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生长因子对增殖期和静止期巨噬细胞中转铁蛋白受体的依赖性调节

Growth factor-dependent regulation of transferrin receptor in proliferating and quiescent macrophages.

作者信息

Lokeshwar B L, Lin H S

机构信息

Division of Radiation Oncology, Mallinckrodt Institute of Radiology, St. Louis, Missouri.

出版信息

Cell Immunol. 1990 Oct 15;130(2):401-15. doi: 10.1016/0008-8749(90)90282-v.

DOI:10.1016/0008-8749(90)90282-v
PMID:2145079
Abstract

Transferrin receptor (TfR) expression in a population of murine macrophages was investigated during the colony-stimulating factor-1 (CSF-1)-induced proliferation and quiescence. Depletion of CSF-1 from the culture medium of bone marrow cell-derived macrophages (BMM) resulted in a simultaneous decrease in the total (cell surface + intracellular) amount of TfR and complete cessation of proliferating activity [( 3H]thymidine incorporation). The addition of CSF-1 to quiescent BMM resulted in a bimodal increase in surface TfR activity. A rapid but transient twofold increase only on the cell surface due to changes in the cycling of TfR was followed by a steady increase of total cellular TfR due to de novo synthesis. A similar transient increase in surface TfR was also induced by another hemopoietic colony-stimulating factor, GM-CSF, which is mitogenic for BMM. IL-3, which did not stimulate the clonal growth of these cells, failed to modulate surface TfR. In contrast to its effect on the cycling rate of TfR in quiescent cells, CSF-1 had little effect on the TfR distribution on proliferating BMM as well as on the J774 cells (a macrophage-like tumor cell line) despite the latter expressing high levels of CSF-1 receptor. This study showed that (i) cell surface modulation by growth factor is a function of state of cellular proliferation, and (ii) rapid changes in the cell surface distribution of TfR result from changes in its cycling rates.

摘要

在集落刺激因子-1(CSF-1)诱导的增殖和静止过程中,研究了一群小鼠巨噬细胞中转铁蛋白受体(TfR)的表达。从骨髓细胞衍生的巨噬细胞(BMM)培养基中去除CSF-1,导致TfR总量(细胞表面+细胞内)同时减少,并且增殖活性([3H]胸苷掺入)完全停止。向静止的BMM中添加CSF-1,导致表面TfR活性出现双峰增加。由于TfR循环的变化,仅在细胞表面迅速但短暂地增加了两倍,随后由于从头合成,细胞内总TfR稳步增加。另一种造血集落刺激因子GM-CSF也诱导了表面TfR的类似短暂增加,GM-CSF对BMM具有促有丝分裂作用。IL-3不刺激这些细胞的克隆生长,也无法调节表面TfR。与它对静止细胞中TfR循环速率的影响相反,尽管J774细胞(一种巨噬细胞样肿瘤细胞系)表达高水平的CSF-1受体,但CSF-1对增殖的BMM以及J774细胞上的TfR分布几乎没有影响。这项研究表明,(i)生长因子对细胞表面的调节是细胞增殖状态的函数,(ii)TfR细胞表面分布的快速变化是其循环速率变化的结果。

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