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HL60细胞向单核细胞分化过程中磷酸化蛋白的变化:多种蛋白激酶参与的证据

Changes in phosphoproteins during commitment of HL60 cells to monocyte differentiation: evidence for multiple protein kinase involvement.

作者信息

Lord J M, Wong A K, Brown G

机构信息

Department of Immunology, Medical School, University of Birmingham, Edgbaston, UK.

出版信息

Exp Hematol. 1988 Aug;16(7):620-6.

PMID:3164685
Abstract

The human promyeloid cell line HL60 differentiates toward monocytes when treated with TPA. We have analyzed, by two-dimensional gel electrophoresis, the phosphoprotein patterns within HL60 cells, labeled to equilibrium with [32P]orthophosphate when cells were treated with suboptimal (1 nM), optimal (5 and 10 nM), and supraoptimal (40 and 100 nM) concentrations of 12-O-tetradecanylphorbol-13-acetate (TPA) as regards the induction of differentiation. No change was detected in the phosphoprotein pattern at 1 nM TPA, whereas four phosphoproteins showed increased levels of phosphorylation at 5 and 10 nM TPA. When cells were treated with 40 and 100 nM TPA, in total eight and ten proteins, respectively, were phosphorylated, including the above four proteins. Two proteins were dephosphorylated when cells were treated with 40 and 100 nM TPA. A 15-kd protein, phosphorylated when HL60 cells were treated with 5 nM TPA, was observed as an intense spot in autoradiographs of total cellular phosphoproteins of two variant HL60 cell lines that are unable to differentiate toward monocytes and prior to treatment with TPA. In the case of three variant cell lines, which like HL60 differentiate toward monocytes, the phosphoprotein spot was almost absent. Thus, paradoxically, the 15-kd phosphoprotein is affected by TPA although its constitutive level of expression or increased phosphorylation state is inversely related to the potential for monocyte differentiation. This observation, together with the TPA dose-response effects on protein phosphorylation, is discussed in relation to multiple protein kinase involvement.

摘要

人早幼粒细胞系HL60在用佛波酯(TPA)处理时会向单核细胞分化。我们通过二维凝胶电泳分析了HL60细胞内的磷蛋白模式,当用次优浓度(1 nM)、最佳浓度(5和10 nM)以及超最佳浓度(40和100 nM)的12 - O - 十四烷酰佛波醇 - 13 - 乙酸酯(TPA)处理细胞以诱导分化时,细胞用[32P]正磷酸盐标记至平衡状态。在1 nM TPA处理时未检测到磷蛋白模式的变化,而在5和10 nM TPA处理时,有四种磷蛋白显示磷酸化水平增加。当细胞用40和100 nM TPA处理时,分别共有八种和十种蛋白质发生磷酸化,包括上述四种蛋白质。当细胞用40和100 nM TPA处理时,有两种蛋白质发生去磷酸化。一种15 kd的蛋白质,在HL60细胞用5 nM TPA处理时发生磷酸化,在两种不能向单核细胞分化且在TPA处理前的HL60变异细胞系的总细胞磷蛋白放射自显影片中表现为一个强烈的斑点。对于三种像HL60一样能向单核细胞分化的变异细胞系,磷蛋白斑点几乎不存在。因此,矛盾的是,15 kd的磷蛋白受TPA影响,尽管其组成型表达水平或磷酸化状态的增加与单核细胞分化的潜能呈负相关。结合多种蛋白激酶的参与,对这一观察结果以及TPA对蛋白质磷酸化的剂量反应效应进行了讨论。

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