Faculty of Medical Technology

川本 保子

カワモト ヤスコ  (Yasuko Kawamoto)

基本情報

所属
藤田保健衛生大学 医療科学部 臨床検査学科 微生物学 教授
学位
博士(医学)(名古屋大学)
農学修士(名古屋大学)

J-GLOBAL ID
200901035445866926
researchmap会員ID
1000208959

MISC

 9
  • 藤田学園医学会誌 22(1) 137-141 1998年  
  • K Sasaki, T Kobayashi, S Imamura, T Shigekura, R Kato, Y Kawamoto, T Tsuji, A Miyama
    IMMUNOLOGY LETTERS 55(1) 11-13 1997年1月  
    There is increasing evidence for the role of the Fas/Fas ligand interaction in the immunoregulation of T-cells. We studied the expression of the Fas ligand (FasL) in activated peripheral T-cells in vitro, and its relation to autonomous cell death by flow cytometry. Following the stimulation of lymph node T-cells with anti-CD3 and rIL2, the mRNA level of FasL increased more than four times during the first 2 days over the level before stimulation. The surface expression of FasL was observed on 27% of the population at day 2 after stimulation and increased to approximately 50% at day 3. Kinetic analysis by flow cytometry, however, indicated that all T-blasts transformed during activation did not express FasL. FasL expression became evident simultaneously with the termination of cell expansion. Since cells remained viable (> 90%) at day 3 as judged by trypan blue-exclusion, cell membranes expressing Fast were supposed to be still intact. Concomitantly with Fast-expression, spontaneous DNA fragmentation was observed. These observations support the idea that autonomous Fas/FasL interaction mediates apoptosis in activated peripheral T-cells as demonstrated in T-cell hybridoma or established T-cells. (C) 1997 Elsevier Science B.V.
  • Immunology 91 17-25 1997年  
  • 藤田学園医学会誌 20(2) 255-258 1996年  
  • Yutaka Kato, Takashi Yokochi, Keiko Sasaki, Yasuko Kawamoto, Takao Tsuji, Akio Miyama
    Immunobiology 196(5) 465-474 1996年  
    Na-CBZ-L-lysine thiobenzyl ester (BLT)-specific proteases in cytoplasmic granules of intraepithelial lymphocytes in the murine intestine (iIEL) were characterized. BLT-specific proteases were isolated with the Sephacryl S-200 column chromatography, and the sample isolated contained a protein with a molecular weight of 58 kDa. The 58 kDa protein consisted of the homodimer of the 30 kDa subunits. The 58 kDa protease was detected by [&lt sup&gt 3&lt /sup&gt ] diisopropylfluorophosphate (DFP)-labeling, and also detectable by the immunoblotting using an antibody against the partial synthetic peptide of granzymce A. The cytoplasmic granules of iIEL were stained positively by an immunofluorescence with anti-granzyme A antibody. Therefore, it was suggested that the major BLT-specific proteases present in cytoplasmic granules of iIEL, might be granzyme A.