Nicolson G L, Lacorbiere M, Eckhart W
Biochemistry. 1975 Jan 14;14(1):172-9. doi: 10.1021/bi00672a029.
The lectin receptors of confluently grown hamster BHK, wild type polyoma virus transformed PyBHK, and temperature-sensitive polyoma transformed ts3-PyBHK fibroblasts were investigated using cell agglutination, quantitative (125I)lectin binding, and ferritin-lectin labeling. PyBHK and permissively grown ts3-PyBHK cells agglutinated more strongly with Ricinus communis I agglutinin (RCA-I)compared to BHK and nonpermissively grown ts3-PyBHK, although saturation binding of (125I)RCA-I to these cells at 4 degrees resulted in a twofold difference in lectin-binding sites on BHK and nonpermissively grown ts3-PyBHK cells (1.0-1.3 x 10 7 sites/cell) compared to PyBHK and permissively grown ts3-PyBHK (0.4-0.6 x 10 7 sites/cell). These cells bound equivalent amounts of (125I)concanavalin A (0.8-1 x 10 7 sites/cell) and (125I)wheat germ agglutinin (1-2.2 x 10 7 sites/cell). Under these binding conditions little endocytosis occurred, as judged by the subsequent release of greater than 90% cell-bound (125I)RCA-I by the RCA-I inhibitor lactose and localization of ferritin-RCA-I exclusively to the extracellular plasma membrane surface. However, if the binding is performed at 22 degrees, only 50% of the bound lectin can be removed by lactose, and ferritin-RCA-I is localized inside the cell within endocytotic vesicles. The relative mobility of RCA-I receptors was examined on ts3-PyBHK cells by the ability of ferritin-RCA-I to induce clustering of its receptors at 22 degrees. RCA-I receptors on permissively grown ts3-PyBHK cells appeared to be more mobile than on nonpermissively grown cells. BHK and PyBHK cells were treated with neuraminidase, and the resulting enzyme-treated cells were assayed for lectin agglutinability and quantitative binding of RCA-I, concanavalin A, and wheat germ agglutinin. Neuraminidase treatment resulted in decreased concanavalin A and wheat germ agglutinability and a slight increase in RCA-I agglutinability. The enzyme-treated BHK and PyBHK cells bound less (125I)wheat germ agglutinin (2.8 x 10 6 and 2.2 x 10 6 sites/cell, respectively) and 2.5 and 6.2 times more (125I)RCA-I (2.5-3 x 10 7) and 3.5-4 x 10 7 sites/per cell, respectively). There was no change in the number of concanavalin A binding sites after neuraminidase treatment. The increase in RCA-I binding sites approximated the decrease in wheat germ agglutinin binding sites indicating that the predominant penultimate oligosaccharide residue to sialic acid on these cells is D-Gal.
运用细胞凝集、定量(125I)凝集素结合及铁蛋白 - 凝集素标记法,对汇合生长的仓鼠BHK细胞、野生型多瘤病毒转化的PyBHK细胞以及温度敏感型多瘤病毒转化的ts3 - PyBHK成纤维细胞的凝集素受体进行了研究。与BHK细胞和非允许生长的ts3 - PyBHK细胞相比,PyBHK细胞以及允许生长的ts3 - PyBHK细胞与蓖麻凝集素I(RCA - I)的凝集作用更强,尽管在4℃条件下(125I)RCA - I与这些细胞的饱和结合显示,BHK细胞和非允许生长的ts3 - PyBHK细胞上的凝集素结合位点(1.0 - 1.3×10^7个位点/细胞)是PyBHK细胞和允许生长的ts3 - PyBHK细胞(0.4 - 0.6×10^7个位点/细胞)的两倍。这些细胞结合等量的(125I)伴刀豆球蛋白A(0.8 - 1×10^7个位点/细胞)和(125I)麦胚凝集素(1 - 2.×10^7个位点/细胞)。在这些结合条件下,内吞作用很少发生,这可通过RCA - I抑制剂乳糖随后释放大于90%细胞结合的(125I)RCA - I以及铁蛋白 - RCA - I仅定位于细胞外质膜表面来判断。然而,如果在22℃进行结合,只有50%的结合凝集素可被乳糖去除,并且铁蛋白 - RCA - I定位于细胞内的内吞小泡中。通过铁蛋白 - RCA - I在22℃诱导其受体聚集的能力,检测了ts3 - PyBHK细胞上RCA - I受体的相对流动性。允许生长的ts3 - PyBHK细胞上的RCA - I受体似乎比非允许生长的细胞上的更具流动性。用神经氨酸酶处理BHK和PyBHK细胞,然后检测所得酶处理细胞的凝集素凝集性以及RCA - I、伴刀豆球蛋白A和麦胚凝集素的定量结合。神经氨酸酶处理导致伴刀豆球蛋白A和麦胚凝集性降低,而RCA - I凝集性略有增加。酶处理的BHK和PyBHK细胞结合较少(125I)麦胚凝集素(分别为2.8×10^6和2.2×10^6个位点/细胞),而(125I)RCA - I结合量分别增加2.5倍和6.2倍(2.5 - 3×10^7和3.5 - 4×10^7个位点/细胞)。神经氨酸酶处理后伴刀豆球蛋白A结合位点数量没有变化。RCA - I结合位点增加量近似于麦胚凝集素结合位点减少量,表明这些细胞上唾液酸的主要倒数第二个寡糖残基是D - 半乳糖。
