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造血生长因子在体外可上调骨髓祖细胞上的Ⅱ型p65白细胞介素-1受体。

Hematopoietic growth factors upregulate the p65 type II interleukin-1 receptor on bone marrow progenitor cells in vitro.

作者信息

Dubois C M, Ruscetti F W, Jacobsen S E, Oppenheim J J, Keller J R

机构信息

Laboratory of Immunoregulation, National Cancer Institute (NCI), Frederick, MD.

出版信息

Blood. 1992 Aug 1;80(3):600-8.

PMID:1379082
Abstract

Having previously shown that interleukin-1 (IL-1) induces the expression of IL-1 receptors (IL-1Rs) on bone marrow (BM) cells in vivo through an indirect mechanism, we studied whether hematopoietic growth factors (HGFs) could induce the expression of IL-1R on BM cells in vitro. In vitro treatment of light-density murine BM (LDBM) cells with either IL-3, IL-6, granulocyte--colony-stimulating factor (CSF), or granulocyte-macrophage--CSF caused a 5- to 10-fold upregulation of IL-1R expression, whereas IL-1, IL-5, IL-7, and macrophage-CSF had no effect. Scatchard analysis showed one class of IL-1Rs on LDBM cells with an average of 66 +/- 20 sites per cells. After 24 hours of treatment with IL-3, the number of IL-1Rs increased to 413 +/- 125, without effecting the affinity. This effect required protein synthesis, but was independent of cell division. Purified lineage-negative progenitor cells (Lin-) did not express detectable levels of IL-1R, but 24 hours of treatment with IL-3, GM-CSF, and G-CSF stimulated IL-1--specific binding. Autoradiographic analysis of Lin- cells showed that IL-1R induction by IL-3 occurs on undifferentiated blast cells. Affinity labeling of Lin- cells treated with HGFs showed an increase in a 65-Kd IL-1 binding protein that did not bind or compete with an anti-type I IL-1R antibody, suggesting that these cells expressed type II IL-1R. These data suggest that IL-1 stimulation of myelopoiesis occurs by a mechanism involving IL-1R upregulation on hematopoietic progenitor cells by HGFs.

摘要

先前我们已经表明,白细胞介素-1(IL-1)通过间接机制在体内诱导骨髓(BM)细胞上白细胞介素-1受体(IL-1Rs)的表达,我们研究了造血生长因子(HGFs)是否能在体外诱导BM细胞上IL-1R的表达。用IL-3、IL-6、粒细胞集落刺激因子(CSF)或粒细胞巨噬细胞集落刺激因子对低密度小鼠BM(LDBM)细胞进行体外处理,导致IL-1R表达上调5至10倍,而IL-1、IL-5、IL-7和巨噬细胞集落刺激因子则无作用。Scatchard分析显示LDBM细胞上有一类IL-1Rs,平均每个细胞有66±20个位点。用IL-3处理24小时后,IL-1Rs的数量增加到413±125,而不影响亲和力。这种效应需要蛋白质合成,但与细胞分裂无关。纯化的谱系阴性祖细胞(Lin-)不表达可检测水平的IL-1R,但用IL-3、粒细胞巨噬细胞集落刺激因子和粒细胞集落刺激因子处理24小时可刺激IL-1特异性结合。对Lin-细胞的放射自显影分析表明,IL-3诱导IL-1R发生在未分化的母细胞上。用HGFs处理的Lin-细胞的亲和标记显示,一种65-Kd的IL-1结合蛋白增加,该蛋白不与抗I型IL-1R抗体结合或竞争,表明这些细胞表达II型IL-1R。这些数据表明,IL-1对骨髓生成的刺激是通过一种机制实现的,该机制涉及HGFs上调造血祖细胞上的IL-1R。

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