首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Mobility of Carbohydrate-Containing Structures on the Surfaces Membrane and the Normal Differentiation of Myeloid Leukemic Cells to Macrophages and Granulocytes
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Mobility of Carbohydrate-Containing Structures on the Surfaces Membrane and the Normal Differentiation of Myeloid Leukemic Cells to Macrophages and Granulocytes

机译:表面膜上含碳水化合物的结构的移动性和髓样白血病细胞向巨噬细胞和粒细胞的正常分化

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摘要

Clones (D+) of a cultured line of myeloid leukemic cells can be induced to undergo normal differentiation to mature macrophages and granulocytes. There are also clones derived from the same cell line (D-) that could not be induced to differentiate. The carbohydrate-binding protein concanavalin A was used as a probe to study the mobility of carbohydrate-containing sites on the surface membrane of these cells. Changes in the distribution of concanavalin A binding sites on the surface membrane can be induced by concanavalin A. With the appropriate site mobility, this induction of a new distribution resulted in a concentration of concanavalin A-membrane site complexes on one pole of the cell to form a cap. D+ and D- clones showed 50 and 5% of cells with caps, respectively, although both types of cells bound a similar number of concanavalin A molecules. Treatment of cells with trypsin increased cap formation from 5 to 40% in D- cells, but did not change the percentage of cells with caps in D+ cells. The results show a difference in the mobility of concanavalin A binding sites in these two types of cells and suggest a difference in the fluid state of these carbohydrate-containing structures on the surface membrane. It is suggested that a gain of the ability of myeloid leukemic cells to undergo normal differentiation is associated with an increase in the fluidity of structures on the surface membrane where the concanavalin A sites are located. Differences in fluidity of specific membrane sites may also explain differences in the response of cells to other differentiation-inducing stimuli.
机译:可以诱导培养的髓系白血病细胞系的克隆(D + )正常分化为成熟的巨噬细胞和粒细胞。也有一些衍生自同一细胞系(D -)的克隆无法诱导分化。使用碳水化合物结合蛋白伴刀豆球蛋白A作为探针来研究这些细胞表面膜上含碳水化合物的位点的迁移性。伴刀豆球蛋白A可诱导表面膜上伴刀豆球蛋白A结合位点分布的变化。以适当的位点迁移率,这种新分布的诱导导致伴刀豆球蛋白A-膜位点复合物在细胞的一个极点上富集。形成一个上限。 D + 和D -克隆分别显示50和5%带帽的细胞,尽管两种类型的细胞都结合了相似数量的伴刀豆球蛋白A分子。用胰蛋白酶处理的细胞将D -细胞中的帽形成率从5%增加到40%,但没有改变D + 细胞中具有帽的细胞的百分比。结果表明这两种类型的细胞中伴刀豆球蛋白A结合位点的迁移率存在差异,并且表明这些糖类结构在表面膜上的流体状态也存在差异。提示髓样白血病细胞经历正常分化的能力的增加与伴刀豆球蛋白A位点所在的表面膜上结构的流动性的增加有关。特定膜部位流动性的差异也可以解释细胞对其他分化诱导刺激的反应差异。

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