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Binding Properties and Proliferative Effects of Human Recombinant Granulocyte‐Macrophage Colony‐stimulating Factor in Primary Leukemia and Lymphoma

机译:人重组粒细胞-巨噬细胞集落刺激因子在原发性白血病和淋巴瘤中的结合特性和增殖作用

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摘要

Binding of radiolabeled human granulocyte‐macrophage colony‐stimulating factor (GM‐CSF) was studied with blast cells front eight patients with acute myeloblastic leukemia (AML), and neoplastic lymphoid cells from one patient with acute lymphoblastic leukemia (ALL), two patients with chronic lymphocytic leukemia (CLL) and one patient with undiagnosed B cell neoplasia. In all AML cases studied, Scatchard graphs of the direct binding data were curvilinear, and were best fitted by curves derived from a two‐binding‐site model; one site with high affinity (Kd1= 12–71 pM; 174–602 sites/cell) and the other with low affinity (Kd2= 0.5–2,7 nM; 1137–6020 sites/cell). A cross‐linking study on blast cells from one AML patient demonstrated specific bands which were similar to those reported for peripheral blood neutrophils. Furthermore, blast colony assays for the same preparations showed remarkable proliferative response to GM‐CSF in the concentration range from 0.3 nM to 7.0 nM (ED50 >0.7 nM). This concentration range is approximately one order of magnitude higher than that which is effective for colony formation from normal bone marrow progenitors (ED50= 0.l nM). No significant correlation could be observed between the responsiveness of blast progenitors to GM‐CSF, and the numbers or affinities of GM‐CSF binding sites demonstrated on blast cells. In studies with neoplastic lymphoid cells from four patients, 125I‐GM‐CSF also specifically bound in two cases, while response to GM‐CSF was not observed in these cases. These results indicate that the expression of GM‐CSF receptor is not restricted to the GM‐CSF‐responsive AML blast cells, but can be observed in other AML blast cells and even in neoplastic lymphoid cells.
机译:研究了放射性标记的人类粒细胞-巨噬细胞集落刺激因子(GM-CSF)的结合,前8名患者患有急性粒细胞白血病(AML),其中1名患有急性淋巴细胞白血病(ALL),2名患有慢性淋巴细胞性白血病(CLL)和一名未确诊的B细胞瘤形成的患者。在所有研究过的AML案例中,直接结合数据的Scatchard图都是曲线的,最好是由两个结合位点模型得出的曲线拟合。一个站点具有高亲和力(Kd1 = 12–71 pM; 174–602个位点/细胞),另一个站点具有低亲和力(Kd2 = 0.5–2.7nM; 1137–6020个位点/细胞)。对一名AML患者的原始细胞进行的交联研究表明,特定的条带与报道的外周血中性粒细胞的条带相似。此外,相同制剂的原始菌落试验在浓度范围为0.3 nM至7.0 nM(ED50> 0.7 nM)时显示出对GM-CSF的显着增殖反应。该浓度范围比对于从正常骨髓祖细胞形成菌落有效的浓度范围高约一个数量级(ED 50 = 0.1nM)。爆炸祖细胞对GM-CSF的反应性与在爆炸细胞上显示的GM-CSF结合位点的数量或亲和力之间没有显着相关性。在来自四名患者的肿瘤性淋巴样细胞的研究中, 125 I-GM-CSF也特异性结合在两例患者中,而在这些病例中未观察到对GM-CSF的反应。这些结果表明GM-CSF受体的表达不仅限于GM-CSF反应性AML原始细胞,而且可以在其他AML原始细胞甚至肿瘤性淋巴样细胞中观察到。

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