Atkinson J P, Jones E A
J Clin Invest. 1984 Nov;74(5):1649-57. doi: 10.1172/JCI111581.
The C3b receptor (C3bR) of the human promyelocytic leukemia cell line (HL-60) was induced by incubating these cells with dimethylsulfoxide (DMSO) or retinoic acid. A majority of differentiated (DMSO- or retinoic acid-treated) but not undifferentiated cells formed rosettes with C3b-coated erythrocytes and were morphologically mature granulocytes. HL-60 cells were surface- or biosynthetically labeled and then solubilized in 1% Nonidet P-40 in the presence of multiple protease inhibitors. The C3bR was isolated either by immunoprecipitation with anti-C3bR antibodies or by affinity chromatography with hemolytically inactive components in which the internal thioester bond within the alpha-chain was cleaved (iC3)- or iC4-Sepharose. Autoradiographs of NaDodSO4-polyacrylamide gels indicated that the surface-labeled C3bR on the differentiated cells had an Mr of 210,000 (nonreduced) or 240,000 (reducing conditions). The bulk (approximately 85%) of the radiolabeled material that was isolated from biosynthetically labeled cells co-migrated with the surface-labeled band. A small fraction (approximately 15%) of the biosynthetically labeled material that was isolated by affinity chromatography or immunoprecipitation had an Mr of 188,000, which did not correspond to any surface-labeled band. This putative precursor molecule was characterized by pulse-chase experiments and by analysis of its carbohydrate. In pulse-chase (15-min pulse) studies of differentiated cells, only the 188,000-mol wt molecule was detected at 0 h. By 2 h, greater than 80% of counts had chased from the 188,000 to the 210,000-mol wt molecule. Treatment of these two molecules with endoglycosidases indicated that the 188,000-mol wt molecule possessed high mannose oligosaccharides, while the mature C3bR had complex oligosaccharides. We conclude from these data that the 188,000-mol wt molecule is a precursor of the C3b receptor of HL-60 cells. Other experiments indicated that the half-maximal time for newly synthesized receptor to attain an Mr of 210,000 was 45 min, and that the t1/2 for the disappearance of the receptor on the surface of differentiated HL-60 cells in tissue culture was approximately 10 h. The ability to observe the induction of the C3b receptor as the HL-60 cell line differentiates is an instructive model system to study the biosynthesis of a human integral membrane receptor glycoprotein.
人早幼粒细胞白血病细胞系(HL - 60)的C3b受体(C3bR)可通过将这些细胞与二甲基亚砜(DMSO)或视黄酸孵育来诱导。大多数分化的(经DMSO或视黄酸处理的)而非未分化的细胞与C3b包被的红细胞形成花环,并且在形态上是成熟的粒细胞。HL - 60细胞进行表面标记或生物合成标记,然后在多种蛋白酶抑制剂存在的情况下用1% Nonidet P - 40溶解。C3bR可通过用抗C3bR抗体进行免疫沉淀或用α链内硫酯键被裂解的溶血无活性成分(iC3)或iC4 - 琼脂糖进行亲和层析来分离。十二烷基硫酸钠 - 聚丙烯酰胺凝胶的放射自显影片表明,分化细胞上表面标记的C3bR在非还原条件下Mr为210,000,在还原条件下为240,000。从生物合成标记细胞中分离出的大部分(约85%)放射性标记物质与表面标记条带共迁移。通过亲和层析或免疫沉淀分离出的一小部分(约15%)生物合成标记物质的Mr为188,000,它与任何表面标记条带都不对应。这个假定的前体分子通过脉冲追踪实验及其碳水化合物分析来表征。在分化细胞的脉冲追踪(15分钟脉冲)研究中,在0小时仅检测到188,000道尔顿分子量的分子。到2小时时,超过80%的计数已从188,000道尔顿分子量的分子追踪到210,000道尔顿分子量的分子。用内切糖苷酶处理这两种分子表明,188,000道尔顿分子量的分子具有高甘露糖寡糖,而成熟的C3bR具有复杂寡糖。从这些数据我们得出结论,188,000道尔顿分子量的分子是HL - 60细胞C3b受体的前体。其他实验表明,新合成的受体达到210,000道尔顿分子量的半数最大时间为45分钟,并且在组织培养中分化的HL - 60细胞表面受体消失的半衰期约为10小时。观察HL - 60细胞系分化过程中C3b受体的诱导情况,是研究人整合膜受体糖蛋白生物合成的一个有启发性的模型系统。
Zotero 插件
