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用激活的c-myc转染成纤维细胞可赋予其对干扰素抗生长作用的抗性。

Transfection of fibroblasts with activated c-myc confers resistance to antigrowth effects of interferon.

作者信息

Einat M, Kimchi A

机构信息

Department of Virology, Weizmann Institute of Science, Rehovot, Israel.

出版信息

Oncogene. 1988 May;2(5):485-91.

PMID:2453829
Abstract

The Go/G1 to S transition in growth factor-stimulated Balb/c 3T3 fibroblasts is efficiently blocked by interferons (IFNs). In the present communication we studied whether deregulated expression of exogenously introduced c-myc changes the growth sensitivity to type I IFNs (alpha + beta). Constructs that link the two coding exons of c-myc to the long terminal repeat (LTR) of Ha-MS virus were introduced into the 3T3 fibroblasts. The steady state levels of exogenous c-myc mRNA in the individual stable clones were 3-10 fold higher than the endogenous mRNA levels in non transfected Balb/c 3T3 cells. The expression directed from the c-myc-construct was found to be completely resistant to inhibition by IFN while it was still partially responsive to addition or depletion of growth factors. To test the possible phenotypic changes after this genetic manipulation, the cell cycle distribution of individual c-myc-transfected clones was analyzed during the growth factor controlled transition from resting phase to proliferating state. We find that entry into S phase of the c-myc-transfected clones became completely resistant to inhibition by low IFN concentrations which blocked this process in the parental cell line and the control clones. It is concluded that deregulated expression of c-myc resulting from substitution of the authentic promoters and the first c-myc exon with a viral promoter reduces the sensitivity of synchronized fibroblasts to the antimitogenic effects of IFN.

摘要

在生长因子刺激的Balb/c 3T3成纤维细胞中,从G0/G1期到S期的转变可被干扰素(IFN)有效阻断。在本通讯中,我们研究了外源性导入的c-myc表达失调是否会改变对I型干扰素(α + β)的生长敏感性。将连接c-myc两个编码外显子与Ha-MS病毒长末端重复序列(LTR)的构建体导入3T3成纤维细胞。各个稳定克隆中外源性c-myc mRNA的稳态水平比未转染的Balb/c 3T3细胞中的内源性mRNA水平高3至10倍。发现由c-myc构建体指导的表达对IFN的抑制作用完全抗性,而对生长因子的添加或去除仍有部分反应。为了测试这种基因操作后可能的表型变化,在生长因子控制的从静止期到增殖状态的转变过程中,分析了各个c-myc转染克隆的细胞周期分布。我们发现,c-myc转染克隆进入S期对低浓度IFN的抑制作用完全抗性,而这种低浓度IFN可阻断亲本细胞系和对照克隆中的这一过程。结论是,用病毒启动子取代真实启动子和第一个c-myc外显子导致的c-myc表达失调降低了同步化成纤维细胞对IFN抗有丝分裂作用的敏感性。

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