Murphy P R, Knee R S
Faculty of Medicine, Dalhousie University, Halifax, Nova Scotia, Canada.
Mol Cell Endocrinol. 1995 Oct 30;114(1-2):193-203. doi: 10.1016/0303-7207(95)96800-w.
Tumor cells of glial origin express high levels of basic fibroblast growth factor (bFGF) which stimulates their proliferation in an autocrine manner. In the present study we examined bFGF receptor (FGFR) expression and 125I-bFGF binding and processing in a human glioma cell line. RT-PCR demonstrated the co-expression of bFGF and FGFR mRNAs in five glioma cell lines examined. The high-affinity FGFR was visualized in U87-MG glioma cells by crosslinking with 125I-bFGF and by Western blotting with anti-receptor antisera. Both techniques identified a discrete 110-kDa moiety associated with the cell membrane, consistent with the reported size of one of the FGFR-1 isoforms. Western blotting also identified an intracellular receptor pool which was not accessible with exogenous 125I-bFGF. Suramin treatment induced a 2-fold increase in immunoreactive FGFR and a 1.5-fold increase in 125I-bFGF binding sites, indicating that FGFRs are chronically down-regulated by endogenous bFGF in U87-MG cells. Removal of extracellular bFGF with heparin resulted in a rapid, cycloheximide-sensitive increase in high-affinity bFGF binding sites. At 37 degrees C, receptor-bound 125I-bFGF was internalized and subjected to limited proteolytic cleavage over 12 h. U87-MG cells also contained abundant low-affinity bFGF binding sites which were removed by digestion with heparinase III but not by chondroitinase ABC. The presence of heparin (25 micrograms/ml) in the binding reaction eliminated the association of 125I-bFGF with the heparin-like sites but did not prevent binding to the high-affinity receptor. Scatchard binding analysis in the presence of heparin revealed a single class of high-affinity sites in U87-MG cells (Kd = 4.9 +/- 0.9 pM; 10-12 x 10(3) sites per cell). Neither heparin nor heparinase digestion prevented the binding of 125I-bFGF to the detergent-extractable high-affinity receptor, although both treatments significantly reduced the extent of 125I-bFGF association with the receptor. These findings indicate that in U87-MG cells, heparan sulfate proteoglycans may be involved in presentation of bFGF to the high-affinity receptor, but are not essential for high-affinity binding to occur.
胶质来源的肿瘤细胞表达高水平的碱性成纤维细胞生长因子(bFGF),该因子以自分泌方式刺激其增殖。在本研究中,我们检测了人胶质瘤细胞系中bFGF受体(FGFR)的表达以及125I-bFGF的结合与加工情况。RT-PCR显示在所检测的5种胶质瘤细胞系中bFGF和FGFR mRNA共表达。通过与125I-bFGF交联以及用抗受体抗血清进行蛋白质印迹法,在U87-MG胶质瘤细胞中观察到了高亲和力FGFR。这两种技术均鉴定出一种与细胞膜相关的110 kDa离散部分,与报道的FGFR-1亚型之一的大小一致。蛋白质印迹法还鉴定出一个细胞内受体池,外源性125I-bFGF无法进入该池。苏拉明处理使免疫反应性FGFR增加了2倍,125I-bFGF结合位点增加了1.5倍,表明在U87-MG细胞中FGFR被内源性bFGF长期下调。用肝素去除细胞外bFGF导致高亲和力bFGF结合位点迅速增加,且对放线菌酮敏感。在37℃时,受体结合的125I-bFGF被内化,并在12小时内进行有限的蛋白水解切割。U87-MG细胞还含有丰富的低亲和力bFGF结合位点,这些位点可被肝素酶III消化去除,但不能被软骨素酶ABC去除。结合反应中肝素(25μg/ml)的存在消除了125I-bFGF与类肝素位点的结合,但不阻止其与高亲和力受体的结合。在肝素存在下进行的Scatchard结合分析显示U87-MG细胞中有一类单一的高亲和力位点(Kd = 4.9±0.9 pM;每个细胞10 - 12×10(3)个位点)。肝素和肝素酶消化均未阻止125I-bFGF与去污剂可提取的高亲和力受体的结合,尽管两种处理均显著降低了125I-bFGF与受体的结合程度。这些发现表明,在U87-MG细胞中,硫酸乙酰肝素蛋白聚糖可能参与将bFGF呈递给高亲和力受体,但对于高亲和力结合的发生并非必不可少。
