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定位于细胞外基质的白血病抑制因子结合蛋白的特性分析

Characterization of a binding protein for leukemia inhibitory factor localized in extracellular matrix.

作者信息

Mereau A, Grey L, Piquet-Pellorce C, Heath J K

机构信息

Department of Biochemistry, University of Oxford, UK.

出版信息

J Cell Biol. 1993 Aug;122(3):713-9. doi: 10.1083/jcb.122.3.713.

Abstract

Leukemia Inhibitory Factor (LIF) interacts with two classes of high affinity binding sites on rat UMR cells cultured in monolayer. One class of binding sites was found to be localized in the extracellular matrix (ECM) after removal of cells from the culture dish. The interaction of LIF with ECM-localized binding sites is not dependent upon either glycosylation of LIF or the presence of extracellular glycosyaminoglycans. Chemical cross-linking studies demonstrate that LIF interacts with a 200-kD cell-associated protein and a 140-kD ECM-localized protein. A 140-kD protein could also be specifically precipitated from solubilised metabolically radiolabeled UMR ECM by antibodies directed against LIF by virtue of its ability to form a stable complex with unlabeled LIF. In addition, soluble LIF associated with this ECM-localized protein is biologically active in terms of inhibition of ES cell differentiation. The properties of ECM-localized 140-kD species are very similar to those of the secreted form of the LIF receptor suggesting that the ECM localization of LIF and LIF signal transduction may be closely coupled.

摘要

白血病抑制因子(LIF)与单层培养的大鼠UMR细胞上的两类高亲和力结合位点相互作用。在将细胞从培养皿中移除后,发现一类结合位点定位于细胞外基质(ECM)中。LIF与定位于ECM的结合位点的相互作用既不依赖于LIF的糖基化,也不依赖于细胞外糖胺聚糖的存在。化学交联研究表明,LIF与一种200-kD的细胞相关蛋白和一种140-kD的定位于ECM的蛋白相互作用。凭借其与未标记LIF形成稳定复合物的能力,一种140-kD的蛋白也可以通过针对LIF的抗体从溶解的代谢放射性标记的UMR ECM中特异性沉淀出来。此外,与这种定位于ECM的蛋白相关的可溶性LIF在抑制ES细胞分化方面具有生物学活性。定位于ECM的140-kD物质的特性与LIF受体分泌形式的特性非常相似,这表明LIF的ECM定位和LIF信号转导可能紧密相关。

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