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幼仓鼠肾细胞成纤维细胞生长因子受体的鉴定及部分特性分析。

The identification and partial characterization of the fibroblast growth factor receptor of baby hamster kidney cells.

作者信息

Neufeld G, Gospodarowicz D

出版信息

J Biol Chem. 1985 Nov 5;260(25):13860-8.

PMID:2997183
Abstract

The binding of biologically active, 125I-labeled basic fibroblast growth factor (FGF) to baby hamster kidney-derived cell line cells (BHK-21) was studied at 4 degrees C. Unlabeled FGF displaced cell surface bound 125I-FGF, but platelet-derived growth factor, epidermal growth factor, insulin, or transferrin did not. Binding was saturable both as a function of time and as a function of increasing 125I-FGF concentrations. Scatchard analysis of the binding data revealed the presence of about 1.2 X 10(5) binding sites/cell with an apparent KD of 270 pM. The number of the binding sites was down-regulated following preincubation of the cells with FGF. The density of binding sites/cell also decreased as an inverse function of cell density. When 125I-FGF binding was studied in a BHK-21 cell membrane preparation, it was found that the membranal binding site displayed a lower KD of 21 pM. 125I-FGF was covalently cross-linked to its cell surface receptor on intact BHK-21 cells using the homobifunctional agent disuccinimidyl suberate. Two macromolecular species with an apparent molecular weight of 145,000 and 125,000, respectively, were labeled under both reducing and nonreducing conditions. Unlabeled FGF competed with 125I-FGF for binding to both macromolecular species. The labeling of the macromolecules was also inhibited by heparin. No labeling was observed in the absence of the cross-linkers or when heat-inactivated 125I-FGF was used instead of radiolabeled, biologically active FGF.

摘要

在4℃下研究了具有生物活性的125I标记的碱性成纤维细胞生长因子(FGF)与幼仓鼠肾衍生细胞系细胞(BHK - 21)的结合。未标记的FGF能取代细胞表面结合的125I - FGF,但血小板衍生生长因子、表皮生长因子、胰岛素或转铁蛋白则不能。结合作用在时间和125I - FGF浓度增加方面均具有饱和性。对结合数据进行Scatchard分析显示,每个细胞存在约1.2×10⁵个结合位点,表观解离常数(KD)为270 pM。在用FGF对细胞进行预孵育后,结合位点的数量下调。每个细胞结合位点的密度也随细胞密度呈反比下降。当在BHK - 21细胞膜制剂中研究125I - FGF结合时,发现膜结合位点的KD较低,为21 pM。使用同双功能试剂辛二酸二琥珀酰亚胺酯将125I - FGF与完整BHK - 21细胞表面的受体进行共价交联。在还原和非还原条件下均标记出两种表观分子量分别为145,000和125,000的大分子物质。未标记的FGF与125I - FGF竞争结合这两种大分子物质。肝素也抑制大分子物质的标记。在没有交联剂的情况下或使用热灭活的125I - FGF代替放射性标记的具有生物活性的FGF时,未观察到标记现象。

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