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干扰素γ对pim-1蛋白激酶基因表达的转录诱导作用以及对与钢因子共刺激的转录后效应。

Transcriptional induction of pim-1 protein kinase gene expression by interferon gamma and posttranscriptional effects on costimulation with steel factor.

作者信息

Yip-Schneider M T, Horie M, Broxmeyer H E

机构信息

Department of Medicine (Hematology/Oncology), Indiana University School of Medicine, Indianapolis 46202-5121, USA.

出版信息

Blood. 1995 Jun 15;85(12):3494-502.

PMID:7540064
Abstract

Steel factor (SLF) synergizes with interferon gamma (IFN gamma) to stimulate proliferation of the human factor-dependent cell line MO7e. We examined the effects of IFN gamma and SLF treatment, alone or in combination, on the expression of a 33-kD cytoplasmic protein serine/threonine kinase designated pim-1 whose expression has been closely associated with proliferation induced by related myeloid cytokines. IFN gamma alone, but not SLF, stimulated expression of pim-1 RNA and protein in MO7e cells; compared with IFN gamma alone, costimulation with IFN gamma and SLF resulted in a twofold to threefold increase in pim-1 message and protein expression, correlating with synergistic effects on cell proliferation. Both IFN gamma and IFN gamma/SLF induced pim-1 mRNA in the absence of de novo protein synthesis. Nuclear run-on assays showed that, although IFN gamma alone increased the rate of pim-1 gene transcription, costimulation with IFN gamma and SLF did not further potentiate this effect; however, the stability of pim-1 message was significantly enhanced in the presence of both cytokines. An IFN gamma-responsive element within the 5' flanking region of the pim-1 gene that could confer IFN gamma responsiveness on a heterologous promoter was identified. This sequence, designated PMGAS, formed a specific complex with Stat (signal transducers and activators of transcription) 1 alpha (the p91 subunit of the transcription factor ISGF3 [interferon-stimulated gene factor 3]) in IFN gamma-treated cell extracts, suggesting that the transcriptional effects of IFN gamma on pim-1 expression may be mediated by Stat 1 alpha.

摘要

Steel因子(SLF)与干扰素γ(IFNγ)协同作用,刺激人因子依赖细胞系MO7e的增殖。我们研究了单独或联合使用IFNγ和SLF处理对一种名为pim-1的33-kD细胞质蛋白丝氨酸/苏氨酸激酶表达的影响,该激酶的表达与相关髓系细胞因子诱导的增殖密切相关。单独的IFNγ而非SLF能刺激MO7e细胞中pim-1 RNA和蛋白的表达;与单独使用IFNγ相比,IFNγ和SLF共同刺激导致pim-1信息和蛋白表达增加两倍至三倍,这与对细胞增殖的协同作用相关。IFNγ和IFNγ/SLF在不存在从头蛋白质合成的情况下均诱导pim-1 mRNA。核转录分析表明,虽然单独的IFNγ增加了pim-1基因的转录速率,但IFNγ和SLF共同刺激并未进一步增强这种作用;然而,在两种细胞因子存在的情况下,pim-1信息的稳定性显著增强。在pim-1基因5'侧翼区域内鉴定出一个IFNγ反应元件,该元件可赋予异源启动子IFNγ反应性。这个序列,命名为PMGAS,在IFNγ处理的细胞提取物中与Stat(信号转导和转录激活因子)1α(转录因子ISGF3 [干扰素刺激基因因子3]的p91亚基)形成特异性复合物,表明IFNγ对pim-1表达的转录作用可能由Stat 1α介导。

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