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首页> 美国卫生研究院文献>Molecular and Cellular Biology >A-myb is expressed in bovine vascular smooth muscle cells during the late G1-to-S phase transition and cooperates with c-myc to mediate progression to S phase.
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A-myb is expressed in bovine vascular smooth muscle cells during the late G1-to-S phase transition and cooperates with c-myc to mediate progression to S phase.

机译:A-myb在G1到S期的晚期过渡过程中在牛血管平滑肌细胞中表达并与c-myc协同作用以介导进展到S期。

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The Myb family of transcription factors is defined by homology within the DNA binding domain and includes c-Myb, A-Myb, and B-Myb. The protein products of the myb genes all bind the Myb-binding site (MBS) [YG(A/G)C(A/C/G)GTT(G/A)]. A-myb has been found to display a limited pattern of expression. Here we report that bovine aortic smooth muscle cells (SMCs) express A-myb. Sequence analysis of isolated bovine A-myb cDNA clones spanning the entire coding region indicated extensive homology with the human gene, including the putative transactivation domain. Expression of A-myb was cell cycle dependent; levels of A-myb RNA increased in the late G1-to-S phase transition following serum stimulation of serum-deprived quiescent SMC cultures and peaked in S phase. Nuclear run-on analysis revealed that an increased rate of transcription can account for most of the increase in A-myb RNA levels. Treatment of SMC cultures with 5,6-dichlorobenzimidazole riboside, a selective inhibitor of RNA polymerase II, indicated an approximate 4-h half-life for A-myb mRNA during the S phase of the cell cycle. Expression of A-myb by SMCs was stimulated by basic fibroblast growth factor, in a cell density-dependent fashion. Cotransfection of a human A-myb expression vector activated a multimerized MBS element-driven reporter construct approximately 30-fold in SMCs. The activity of c-myb and c-myc promoters, which both contain multiple MBS elements, were similarly transactivated, approximately 30- and 50-fold, respectively, upon cotransfection with human A-myb. Lastly, A-myb RNA levels could be increased by a combination of phorbol ester plus insulin-like growth factor 1. To test the role of myb family members in progression through the cell cycle, we comicroinjected c-myc and myb expression vectors into serum-deprived quiescent SMCs. The combination of c-myc and either A-myb or c-myb but not B-myb synergistically led to entry into S phase, whereas microinjection of any vector alone had little effect on S phase entry. Thus, these results suggest that A-myb is a potent transactivator in bovine SMCs and that its expression induces progression into S phase of the cell cycle.
机译:Myb转录因子家族由DNA结合域内的同源性定义,包括c-Myb,A-Myb和B-Myb。 myb基因的蛋白质产物均结合Myb结合位点(MBS)[YG(A / G)C(A / C / G)GTT(G / A)]。已经发现A-myb显示有限的表达模式。在这里,我们报告牛主动脉平滑肌细胞(SMCs)表达A-myb。跨越整个编码区的分离的牛A-myb cDNA克隆的序列分析表明与人基因具有广泛的同源性,包括推定的反式激活结构域。 A-myb的表达是细胞周期依赖性的。在血清刺激缺乏血清的静止SMC培养物后,在G1到S相的晚期转变中,A-myb RNA的水平增加,并在S期达到峰值。核运行分析表明,转录速率的增加可以解释A-myb RNA水平增加的大部分原因。用5,6-二氯苯并咪唑核糖苷(一种RNA聚合酶II的选择性抑制剂)处理SMC培养物,表明在细胞周期的S期,A-myb mRNA的半衰期约为4小时。碱性成纤维细胞生长因子以细胞密度依赖性方式刺激SMCs表达A-myb。人A-myb表达载体的共转染激活了SMC中约30倍的多聚MBS元件驱动的报道基因构建体。与人A-myb共转染后,都包含多个MBS元件的c-myb和c-myc启动子的活性被相似地分别激活,分别约为30倍和50倍。最后,佛波酯加胰岛素样生长因子1可以增加A-myb RNA的水平。为测试myb家族成员在整个细胞周期进程中的作用,我们将c-myc和myb表达载体共注射了血清剥夺的静态SMC。 c-myc与A-myb或c-myb但不是B-myb的组合协同作用导致进入S期,而单独注射任何载体对S期进入几乎没有影响。因此,这些结果表明,A-myb在牛SMC中是有效的反式激活因子,其表达诱导细胞周期进入S期。

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