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Role of transferrin, Fe, and transferrin receptors in myeloid leukemia cell growth. Studies with an antitransferrin receptor monoclonal antibody.

机译:转铁蛋白,铁和转铁蛋白受体在髓样白血病细胞生长中的作用。用抗转铁蛋白受体单克隆抗体进行研究。

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摘要

In previous studies, antitransferrin receptor antibody 42/6 inhibited growth of normal granulocyte/macrophage progenitors and some malignant myeloid cells. In these studies, leukemia cell lines cultured without serum and fresh leukemia cells were used to investigate the roles of Fe, transferrin receptors, and transferrin in leukemia cell growth, and mechanisms of 42/6 inhibition and resistance. HL60 and KG-1 leukemia cells grown in serum-free medium were inhibited by 42/6. In contrast to results in fetal calf serum (FCS), soluble Fe (ferric nitriloacetate) reversed 42/6 growth inhibition of serum-free HL60 cells. When HL60 cells were adapted for growth in serum-free, transferrin-free medium, they became refractory to 42/6 growth inhibition. By using radiolabeled transferrin and 42/6, HL60 cells cultured in FCS and transferrin displayed similar quantities of transferrin receptors (29,000-30,000/cell) and similar Kd's (3.8-4.9 X 10(-9) M). Cells grown in transferrin-free medium showed a similar Kd (3.1 X 10(-9) M), but fewer transferrin binding sites (5,000/cell). Transferrin-independent cells contained a log higher concentration of intracellular ferritin. For both FCS and serum-free HL60 cells, calculated affinities for 42/6 were lower (5.7-10.0 X 10(-9) M), but the number of binding sites was three- to fourfold higher. To investigate further the relationship between receptor display and antibody inhibition in proliferating normal and malignant myeloid cells, simultaneous immunofluorescence was used to determine the cell cycle status of transferrin receptor-positive cells. Malignant cells in S + G2/M displayed approximately 50% of the amount of transferrin receptors detected in normal dividing colony-stimulating factor-stimulated marrow cells. Receptor display by dividing cells from two patients with acute nonlymphocytic leukemia was variable. When HL60 cells were exposed to dimethyl sulfoxide, transferrin receptor display decreased, and 42/6 growth inhibition was abrogated or greatly diminished. The presence of 42/6 did not prevent dimethyl sulfoxide-induced HL60 differentiation in serum-containing or serum-free cultures. We conclude that human leukemia cells require Fe for growth and that 42/6 inhibits transferrin-dependent cells by Fe deprivation. Some dividing normal and differentiating malignant cells display reduced transferrin receptors, and can also escape antibody inhibition. The increased ferritin levels and decreased transferrin receptors in transferrin-independent HL60 cells confirm the inverse relationship between cell ferritin content and transferrin receptor display. These studies indicate a critical role for Fe in leukemia cell growth and possible roles in cellular differentiation.
机译:在以前的研究中,抗运铁蛋白受体抗体42/6抑制正常粒细胞/巨噬细胞祖细胞和某些恶性骨髓细胞的生长。在这些研究中,未培养血清和新鲜白血病细胞的白血病细胞系用于研究Fe,转铁蛋白受体和转铁蛋白在白血病细胞生长中的作用,以及42/6抑制和耐药机制。在无血清培养基中生长的HL60和KG-1白血病细胞被42/6抑制。与胎牛血清(FCS)的结果相反,可溶性Fe(次氮基乙酸铁)逆转了无血清HL60细胞对42/6生长的抑制作用。当HL60细胞适合在无血清,无转铁蛋白的培养基中生长时,它们对42/6的生长抑制作用变得难以抵抗。通过使用放射性标记的运铁蛋白和42/6,在FCS和运铁蛋白中培养的HL60细胞显示出相似数量的运铁蛋白受体(29,000-30,000 /细胞)和相似的Kd(3.8-4.9 X 10(-9)M)。在无转铁蛋白的培养基中生长的细胞显示出相似的Kd(3.1 X 10(-9)M),但转铁蛋白结合位点较少(5,000 /细胞)。不依赖转铁蛋白的细胞中含有较高浓度的细胞内铁蛋白。对于FCS和无血清HL60细胞,计算得出的42/6亲和力较低(5.7-10.0 X 10(-9)M),但结合位点的数量则高三至四倍。为了进一步研究在正常和恶性骨髓细胞中受体展示与抗体抑制之间的关系,同时免疫荧光用于确定转铁蛋白受体阳性细胞的细胞周期状态。 S + G2 / M中的恶性细胞显示出正常分裂菌落刺激因子刺激的骨髓细胞中检测到的转铁蛋白受体量的大约50%。通过分裂来自两个急性非淋巴细胞性白血病患者的细胞的受体展示是可变的。当HL60细胞暴露于二甲基亚砜时,转铁蛋白受体的展示减少,并且42/6的生长抑制作用被消除或大大降低。 42/6的存在不能阻止二甲基亚砜诱导的HL60在含血清或无血清培养物中的分化。我们得出的结论是,人类白血病细胞需要Fe才能生长,而42/6通过Fe剥夺抑制转铁蛋白依赖性细胞。一些分裂的正常和分化中的恶性细胞显示出降低的转铁蛋白受体,并且还可以逃避抗体的抑制。在不依赖转铁蛋白的HL60细胞中,铁蛋白水平的增加和转铁蛋白受体的减少证实了细胞铁蛋白含量与转铁蛋白受体展示之间的反比关系。这些研究表明Fe在白血病细胞生长中的关键作用以及在细胞分化中的可能作用。

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