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一种新型细胞因子反应性细胞表面糖蛋白在原位定义了髓质胸腺上皮的一个亚群。

A novel cytokine-responsive cell surface glycoprotein defines a subset of medullary thymic epithelium in situ.

作者信息

Farr A, Nelson A, Hosier S, Kim A

机构信息

Department of Biological Structure, University of Washington, Seattle 98195.

出版信息

J Immunol. 1993 Feb 15;150(4):1160-71.

PMID:8432973
Abstract

A hamster mAb (10.1.1), raised against long term cultures of uncloned thymic stromal cells, selectively labeled a subpopulation of medullary stromal cells in situ. By ultrastructural and phenotypic criteria, the stromal cells labeled by this mAb were judged to be epithelial. Although some of the 10.1.1+ epithelial cells were reticular, others were globular and some were associated with structures resembling Hassal's bodies. Ultrastructural immunohistochemistry suggested that 10.1.1 labeling of some of the epithelial cells was preferentially associated at areas of epithelial cell contact with adjacent thymocytes. Reactivity of thymic stromal cells with this antibody was developmentally regulated. A few scattered 10.1.1+ cells were observed at day 14 of gestation, and there were progressive increases in both the extent and intensity of 10.1.1 labeling evident through birth. One thymic stromal cell line, Z210.1, exhibited low levels of constitutive reactivity with this antibody. Exposure to IL-1 resulted in enhanced 10.1.1 reactivity of this cell line, with little, if any, additional response to TNF-alpha or IFN-gamma. Under the same conditions, ICAM-1 expression by this cell line was elevated in response to IL-1, TNF-alpha, or INF-gamma. Immunoprecipitation of detergent lysates prepared from Z210.1.7 cells exposed to IL-1 24 h before cell surface iodination identified a cell surface protein with a molecular mass of about 92 kDa under nonreducing conditions and about 95 kDa under reducing conditions. Digestion of 10.1.1 immunoprecipitates with N-glyconase resulted in a small (5 kDa) reduction in molecular mass. The molecule recognized by the 10.1.1 mAb was distinct from ICAM-1, which possessed a molecular mass of 100 kDa (nonreduced) and 110 kDa (reduced), and also displayed a smaller N-glyconase-resistant molecular mass (65 to 85 kDa).

摘要

一种针对未克隆胸腺基质细胞长期培养物产生的仓鼠单克隆抗体(10.1.1),能在原位选择性标记髓质基质细胞的一个亚群。根据超微结构和表型标准,被该单克隆抗体标记的基质细胞被判定为上皮细胞。尽管部分10.1.1 +上皮细胞呈网状,但其他细胞呈球状,还有一些与类似哈索尔小体的结构相关。超微结构免疫组织化学表明,部分上皮细胞的10.1.1标记优先出现在上皮细胞与相邻胸腺细胞接触的区域。胸腺基质细胞与该抗体的反应性受发育调控。在妊娠第14天观察到少数散在的10.1.1 +细胞,从出生前到出生,10.1.1标记的范围和强度都有逐渐增加。一种胸腺基质细胞系Z210.1与该抗体的组成型反应性水平较低。暴露于白细胞介素-1会增强该细胞系的10.1.1反应性,对肿瘤坏死因子-α或干扰素-γ几乎没有额外反应(如果有也极少)。在相同条件下,该细胞系的细胞间黏附分子-1(ICAM-1)表达会因白细胞介素-1、肿瘤坏死因子-α或干扰素-γ而升高。对在细胞表面碘化前24小时暴露于白细胞介素-1的Z210.1.7细胞制备的去污剂裂解物进行免疫沉淀,在非还原条件下鉴定出一种分子量约为92 kDa的细胞表面蛋白,在还原条件下约为95 kDa。用N-糖苷酶消化10.1.1免疫沉淀物会导致分子量小幅降低(5 kDa)。被10.1.1单克隆抗体识别的分子与ICAM-1不同,ICAM-1的分子量为100 kDa(非还原)和110 kDa(还原),且其对N-糖苷酶抗性的分子量也较小(65至85 kDa)。

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