Alexandropoulos K, Qureshi S A, Rim M, Sukhatme V P, Foster D A
Institute for Biomolecular Structure and Function, Hunter College, City University of New York, NY 10021.
Nucleic Acids Res. 1992 May 11;20(9):2355-9. doi: 10.1093/nar/20.9.2355.
Egr-1, a mitogen-responsive transcription factor, is rapidly induced by v-Fps in the absence of protein synthesis. Thus, Egr-1 is a primary response to the protein-tyrosine kinase activity of v-Fps. To determine the v-Fps-responsive elements in the Egr-1 promoter, deletion mutants of the Egr-1 promoter were used in transient expression assays. A v-Fps expression vector was contransfected into NIH 3T3 cells with chloramphenicol acetyl transferase (CAT) gene expression vectors under the control of the Egr-1 promoter or the Egr-1 promoter containing various deletions. Responsiveness to v-Fps was restricted to a region that contained repeated CC(A/T)6GG sequences, known as CArG boxes. CArG boxes form the core of serum response element (SREs). v-Fps-induced Egr-1 promoter activation was lost by sequential removal of four tandemly repeated SREs. This region, containing four SREs, was found to be sufficient for maximal Egr-1 induction by v-Fps when placed upstream from a heterologous promoter. Individual SREs from this region were able to respond to v-Fps, however, the activation of the individual SREs was lower than that observed for the clustered SREs. These data suggest that v-Fps-responsiveness in the Egr-1 promoter is mediated by SREs.
Egr-1是一种有丝分裂原反应性转录因子,在缺乏蛋白质合成的情况下,它会被v-Fps迅速诱导。因此,Egr-1是对v-Fps蛋白酪氨酸激酶活性的主要反应。为了确定Egr-1启动子中的v-Fps反应元件,在瞬时表达分析中使用了Egr-1启动子的缺失突变体。将一个v-Fps表达载体与在Egr-1启动子或含有各种缺失的Egr-1启动子控制下的氯霉素乙酰转移酶(CAT)基因表达载体共转染到NIH 3T3细胞中。对v-Fps的反应性仅限于一个包含重复的CC(A/T)6GG序列的区域(称为CArG盒)。CArG盒构成血清反应元件(SREs)的核心。通过顺序去除四个串联重复的SREs,v-Fps诱导的Egr-1启动子激活丧失。当置于异源启动子上游时,发现该包含四个SREs的区域足以实现v-Fps对Egr-1的最大诱导。该区域的单个SREs能够对v-Fps作出反应,然而,单个SREs的激活低于成簇SREs所观察到的激活。这些数据表明,Egr-1启动子中的v-Fps反应性是由SREs介导的。
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