Your search keyword '"Masao Ono"' showing total 4 results

1. State of histone modification in the rat Ig-beta/growth hormone locus

Author

Kyoichi Osano and Masao Ono

Subjects

Histone-modifying enzymes, Biology, Biochemistry, Chromatin remodeling, Cell Line, Histones, Histone H1, Antigens, CD, Histone H2A, Tumor Cells, Cultured, Animals, Histone code, Nucleosome, Promoter Regions, Genetic, Models, Genetic, Reverse Transcriptase Polymerase Chain Reaction, Temperature, Acetylation, Precipitin Tests, Molecular biology, Chromatin, Introns, Nucleosomes, Rats, Growth Hormone, Histone methyltransferase, CD79 Antigens

Abstract

The state of acetylation in H3 and H4 histones and dimethylation in the H3 histone Lys4 residue were examined by chromatin immunoprecipitation (ChIP) at 11 targets in the rat Ig-beta/growth hormone locus. Marked enhancement of the acetylation of histones H3 and H4 and the dimethylation of H3 Lys4 was observed in the chromatin situated close to the promoter of an actively transcribed gene. Chromatin positioned near a cell-type-specific DNase I-hypersensitive site with enhancer activity had the same histone modifications as the active promoter. In one transcribed intron, chromatin with fewer histone modifications was found, and in another transcribed intron, chromatin with markedly enhanced modifications was found. In most cases, no appreciable difference in the acetylation of histones H3 and H4 was found at prominently enhanced targets. However, different acetylation levels of H3 and H4 were found at one target. The targets with enhanced dimethylation of the H3 Lys4 residue coincided with those with prominently enhanced acetylation of histones H3 and H4.

Published

2003

2. Novel regulatory regions found downstream of the ratB29/Ig-βgene

Author

Ayano Komatsu, Akira Otsuka, and Masao Ono

Subjects

chemistry.chemical_compound, Intergenic region, chemistry, Regulatory sequence, Electrophoretic mobility shift assay, Binding site, Biology, Biochemistry, Gene, Molecular biology, DNA, Conserved sequence, Chromatin

Abstract

To search for novel regulatory regions, we examined the features of chromatin structure in the rat B29/Ig-β gene and its flanking regions by determining DNase I hypersensitive sites (DHS) in plasmacytoma-derived Y3 cells. Six Y3 cell-specific DHS were detected at −8.6, promoter, +0.7, +4.4, +6.0, and +8.7 kb. The DHS at +4.4, +6.0, and +8.7 kb were present in the intergenic region between B29/Ig-β and growth hormone (GH) genes and were mapped inside conserved sequences in rat and humans. In transient transfection into Y3 cells, 2.9-kb DNA containing the +4.4 and +6.0-kb DHS demonstrated six times more enhancing activity than B29/Ig-β promoter alone. Three intergenic DHS each possessed enhancing activity that was highest in the +4.4-kb region. In the electrophoretic mobility shift assay, a major band shift was demonstrated with Y3 nuclear extract and 0.3-kb DNA containing the +4.4-kb region with a conserved 0.22-kb sequence. By footprint analysis, 20 bases in the middle of the 0.3-kb DNA were protected by Y3 nuclear extract in which the consensus binding site for the OCT family was present. Deletion of the footprinted region reduced enhancing activity to that of the B29/Ig-β promoter alone. The sequence responsible for the major band shift and transcriptional enhancing activity in the conserved +4.4-kb region thus coincided with the 20-bp footprinted region.

Published

2002

3. Novel regulatory regions found downstream of the rat B29/Ig-beta gene

Author

Ayano, Komatsu, Akira, Otsuka, and Masao, Ono

Subjects

Binding Sites, Base Sequence, Molecular Sequence Data, Plasma Cells, Regulatory Sequences, Nucleic Acid, Rats, Enhancer Elements, Genetic, Antigens, CD, Tumor Cells, Cultured, Animals, Deoxyribonuclease I, CD79 Antigens, Conserved Sequence, Protein Binding

Abstract

To search for novel regulatory regions, we examined the features of chromatin structure in the rat B29/Ig-beta gene and its flanking regions by determining DNase I hypersensitive sites (DHS) in plasmacytoma-derived Y3 cells. Six Y3 cell-specific DHS were detected at -8.6, promoter, +0.7, +4.4, +6.0, and +8.7 kb. The DHS at +4.4, +6.0, and +8.7 kb were present in the intergenic region between B29/Ig-beta and growth hormone (GH) genes and were mapped inside conserved sequences in rat and humans. In transient transfection into Y3 cells, 2.9-kb DNA containing the +4.4 and +6.0-kb DHS demonstrated six times more enhancing activity than B29/Ig-beta promoter alone. Three intergenic DHS each possessed enhancing activity that was highest in the +4.4-kb region. In the electrophoretic mobility shift assay, a major band shift was demonstrated with Y3 nuclear extract and 0.3-kb DNA containing the +4.4-kb region with a conserved 0.22-kb sequence. By footprint analysis, 20 bases in the middle of the 0.3-kb DNA were protected by Y3 nuclear extract in which the consensus binding site for the OCT family was present. Deletion of the footprinted region reduced enhancing activity to that of the B29/Ig-beta promoter alone. The sequence responsible for the major band shift and transcriptional enhancing activity in the conserved +4.4-kb region thus coincided with the 20-bp footprinted region.

Published

2002

4. Chromatin structure of the rat somatotropin gene locus and physical linkage of the rat somatotropin gene and skeletal-muscle sodium-channel gene

Author

Masao Ono, Koji Kazahari, Eiji Sano, and Nobuo Matsuura

Subjects

DNA, Complementary, Genetic Linkage, Molecular Sequence Data, Restriction Mapping, Gene Expression, Biology, Biochemistry, Sodium Channels, Gene expression, medicine, Animals, Deoxyribonuclease I, Humans, Cloning, Molecular, Muscle, Skeletal, Gene, Binding Sites, Base Sequence, Skeletal muscle, Cosmids, Molecular biology, Prolactin, Chromatin, Rats, medicine.anatomical_structure, Growth Hormone, Pituitary Gland, Nucleic acid, Cosmid, hormones, hormone substitutes, and hormone antagonists

Abstract

Cosmid clones from -32 kb to +74 kb region of the rat somatotropin gene locus were isolated for examination of the chromatin structure in the region from -39 kb to +47 kb by DNase I-sensitivity analysis using rat pituitary-derived GC (somatotropin+, prolactin-), and 235 (somatotropin-, prolactin+) cells, and liver-derived BRL (somatotropin-, prolactin-) cells. DNase I-hypersensitive sites (DHS) specific for somatotropin-producing cells were previously shown to be located exclusively in the -2 kb to +9 kb region [Aizawa, A., Yoneyama, T., Kazahari, K.Ono, M. (1995) Nucleic Acids Res. 23, 2236-2244]. No other DHS having this specificity was found in the region examined in this study. Except for these and two other DHS located in a cluster in this region, no DHS could be found from -23 kb to +22 kb. DHS having no or less cell-type specificity were scattered about in the -39 kb to -23 kb and +22 kb to +47 kb regions. The polyadenylation site of the human skeletal-muscle Na-channel alpha-subunit gene has been shown present 22 kb upstream from the somatotropin gene [Bennani-Baiti, I. M., Jones, B. K., Liebhaber, S. A.Cooke, N. E. (1995) Genomics 29, 647-652]. Polyadenylation site of the rat skeletal-muscle Na-channel gene was shown in this study to be at -15.7 kb. The skeletal-muscle Na-channel gene was specifically expressed in skeletal-muscle cells but not in somatotropin-producing cells, and thus the boundary region that ensures the cell-type-specific expression of each gene would appear to be situated between two genes. The region prerequisite for cell-type-specific expression of the rat somatotropin gene was estimated based on the present findings.

Published

1997