IDENTIFICATION OF A SOLUBLE IL-2 RECEPTOR BETA-CHAIN FROM HUMAN LYMPHOID-CELL LINE CELLS

被引:0
作者
HONDA, M
KITAMURA, K
TAKESHITA, T
SUGAMURA, K
TOKUNAGA, T
机构
[1] NATL INST HLTH,DEPT CELLULAR IMMUNOL,TOKYO 141,JAPAN
[2] TOHOKU UNIV,SCH MED,DEPT BACTERIOL,SENDAI,MIYAGI 980,JAPAN
来源
JOURNAL OF IMMUNOLOGY | 1990年 / 145卷 / 12期
关键词
D O I
暂无
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
A clone was isolated from the human lymphoid cell line YT that displayed IL-2R-beta, and was found to express much higher levels of IL-2R-beta than the original cells. Combining cell surface iodination, affinity labeling of the released soluble protein, and fluorescence sandwich-ELISA for both IL-2 and IL-2. (soluble)(s) IL-2R-beta reactants revealed the presence of IL-2-binding protein in the culture supernatant as soluble forms of IL-2R-beta. By using the fluorescence sandwich-ELISA elevated levels of sIL-2R-beta were measured in culture supernatants of human T cell leukemia virus I positive T cell lines. In addition to this constitutive production of sIL-2R-beta, normal PBMC could release low levels of IL-2R-beta by stimulation with PHA. In contrast, this was not found in certain human T cell leukemia virus I negative T cell, B cell and macrophage lines. Immunoprecipitation of the soluble protein with IL-2R-beta-specific mAb characterized it as an apparent 50- to 55-kDa molecule that is distinct from the 45-kDa soluble IL-2R-alpha. Moreover, 10 to 15% of the total cell surface molecules were release into culture supernatants. These results suggest that the released IL-2R-beta might serve as an immunoregulatory function in IL-2 dependent both normal and abnormal immune responses.
引用
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页码:4131 / 4135
页数:5
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