Raboudi N, Julian J, Rohde L H, Carson D D
Department of Biochemistry and Molecular Biology, University of Texas, M. D. Anderson Cancer Center, Houston 77030.
J Biol Chem. 1992 Jun 15;267(17):11930-9.
The interaction of heparin (HP) with the cell-surface components of a human uterine epithelial carcinoma cell line (RL95) was studied. Binding of [3H]HP to cell surfaces was saturable in a dose- and time-dependent manner. HP and certain forms of heparan sulfate (HS) efficiently compete for [3H]HP binding. In contrast, other glycosaminoglycans, such as chondroitin sulfate, keratan sulfate, hyaluronic acid, and dermatan sulfate, do not compete for binding to these sites. Scatchard analysis revealed that [3H]HP bound to these sites with an apparent KD of 0.7-0.9 microM and a binding capacity of 9 x 10(6) sites/cell to attached cells. EDTA-detached cells displayed a similar apparent KD, but an approximately 2-fold increase in binding capacity. Protease digestion of cells on ice markedly reduced [3H]HP binding, indicating that these binding sites were associated with proteins. In contrast, heparinase treatment of cells stimulated binding by approximately 2-fold, indicating that a large fraction of these binding sites were occupied with endogenous ligand. We examined the structural features of HP/HS required for HP/HS binding. O-Sulfation, substitution of amino groups, and, to a lesser extent, the presence of carboxyl groups were important recognition features of HP/HS by cell-surface HP/HS-binding sites. N-Sulfation was not required. Photoaffinity labeling with 125I-sulfosuccinimidyl 2-(p-azidosalicylamido)-ethyl-1, 3-dithiopropionate-HP was used to identify HP/HS-binding proteins on RL95 cell surfaces. Proteins with M(r) values of 14,000-18,500 and 31,000 were photolabeled at the surfaces of attached cells. Photolabeling was blocked by the addition of excess HP, but not chondroitin sulfate. Additional proteins with M(r) values greater than 31,000 were photolabeled specifically on EDTA-detached cells. Moreover, the M(r) 14,000-18,500 and 31,000 proteins were retained on the EDTA-detached cells. These observations indicated that certain cell-surface HP/HS-binding proteins were not exposed when cells were attached to substrata. Proteins of similar M(r) values as the photolabeled components as well as many additional proteins were identified by heparin-agarose chromatographic selection of extracts of cells labeled metabolically with [35S]methionine or vectorially with Na125I at the cell surface. Fragments of cell-surface HP/HS-binding proteins were released from intact RL95 and mouse uterine epithelial cells by mild trypsinization and isolated by heparin-agarose affinity chromatography. Three peptides with M(r) values between 6000 and 14,000 required greater than 0.5 M salt for elution from heparin-agarose, retained HP binding activity in a 125I-HP gel overlay assay, and selectively bound [3H]HP in a solid-phase binding assay.(ABSTRACT TRUNCATED AT 400 WORDS)
研究了肝素(HP)与人子宫上皮癌细胞系(RL95)细胞表面成分的相互作用。[3H]HP与细胞表面的结合呈剂量和时间依赖性饱和。HP和某些形式的硫酸乙酰肝素(HS)能有效竞争[3H]HP的结合。相比之下,其他糖胺聚糖,如硫酸软骨素、硫酸角质素、透明质酸和硫酸皮肤素,不竞争这些位点的结合。Scatchard分析显示,[3H]HP与这些位点结合的表观解离常数(KD)为0.7 - 0.9微摩尔,贴壁细胞的结合容量为9×10⁶个位点/细胞。经乙二胺四乙酸(EDTA)处理分离的细胞表现出相似的表观KD,但结合容量增加约2倍。在冰上用蛋白酶消化细胞显著降低了[3H]HP的结合,表明这些结合位点与蛋白质相关。相反,用肝素酶处理细胞可使结合增加约2倍,表明这些结合位点的很大一部分被内源性配体占据。我们研究了HP/HS结合所需的HP/HS结构特征。O-硫酸化、氨基取代以及在较小程度上羧基的存在是细胞表面HP/HS结合位点识别HP/HS的重要特征。N-硫酸化并非必需。用125I-磺基琥珀酰亚胺2-(对叠氮水杨酰胺基)-乙基-1,3-二硫代丙酸酯-HP进行光亲和标记,以鉴定RL95细胞表面的HP/HS结合蛋白。在贴壁细胞表面,分子量(M(r))为14,000 - 18,500和31,000的蛋白质被光标记。加入过量HP可阻断光标记,但硫酸软骨素不能。在EDTA分离的细胞上,特异性光标记了另外一些M(r)大于3,1000的蛋白质。此外,M(r) 14,000 - 18,500和31,000的蛋白质保留在EDTA分离的细胞上。这些观察结果表明,当细胞附着于基质时,某些细胞表面的HP/HS结合蛋白未暴露。通过肝素-琼脂糖色谱法从用[35S]甲硫氨酸代谢标记或在细胞表面用Na125I向量标记的细胞提取物中选择,鉴定出了与光标记成分M(r)值相似的蛋白质以及许多其他蛋白质。通过温和胰蛋白酶消化从完整的RL95和小鼠子宫上皮细胞中释放细胞表面HP/HS结合蛋白的片段,并通过肝素-琼脂糖亲和色谱法分离。三种M(r)值在6000至14,000之间的肽从肝素-琼脂糖上洗脱需要大于0.5 M的盐,在125I-HP凝胶覆盖试验中保留HP结合活性,并在固相结合试验中选择性结合[3H]HP。(摘要截短于400字)
