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伴刀豆球蛋白A与兔胸腺细胞质膜的相互作用。低亲和力结合与由特定糖蛋白介导的正协同结合之间的区别。

Interaction of concanavalin A with rabbit thymocyte plasma membranes. Distinction between low affinity assoication and positively cooperative binding mediated by a specific glycoprotein.

作者信息

Schmidt-Ullrich R, Wallach D F, Hendricks J

出版信息

Biochim Biophys Acta. 1976 Sep 7;443(3):587-600. doi: 10.1016/0005-2736(76)90475-2.

Abstract
  1. We have analyzed the interaction of the mitogenic lectin, concanavalin A, with purified plasma membranes isolated from rabbit thymocytes. 2. Scatchard analyses show that in native membranes binding is positively cooperative at low concanavalin A concentrations and non-interacting at high lectin levels. 3. In contrast, membranes treated with 0.0064 M glutaraldehyde exhibit diphasic Scatchard plots, indicating the presence of high- and low-affinity binding sites. The high-affinity zone corresponds to the region of positive cooperativity in native membranes. 4. The number of high-affinity binding sites per cell-equivalent corresponds approximately to the number of glycoprotein (mol. wt. 55000) molecules (1-10(6)/cell), but account for less than 25% of the total lectin binding. 5. Treatment of membranes with 0.0064 M glutaraldehyde selectively crosslinks the glycoprotein (mol. wt. 55000) and its multimers, correlating directly with the modifications of concanavalin A-binding. 6. We conclude that high-affinity binding of concanavalin A to thymocyte membranes is a cooperative process mediated by the glycoprotein (mol. wt. 55000). We further conclude that the bulk of concanavalin A binding is through low-affinity associations, not involving specific membrane macromolecules.
摘要
  1. 我们分析了促有丝分裂凝集素伴刀豆球蛋白A与从兔胸腺细胞分离的纯化质膜之间的相互作用。2. 斯卡查德分析表明,在天然膜中,在低伴刀豆球蛋白A浓度下结合是正协同的,而在高凝集素水平下是非相互作用的。3. 相比之下,用0.0064 M戊二醛处理的膜呈现双相斯卡查德图,表明存在高亲和力和低亲和力结合位点。高亲和力区对应于天然膜中正协同作用的区域。4. 每细胞当量的高亲和力结合位点数量大约对应于糖蛋白(分子量55000)分子的数量(1 - 10⁶/细胞),但占总凝集素结合的不到25%。5. 用0.0064 M戊二醛处理膜会选择性地交联糖蛋白(分子量55000)及其多聚体,这与伴刀豆球蛋白A结合的改变直接相关。6. 我们得出结论,伴刀豆球蛋白A与胸腺细胞膜的高亲和力结合是一个由糖蛋白(分子量55000)介导的协同过程。我们进一步得出结论,大部分伴刀豆球蛋白A的结合是通过低亲和力关联,不涉及特定的膜大分子。

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