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Featured researches published by Tamura Gakuzo.


Gene | 1985

Synthesis and secretion of biologically active mouse Interferon-β using a Bacillus subtilis α-amylase secretion vector

Shiroza Teruaki; Nakazawa Kiyoshi; Tashiro Naoyuki; Yamane Kunio; Yanagi Kazuo; Yamasaki Makari; Tamura Gakuzo; Saito Hiuga; Kawade Yoshimi; Taniguchi Tadatsugu

Mouse interferon-beta (IFN-beta) cDNA, whose signal sequence had been removed by BAL 31 digestion, was introduced into a Bacillus subtilis secretion vector constructed by using the promoter and signal sequence of the B. subtilis alpha-amylase gene. The resultant chimeric plasmids were transferred into B. subtilis 207-25. Four kanamycin-resistant transformants were selected by both colony hybridization and a new immunoblot method for secretory proteins. They secrete the proteins which cross-react with sheep anti-mouse IFN-beta serum into the culture medium. One of them expressed a high IFN-beta activity as assayed by the L cell and vesicular stomatitis virus system, while the other three showed weak or little IFN activities. Based on our previous study [Ohmura et al., Nucl. Acids Res. 12 (1984) 5307-5319], it was suggested that the secreted IFN molecules are hybrid proteins in which the NH2-terminal region consists of part of the alpha-amylase signal peptide. Nucleotide sequence analysis revealed that plasmid pTUB502, which expressed high IFN activity, is joined to the mouse IFN-beta gene from the codon position 6 of its mature protein. The other three plasmids, pTUB506, pTUB509, and pTUB519, contain the mouse IFN-beta gene from the codon positions 3, 1, and -5, respectively. The NH2-terminal region of the mouse IFN-beta seems to be closely related to its biological activity.


Gene | 1991

Nucleotide sequence and expression of the glucoamylase-encoding gene (glaA) from Aspergillus oryzae

Hata Yoji; Tsuchiya Kozo; Kitamoto Katsuhiko; Gomi Katsuya; Kmnagai Chieko; Tamura Gakuzo; Hara Shodo


Archive | 1990

Selective medium for orginase gene-deficient strain, breeding of urea-nonproductive yeast using the same and preparation of liquor using the yeast

Kitamoto Katsuhiko; Oda Kaoko; Gomi Katsuya; Kumagai Chieko; Hara Masamichi; Tamura Gakuzo


Archive | 1988

Plasmid vector for gene destruction or gene replacement, transformant therefrom and its use

Takahashi Kojiro; Iimura Minoru; Gomi Katsuya; Hara Masamichi; Yoshizawa Kiyoshi; Minazu Tetsuyoshi; Tamura Gakuzo


Archive | 1986

MICROBIAL PRODUCTION OF UROGASTRONE

Kishimoto Fumitaka; Ito Akira; Gomi Hideyuki; Yasukui Hideo; Ogino Shigeo; Yoda Koji; Yamazaki Masakari; Tamura Gakuzo


Archive | 1994

PRODUCION OF YEAST CELL WALL-LYSING ENZYME AND METHOD FOR LYSING THE SAME

Hara Masamichi; Tadenuma Makoto; Sato Shunichi; Ietou Haruyuki; Shimoii Hitoshi; Sugiyama Ryuichi; Tamura Gakuzo


Archive | 1996

BETA-GALACTOSIDASE GENE

Ito Yoshiyuki; Sasaki Takashi; Gomi Katsuya; Kitamoto Katsuhiko; Takahashi Kojiro; Kumagai Chieko; Tamura Gakuzo


Archive | 1994

ALPHA-GLUCOSIDASE GENE, VECTOR, TRANSFORMED ORGANISM AND PRODUCTION OF ALPHA-GLUCOSIDASE USING THE ORGANISM

Minetoki Toshiki; Tamura Gakuzo; Gomi Katsuya; Kitamoto Katsuhiko; Kumagai Chieko


Archive | 1993

PHOSPHOGLYCERATE KINASE GENE PROMOTER, ITS TERMINATOR OR/AND GENE EXPRESSION UNIT COMPOSED OF THE SAME, GENOME GENE OF PHOSPHOGLYCERATE KINASE AND CDNA GENE

Ogawa Masahiro; Tamura Gakuzo; Gomi Katsuya; Kitamoto Katsuhiko; Kumagai Chieko


Archive | 1992

PRODUCTION OF YEAST CELL WALL-LYSING ENZYME AND ITS UTILIZATION

Hara Masamichi; Tadenuma Makoto; Sato Shunichi; Ietou Haruyuki; Shimoii Hitoshi; Sugiyama Ryuichi; Tamura Gakuzo

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