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分化中的ML-1人髓系白血病细胞中c-myc蛋白的胞质/核分布改变。

Altered cytoplasmic/nuclear distribution of the c-myc protein in differentiating ML-1 human myeloid leukemia cells.

作者信息

Craig R W, Buchan H L, Civin C I, Kastan M B

机构信息

Department of Physiology, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205.

出版信息

Cell Growth Differ. 1993 May;4(5):349-57.

PMID:8518229
Abstract

The c-myc gene is thought to play a role in cell proliferation and differentiation; for example, constitutive expression of an exogenously introduced c-myc gene can inhibit differentiation in hematopoietic cell lines. Expression of the endogenous c-myc gene has now been monitored during the differentiation, and associated loss of proliferation, of ML-1 human myeloblastic leukemia cells: c-myc mRNA remains detectable, at decreased levels, during differentiation along the monocyte/macrophage pathway induced with 12-O-tetradecanoylphorbol-13-acetate. c-myc protein also remains present, at undiminished levels, in mature, nonproliferative cells (assessed by immunoblotting and flow cytometry). The protein is, however, readily detectable in the cytoplasm of 12-O-tetradecanoylphorbol-13-acetate-induced cells, and some of this cytoplasmic c-myc exhibits a shift in electrophoretic mobility compared to the predominantly nuclear c-myc in uninduced cells. Furthermore, although c-myc protein continues to be synthesized in the mature cells (assessed by metabolic labeling/immunoprecipitation), loss of the protein from the cytoplasm and accumulation in the nucleus are slowed (assessed by pulse-chase metabolic labeling). These findings suggest that, during the 12-O-tetradecanoylphorbol-13-acetate-induced differentiation and loss of proliferation of ML-1 cells, c-myc protein is regulated through alterations that affect its cytoplasmic/nuclear distribution rather than its total cellular content.

摘要

c-myc基因被认为在细胞增殖和分化中发挥作用;例如,外源性导入的c-myc基因的组成型表达可抑制造血细胞系的分化。现已监测了内源性c-myc基因在ML-1人髓母细胞白血病细胞分化及相关增殖丧失过程中的表达情况:在用12-O-十四烷酰佛波醇-13-乙酸酯诱导的沿单核细胞/巨噬细胞途径分化过程中,c-myc mRNA仍可检测到,但其水平降低。c-myc蛋白在成熟的、非增殖细胞中(通过免疫印迹和流式细胞术评估)也仍然存在,且水平未降低。然而,在12-O-十四烷酰佛波醇-13-乙酸酯诱导的细胞胞质中可轻易检测到该蛋白,与未诱导细胞中主要位于细胞核的c-myc相比,部分胞质c-myc的电泳迁移率发生了改变。此外,尽管c-myc蛋白在成熟细胞中仍持续合成(通过代谢标记/免疫沉淀评估),但其从胞质中的丧失和在细胞核中的积累速度减慢(通过脉冲追踪代谢标记评估)。这些发现表明,在12-O-十四烷酰佛波醇-13-乙酸酯诱导的ML-1细胞分化及增殖丧失过程中,c-myc蛋白是通过影响其胞质/核分布而非其总细胞含量的改变来进行调控的。

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