic hormone receptors, because they share sequence similarity with the human estrogen receptor. First, the genes were cloned and expressed in Escherichia coli, and then the affinity of each protein for estrogen was determined using a surface plasmon resonance (SPR) biosensor. All three NHRs bound estrogen in a dose-dependent fashion. To evaluate the specificity of the binding, we performed a solution competition assay using an SPR biosensor. According to our results, only NHR-14 was able to interact with estrogen. Therefore, we next examined whether nhr-14 regulates estrogen signaling in vivo. To investigate whether these interactions actually control the response of C. elegans to hormones, we investigated the expression of vitellogenin, an estrogen responsive gene, in an nhr-14 mutant. Semi-quantitative RT-PCR showed that vitellogenin expression was significantly reduced in the mutant. This suggests that NHR-14 is a C. elegans estrogenic hormone receptor and that it controls gene expression in response to estrogen.

Published
2007
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47. Endoplasmic reticulum stress caused by aggregate-prone proteins containing homopolymeric amino acids.

Author

Uchio N, Oma Y, Toriumi K, Sasagawa N, Tanida I, Fujita E, Kouroku Y, Kuroda R, Momoi T, and Ishiura S

Subjects
Amino Acids analysis, Animals, Bacterial Proteins metabolism, Cells, Cultured, Hydrophobic and Hydrophilic Interactions, Leucine metabolism, Luminescent Proteins metabolism, Mice, Microscopy, Fluorescence, Peptides chemistry, Peptides metabolism, Proteasome Endopeptidase Complex metabolism, Transfection, Ubiquitin metabolism, Amino Acids chemistry, Endoplasmic Reticulum physiology
Abstract

Many human proteins have homopolymeric amino acid (HPAA) tracts, but their physiological functions or cellular effects are not well understood. Previously, we expressed 20 HPAAs in mammalian cells and showed characteristic intracellular localization, in that hydrophobic HPAAs aggregated strongly and caused high cytotoxicity in proportion to their hydrophobicity. In the present study, we investigated the cytotoxicity of these aggregate-prone hydrophobic HPAAs, assuming that the ubiquitin proteasome system is impaired in the same manner as other well-known aggregate-prone polyglutamine-containing proteins. Some highly hydrophobic HPAAs caused a deficiency in the ubiquitin proteasome system and excess endoplasmic reticulum stress, leading to apoptosis. These results indicate that the property of causing excess endoplasmic reticulum stress by proteasome impairment may contribute to the strong cytotoxicity of highly hydrophobic HPAAs, and proteasome impairment and the resulting excess endoplasmic reticulum stress is not a common cytotoxic effect of aggregate-prone proteins such as polyglutamine.

Published
2007
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48. Interactions between homopolymeric amino acids (HPAAs).

Author

Oma Y, Kino Y, Toriumi K, Sasagawa N, and Ishiura S

Subjects
Animals, COS Cells, Chlorocebus aethiops, Hydrophobic and Hydrophilic Interactions, Proteins analysis, Proteins chemistry, Two-Hybrid System Techniques, Peptides chemistry, Repetitive Sequences, Amino Acid
Abstract

Many human proteins contain consecutive amino acid repeats, known as homopolymeric amino acid (HPAA) tracts. Some inherited diseases are caused by proteins in which HPAAs are expanded to an excessive length. To this day, nine polyglutamine-related diseases and nine polyalanine-related diseases have been reported, including Huntington's disease and oculopharyngeal muscular dystrophy. In this study, potential HPAA-HPAA interactions were examined by yeast two-hybrid assays using HPAAs of approximately 30 residues in length. The results indicate that hydrophobic HPAAs interact with themselves and with other hydrophobic HPAAs. Previously, we reported that hydrophobic HPAAs formed large aggregates in COS-7 cells. Here, those HPAAs were shown to have significant interactions with each other, suggesting that hydrophobicity plays an important role in aggregation. Among the observed HPAA-HPAA interactions, the Ala28-Ala29 interaction was notable because polyalanine tracts of these lengths have been established to be pathogenic in several polyalanine-related diseases. By testing several constructs of different lengths, we clarified that polyalanine self-interacts at longer lengths (>23 residues) but not at shorter lengths (six to approximately 23 residues) in a yeast two-hybrid assay and a GST pulldown assay. This self-interaction was found to be SDS sensitive in SDS-PAGE and native-PAGE assays. Moreover, the intracellular localization of these long polyalanine tracts was also observed to be disturbed. Our results suggest that long tracts of polyalanine acquire SDS-sensitive self-association properties, which may be a prerequisite event for their abnormal folding. The misfolding of these tracts is thought to be a common molecular aspect underlying the pathogenesis of polyalanine-related diseases.

Published
2007
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49. Expression of MBNL and CELF mRNA transcripts in muscles with myotonic dystrophy.

Author

Nezu Y, Kino Y, Sasagawa N, Nishino I, and Ishiura S

Subjects
Adolescent, Adult, Aged, CCAAT-Enhancer-Binding Protein-delta genetics, Female, Humans, Male, Middle Aged, Myotonic Dystrophy genetics, Myotonic Dystrophy pathology, RNA, Messenger metabolism, RNA-Binding Proteins genetics, Reverse Transcriptase Polymerase Chain Reaction methods, CCAAT-Enhancer-Binding Protein-delta metabolism, Gene Expression physiology, Muscle, Skeletal metabolism, Myotonic Dystrophy metabolism, RNA-Binding Proteins metabolism
Abstract

Myotonic dystrophy type 1 (DM1) is an autosomal dominant disorder that causes muscle wasting, myotonia, cardiac conduction abnormalities, and other multi-systemic symptoms. Current evidence supports a pathogenic mechanism involving aberrantly expanded CTG repeats in the 3'-untranslated region of the DM protein kinase (DMPK) gene. The repeats are thought to recruit various RNA-binding proteins such as muscleblind-like (MBNL) proteins into foci in the nuclei of DM cells, resulting in loss of function. However, aberrant regulation of transcription or subsequent RNA processing of MBNL-family mRNAs might also be part of the pathogenic mechanism of DM. We used real-time RT-PCR analysis to examine the possibility that MBNL mRNA expression is altered in DM1 patients. We also examined mRNA expression for members of the CUG-BP and ETR-3-like factor (CELF) family of RNA-binding proteins given that CELF proteins regulate alternative splicing and are also implicated in DM. We found that DM1 muscles displayed aberrant regulation of alternative splicing as reported previously; however, the levels of MBNL and CELF mRNA expression did not show any significant changes. Our results suggest that the expression and stability of the mRNA for these RNA-binding proteins are unaffected in DM1.

Published
2007
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50. Neuroligins 3 and 4X interact with syntrophin-gamma2, and the interactions are affected by autism-related mutations.

Author

Yamakawa H, Oyama S, Mitsuhashi H, Sasagawa N, Uchino S, Kohsaka S, and Ishiura S

Subjects
Autistic Disorder pathology, Carrier Proteins genetics, Cell Adhesion Molecules, Neuronal, Cloning, Molecular, Humans, Membrane Proteins genetics, Muscle Proteins genetics, Nerve Tissue Proteins genetics, Recombinant Fusion Proteins metabolism, Recombinant Proteins metabolism, Restriction Mapping, Saccharomyces cerevisiae genetics, Synapses pathology, gamma-Aminobutyric Acid physiology, Autistic Disorder genetics, Carrier Proteins metabolism, Membrane Proteins metabolism, Muscle Proteins metabolism, Mutation, Nerve Tissue Proteins metabolism
Abstract

Recently, neuroligins (NLs)3 and 4X have received much attention as autism-related genes. Here, we identified syntrophin-gamma2 (SNTG2) as a de novo binding partner of NL3. SNTG2 also bound to NL4X and NL4Y. Interestingly, the binding was influenced by autism-related mutations, implying that the impaired interaction between NLs and SNTG2 contributes to the etiology of autism.

Published
2007
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