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一种胞外蛋白激酶的主要细胞表面定位蛋白底物是已知核蛋白的同源物。

Major cell surface-located protein substrates of an ecto-protein kinase are homologs of known nuclear proteins.

作者信息

Jordan P, Heid H, Kinzel V, Kübler D

机构信息

Department of Pathochemistry, German Cancer Research Center, Heidelberg, Federal Republic of Germany.

出版信息

Biochemistry. 1994 Dec 13;33(49):14696-706. doi: 10.1021/bi00253a007.

DOI:10.1021/bi00253a007
PMID:7993898
Abstract

Cell surface polypeptides serve as substrates for a casein kinase-like ecto-protein kinase activity which is demonstrable under stringent criteria with intact cells using micromolar levels of extracellular [gamma-32P]ATP. Two major 32P-labeled proteins, designated as pp100 and pp120 after their apparent molecular masses on SDS-PAGE under reducing and nonreducing conditions, have repeatedly appeared in the phosphoprotein spectra of different cell types. We have chosen HeLa cells as a source for the biochemical characterization and isolation of pp100 and pp120. Phosphorylation of pp100 and pp120 occurs in their extracellular domains at seryl residues of amino acid side chains. Several criteria deduced from the heparin sensitivity of the ecto-protein kinase and its substrate-induced shedding into the cell supernatant indicated that surface phosphorylation is a function of the ecto-protein kinase. The radioactive phosphorylation of pp100 and pp120 which coincides with their biotinylation on 2D-blots can be reversed by mild trypsination of intact cells. Purification and enrichment of pp100 and pp120 were achieved on the basis of radioactivity detection on and isolation from 1D- and 2D-gels. Amino acid sequence analysis performed on tryptic digests of purified ecto-phosphoproteins in most cases showed significant consensus sequences between pp100 and the nuclear RNA-binding protein nucleolin while pp120 sequences proved to be related to hnRNP U, a nucleoplasmic pre-mRNA-binding protein. Immunochemical analysis using anti-nucleolin and anti-hnRNP U antibodies combined with comparative phosphorylation and characterization of the ecto-proteins with authentic nucleolin and hnRNP U further established the close relationship, suggesting surface membrane versions of the nuclear proteins.

摘要

细胞表面多肽是一种酪蛋白激酶样胞外蛋白激酶活性的底物,在严格条件下,使用微摩尔浓度的细胞外[γ-32P]ATP,完整细胞可显示出这种活性。在还原和非还原条件下,根据SDS-PAGE上的表观分子量,两种主要的32P标记蛋白分别命名为pp100和pp120,它们反复出现在不同细胞类型的磷蛋白谱中。我们选择了HeLa细胞作为pp100和pp120生化特性鉴定及分离的来源。pp100和pp120在其细胞外结构域的氨基酸侧链丝氨酸残基处发生磷酸化。从胞外蛋白激酶的肝素敏感性及其底物诱导释放到细胞上清液中推导出来的几个标准表明,表面磷酸化是胞外蛋白激酶的一种功能。pp100和pp120的放射性磷酸化与其在二维印迹上的生物素化同时发生,可通过对完整细胞进行温和胰蛋白酶处理来逆转。基于一维和二维凝胶上的放射性检测以及从凝胶上进行分离,实现了pp100和pp120的纯化和富集。对纯化的胞外磷蛋白的胰蛋白酶消化产物进行的氨基酸序列分析,在大多数情况下显示pp100与核RNA结合蛋白核仁素之间有显著的共有序列,而pp120序列被证明与hnRNP U相关,hnRNP U是一种核质前体mRNA结合蛋白。使用抗核仁素和抗hnRNP U抗体的免疫化学分析,结合对胞外蛋白与真实核仁素和hnRNP U的比较磷酸化及特性鉴定,进一步证实了这种密切关系,表明存在核蛋白的表面膜形式。

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