Your search keyword '"Y. Futsuhara"' showing total 13 results

1. Diallel analysis of callus growth and plant regeneration in rice

Author

T. Abe and Y. Futsuhara

Published

2008

2. Slender ricemutant is caused by null mutation of theSLRgene, an ortholog of the height-regulating geneGAI/RGA/RHT/D8

Author

A. Ikeda, M. Ueguchi-Tanaka, Y. Sonoda, H. Kitano, Y. Futsuhara, M. Matsuoka, and J. Yamaguchi

Published

2008

3. Abstracts of Posters Presentations

Author

T. E. Bureau, G. S. Khush, S. R. Wessler, A. S. Reddy, F. Cordesse, M. Delseny, A. Kanno, K. Hattori, A. Hirai, Y. Sano, R. Sano, H. -Y. Hirano, T. Ishii, T. Terachi, N. Mori, K. Tsunewaki, J. P. Gustafson, C. L. Mclntyre, J. E. Dillé, Jinshui Yang, Koulin Ge, Yunzhu Wang, C. C. Tan, Shanbao Chen, Xiaolan Duan, Changsheng Yan, Guandang Xing, Yan Zhang, B. Wang, H. G. Zheng, Q. F. Xu, J. Z. Wang, D. D. Li, S. T. Li, Z. T. Zhang, O. Panaud, G. Magpantay, E. Galinato, D. Mahapatra, L. A. Sitch, S. Yoshimura, A. Yoshimura, N. Iwata, A. Saito, N. Kishimoto, M. Kawase, M. Nakagahra, M. Yano, N. Mitsukawa, K. Tanaka, E. C. Cocking, S. L. Kothari, H. Zhang, P. T. Lynch, P. S. Eyles, E. L. Rech, M. R. Davey, I. H. Slamet, R. P. Finch, K. -I. Mori, T. Kinoshita, A. Tanaka, S. Tano, A. B. Mendoza, Y. Futsuhara, Y. Takeoka, Wang Zixuan, E. Guiderdoni, P. B. Kavi Kishor, G. M. Reddy, N. R. Yadav, D. R. Sharma, J. B. Chowdhury, Jiadao Wu, Zhongxiang Huang, Zuling Liu, Leya Zheng, Jianbo Yan, Yan Chen, K. Fukui, K. Iijima, H. Fukuoka, Y. Kageyama, K. Yamamoto, G. Takeda, I. Imuta, F. Kikuchi, I. Watanabe, M. Yusa, O. Kamijima, H. Kitano, Y. Nagato, S. Kikuchi, H. Satoh, I. Takamure, S. Oba, M. Ichii, Shui Shan Li, H. Hasegawa, A. Matsuzaki, T. Takano, T. Kato, D. A. Vaughan, K. K. Jena, D. S. Multani, A. Ghesquiere, P. Barbier, A. Ishihama, A. A. Flores-Nimedez, K. Dörffling, B. S. Vergara, T. Nagamine, K. Watanabe, T. Nishimura, T. Ogawa, R. E. Tabien, T. Yamamoto, G. A. Busto, R. Ikeda, C. Hamamatsu, Y. -I. Sato, H. Morishima, J. Abadassi, J. C. Glaszmann, J. L. Notteghem, B. Courtois, O. Mohamad, M. Z. Abdullah, O. Othman, K. Hadzim, J. Mahmud, O. Ramli, J. L. Minocha, J. S. Sidhu, R. K. Gupta, H. Sano, S. Youssefian, I. Kamada, M. Itoh, M. T. Mei, Q. F. Zuo, Y. G. Lu, H. Deng, T. C. Yang, T. Tanisaka, H. Yamagata, B. Mishra, J. P. Tilquin, J. P. Chapeaux, J. F. Detry, Yi-Shin Chen, Chia-Yi Aes, Bui Chi Buu, Thai Thi Hanh, Minghong Gu, Aiqing You, Xuebiao Pan, Zu-bai Qi, Ye-Tong Cai, Bao-jian Li, T. Nomura, K. Yonezawa, T. Sato, N. Watanabe, R. B. Austin, C. L. Morgan, Y. Okumoto, Y. Shimamoto, Shih-Cheng Lin, K. Hinata, M. Oka, M. P. Pandey, D. V. Seshu, M. Akbar, Moo Young Eun, Yong Gu Cho, Yong Kwon Kim, Tae Young Chung, Gun-Sik Chung, Sae-Jun Yang, Byeong-Geun Oh, G. L. Shrestha, S. Mallik, A. M. Aguilar, G. Kochert, and I. Nakamura

Published

2008

4. Characterizing a slender mutant with constitutive gibberellin-response in rice

Author

A. Ikeda, H. Kitano, Y. Sonoda, Y. Futsuhara, and J. Yamaguchi

Published

2008

5. Regeneration of Rice Plants from Suspension Cultures

Author

Y. Futsuhara and T. Abe

Subjects

Somatic embryogenesis, Callus, Regeneration (biology), fungi, Botany, Stamen, food and beverages, Organogenesis, Cultivar, Protoplast, Biology, Suspension culture

Abstract

Suspension culture of single cells and plant regeneration are of great importance to establish the new crop improvement system through cellular and chromosomal manipulation as well as clonal propagation. Mutant cell lines or variants have been obtained through cell selection (Wakasa and Widholm 1987). On the other hand, in general it is difficult to recover plants from suspension cultures. Cell suspension cultures of rice have been examined from the physiological and cytological view points (Maeda 1969, 1973; Ohira et al. 1973; Igaue et al. 1980). Plant regeneration from suspension cultures of rice has been reported by Ye (1984) and Abe and Futsuhara (1986). We also reported that plantlets regenerated at high rates from rice root callus via somatic embryogenesis in some indica cultivars (Abe and Futsuhara 1986). Plant regeneration via somatic embryogenesis from suspension cultures of cereals is preferable to organogenesis. Recently, plant regeneration from rice protoplast isolated from suspension cultures which originated from seeds and anthers has also been demonstrated (Fujimura et al. 1985; Toriyama et al. 1986; Kyozuka et al. 1987), in which plant regeneration was attained at a high rate through somatic embryogenesis (Kyozuka et al. 1987).

Published

1991

6. Selection of higher regenerative callus and change in isozyme pattern in rice (Oryza sativa L.)

Author

Y Futsuhara and T. Abe

Subjects

chemistry.chemical_classification, Oryza sativa, biology, fungi, food and beverages, General Medicine, Meristem, Murashige and Skoog medium, chemistry, Auxin, Callus, Shoot, Botany, Genetics, biology.protein, Primordium, Agronomy and Crop Science, Biotechnology, Peroxidase

Abstract

Calli were initiated from seedling roots in rice (Oryza sativa L. var. Tadukan) and subcultured at 45-day intervals on MS medium supplemented with 2 mg/l 2,4-D. Sectors of callus which differentiated shoot meristems (green spots) under the same 2,4-D concentration were selected from the calli subcultured 90 days after initiation. The selection was continued for about 2 years. Responses to 2,4-D between original and selected lines differed considerably, although differentiation was not generally seen in rice callus in the presence of 2 mg/l 2,4-D. After 180 days, calli of the selected line differentiated into numerous shoot-bud primordia and grew out new callus tissues under 2 mg/l 2,4-D concentration; the frequency of the differentiation exceeded 90%. On the other hand, no calli of non-selected line differentiated into shootbuds under 2 mg/l 2,4-D, and the frequency of the shootbud was only about 50% under lower 2,4-D concentration (0.1 mg/l). The pattern and activity of peroxidase isozyme varied markedly between calli of the selected and non-selected lines. First, two strong peroxidase bands which show fast mobility and one intermediate peroxidase band with slow mobility were detected only in the calli of selected line. Secondly, changes in band pattern of proteins separated by SDS-PAGE were observed. In the calli of selected line, there was a loss of the polypeptide bands with molecular weight of 24 and 42 K in the selected calli, but they were clearly present in the unselected line. The appearance of new peroxidase isozyme bands and loss of polypeptide bands, change in response to auxin and increased ability for shoot bud differentiation are closely correlated to each other.

Published

1989

7. Effects of gamma-ray irradiation on the growth of calli in Nicotiana species

Author

L.P. Balito, K. Hattori, and Y. Futsuhara

Subjects

Tissue culture, biology, Callus, fungi, Botany, Growth rate, Radiosensitivity, Ploidy, biology.organism_classification, Incubation, Solanaceae, Nicotiana

Abstract

Haploid and diploid calli of Nicotiana glauca (n=12) and N. langsdorffii (n=9) together with dlploid calli of N. tabacum (n=24) cv. Bright Yellow which were taken as control were ex-posed to various doses of 60co gamma rays at 7 days and 10 days after incubation. Calli were subsequently weighed for a period of 12-14 days after radiation (19-24 clays after incubation) and the effect of irradiation on the growth was studied. A sigmoid curve was observed for the growth rate as well as for the growth pattern. The radiosensitivlty were estimate.d on the basis of the following different two criteria: 1) the difference in the diploid callus volumes at 12 or 14 days after irradiatlon and at the time of radiation, 2) the growth rate of diploid and haploid calli during these period. In 2 species except in N. langsdorffii, calli irradiated ten days after incubation (at the beginning of the actively growing stage) were more sensitive to gamma irradiation than calli lrradiated seven days after incubation (at a relatively slow growing stage). Each species had its own distinctive color before irradiation; golden yellow, green and yellow green for N. glauca, N. langsdorffii and N. tabacum, respectively. The color of some of the calli tended to darken with increasing" irradiation doses. When the rate of increase of the irradiated calli to that of the unlrradiated ones was used as an indicator of radiosensitivity, there was a significant difference in the radiosen-sitivity of the calli among the species: N. tabacum was more sensitive followed by N. glauca and N. langsdorffii, which was the least sensitive. On the other hand, when the curve of the increase of the growth rate was used as the criterion of radiosensitivity, N. langsdorffii appeared to be more sensitive than N. tabacum and N. glauca. Haploid calli were more radiosensitive than diploid ones in N. glauca, but no significant difference was observed between them in N. lanegsdorffii.

Published

1989

8. Functional characterization of betaine/proline transporters in betaine-accumulating mangrove.

Author

Waditee R, Hibino T, Tanaka Y, Nakamura T, Incharoensakdi A, Hayakawa S, Suzuki S, Futsuhara Y, Kawamitsu Y, Takabe T, and Takabe T

Subjects

Amino Acid Sequence, Amino Acid Transport Systems, Neutral chemistry, Amino Acid Transport Systems, Neutral genetics, Carrier Proteins chemistry, Carrier Proteins genetics, Cloning, Molecular, GABA Plasma Membrane Transport Proteins, Kinetics, Molecular Sequence Data, Proline metabolism, Sequence Homology, Amino Acid, Amino Acid Transport Systems, Neutral physiology, Betaine metabolism, Carrier Proteins physiology, Trees metabolism

Abstract

Betaine is an important osmoprotectant in many plants, but its transport activity has only been demonstrated using a proline transporter from tomato, a betaine-nonaccumulating plant. In this study, two full-length and one partial transporter genes were isolated from betaine-accumulating mangrove Avicennia marina. Their homologies to betaine transporters from bacteria and betaine/4-aminobutyrate transporters from mammalian cells were low but were high to proline transporters from Arabidopsis and tomato. Two full-length transporters could complement the Na(+)-sensitive phenotype of the Escherichia coli mutant deficient in betT, putPA, proP, and proU. Both transporters could efficiently take up betaine and proline with similar affinities (K(m), 0.32-0.43 mm) and maximum velocities (1.9-3.6 nmol/min/mg of protein). The uptakes of betaine and proline were significantly inhibited by mono- and dimethylglycine but only partially inhibited by betaine aldehyde, choline, and 4-aminobutyrate. Sodium and potassium chloride markedly enhanced betaine uptake rates with optimum concentrations at 0.5 m, whereas sucrose showed only modest activation. The change of amino acids Thr(290)-Thr-Ser(292) in a putative periplasmic loop to Arg(290)-Gly-Arg(292) yielded the active transporter independent of salts, suggesting the positive charge induced a conformational change to the active form. These data clearly indicate that the betaine-accumulating mangrove contains betaine/proline transporters whose properties are distinct from betaine transporters of bacteria and mammalian cells.

Published

2002

9. slender rice, a constitutive gibberellin response mutant, is caused by a null mutation of the SLR1 gene, an ortholog of the height-regulating gene GAI/RGA/RHT/D8.

Author

Ikeda A, Ueguchi-Tanaka M, Sonoda Y, Kitano H, Koshioka M, Futsuhara Y, Matsuoka M, and Yamaguchi J

Subjects

Amino Acid Motifs genetics, Chromosome Mapping, Cloning, Molecular, Genetic Complementation Test, Mutation, Phenotype, Plant Leaves cytology, Sequence Deletion, Signal Transduction, Transcription Factors genetics, alpha-Amylases metabolism, Genes, Plant, Gibberellins metabolism, Oryza anatomy & histology, Oryza genetics, Plant Proteins genetics

Abstract

The rice slender mutant (slr1-1) is caused by a single recessive mutation and results in a constitutive gibberellin (GA) response phenotype. The mutant elongates as if saturated with GAs. In this mutant, (1) elongation was unaffected by an inhibitor of GA biosynthesis, (2) GA-inducible alpha-amylase was produced by the aleurone layers without gibberellic acid application, and (3) endogenous GA content was lower than in the wild-type plant. These results indicate that the product of the SLR1 gene is an intermediate of the GA signal transduction pathway. SLR1 maps to OsGAI in rice and has significant homology with height-regulating genes, such as RHT-1Da in wheat, D8 in maize, and GAI and RGA in Arabidopsis. The GAI gene family is likely to encode transcriptional factors belonging to the GRAS gene superfamily. DNA sequence analysis revealed that the slr1-1 mutation is a single basepair deletion of the nuclear localization signal domain, resulting in a frameshift mutation that abolishes protein production. Furthermore, introduction of a 6-kb genomic DNA fragment containing the wild-type SLR1 gene into the slr1-1 mutant restored GA sensitivity to normal. These results indicate that the slr1-1 mutant is caused by a loss-of-function mutation of the SLR1 gene, which is an ortholog of GAI, RGA, RHT, and D8. We also succeeded in producing GA-insensitive dwarf rice by transforming wild-type rice with a modified SLR1 gene construct that has a 17-amino acid deletion affecting the DELLA region. Thus, we demonstrate opposite GA response phenotypes depending on the type of mutations in SLR1.

Published

2001

10. Sugar sensing and alpha-amylase gene repression in rice embryos.

Author

Umemura Ta, Perata P, Futsuhara Y, and Yamaguchi J

Subjects

Gene Expression Regulation, Developmental, Glucosamine metabolism, Hexokinase metabolism, Oryza embryology, Oryza genetics, Phosphorylation, Promoter Regions, Genetic, Carbohydrate Metabolism, Gene Expression Regulation, Enzymologic, Gene Expression Regulation, Plant, Oryza enzymology, alpha-Amylases genetics

Abstract

We used a transient expression system to study the mechanism by which carbohydrates repress a rice (Oryza sativa L.) alpha-amylase (EC 3.2.1.1) gene. Exogenously fed metabolizable carbohydrates are able to elicit repression of the alpha-amylase gene RAmy3D in the rice embryo, and our results indicate that repression is also triggered efficiently by endogenous carbohydrates. Glucose analogs that are taken up by plant cells but not phosphorylated by hexokinase are unable to repress the alpha-amylase gene studied, while 2-deoxyglucose, which is phosphorylable but not further metabolized, down-regulates RAmy3D promoter activity, indicating a role for hexokinase in the sugar-sensing mechanism triggering repression of the RAmy3D gene. We tested two different hexokinase inhibitors, mannoheptulose and glucosamine, but only the latter was able to relieve RAmy3D promoter activity from repression by endogenous carbohydrates. This correlates with the higher ability of glucosamine to inhibit the activity of rice hexokinases in vitro. The glucosamine-mediated relief of RAmy3D promoter activity from repression by endogenous carbohydrates does not correlate with a reduced rate of carbohydrate utilization.

Published

1998

11. Functional dissection of a sugar-repressed alpha-amylase gene (RAmy1 A) promoter in rice embryos.

Author

Morita A, Umemura T, Kuroyanagi M, Futsuhara Y, Perata P, and Yamaguchi J

Subjects

Culture Media pharmacology, Gibberellins pharmacology, Oryza embryology, Oryza genetics, RNA, Messenger metabolism, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins genetics, alpha-Amylases biosynthesis, Gene Expression Regulation, Enzymologic drug effects, Gene Expression Regulation, Plant drug effects, Genes, Plant, Glucose pharmacology, Oryza enzymology, Promoter Regions, Genetic, alpha-Amylases genetics

Abstract

The gibberellin-inducible rice alpha-amylase gene, RAmy1 A, was demonstrated to be sugar repressed in rice embryos and functional dissection of the promoter of RAmy1 A in relation of its sugar-modulated expression was performed. Gibberellin-response cis-elements of GARE (TAACAAA) and pyrimidine box (CCTTTT) were partially involved in the sugar repression.

Published

1998

12. Genotypic variability for callus formation and plant regeneration in rice (Oryza sativa L.).

Author

Abe T and Futsuhara Y

Abstract

Sixty rice varieties (Oryza sativa L.), belonging to three subspecies, japonica, indica and javanica (some japonicaXindica hybrids were included), were compared for their capacity for callus growth and plant regeneration. Tissue cultures initiated from mature seeds on Murashige and Skoog's (1962) medium with 2 mg/l 2,4-dichlorophenoxyacetic acid (2,4-D) were transferred to a medium containing 0.02 mg/l 2,4-D and 10 mg/l kinetin, from which plantlets were regenerated. Large variabilities in callus growth and plant regeneration potentials were revealed among the varieties tested. Most japonica varieties formed a callus that weighed more than 100 mg per seed 30 days after inoculation, and showed a relatively high regenerative potential, whereas indica varieties, japonica-indica hybrids and javanica varieties showed poor callus growth and plant regeneration, although considerable varietal variation was observed in each subspecies. The callus growth potential was not correlated with the plant regeneration potential. Histological observations revealed that the epithelium cells of the scutellum mainly proliferated to form a callus, from which shoot and root primordia were differentiated independently from each other. The shoot primordia developed into plantlets when roots were formed adventitiously. In a few cases, shoots and roots were bilaterally initiated from a single primordium.

Published

1986

13. Selection of higher regenerative callus and change in isozyme pattern in rice (Oryza sativa L.).

Author

Abe T and Futsuhara Y

Abstract

Calli were initiated from seedling roots in rice (Oryza sativa L. var. Tadukan) and subcultured at 45-day intervals on MS medium supplemented with 2 mg/l 2,4-D. Sectors of callus which differentiated shoot meristems (green spots) under the same 2,4-D concentration were selected from the calli subcultured 90 days after initiation. The selection was continued for about 2 years. Responses to 2,4-D between original and selected lines differed considerably, although differentiation was not generally seen in rice callus in the presence of 2 mg/l 2,4-D. After 180 days, calli of the selected line differentiated into numerous shoot-bud primordia and grew out new callus tissues under 2 mg/l 2,4-D concentration; the frequency of the differentiation exceeded 90%. On the other hand, no calli of non-selected line differentiated into shootbuds under 2 mg/l 2,4-D, and the frequency of the shootbud was only about 50% under lower 2,4-D concentration (0.1 mg/l). The pattern and activity of peroxidase isozyme varied markedly between calli of the selected and non-selected lines. First, two strong peroxidase bands which show fast mobility and one intermediate peroxidase band with slow mobility were detected only in the calli of selected line. Secondly, changes in band pattern of proteins separated by SDS-PAGE were observed. In the calli of selected line, there was a loss of the polypeptide bands with molecular weight of 24 and 42 K in the selected calli, but they were clearly present in the unselected line. The appearance of new peroxidase isozyme bands and loss of polypeptide bands, change in response to auxin and increased ability for shoot bud differentiation are closely correlated to each other.

Published

1989