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位于第一个内含子中的一个E盒元件介导c-myc对前胸腺素α基因的调控。

An E-box element localized in the first intron mediates regulation of the prothymosin alpha gene by c-myc.

作者信息

Gaubatz S, Meichle A, Eilers M

机构信息

Zentrum für Molekulare Biologie Heidelberg, Federal Republic of Germany.

出版信息

Mol Cell Biol. 1994 Jun;14(6):3853-62. doi: 10.1128/mcb.14.6.3853-3862.1994.

Abstract

In RAT1A fibroblasts, expression of the prothymosin alpha gene is under the transcriptional control of the c-myc proto-oncogene. We have now cloned the rat gene encoding prothymosin alpha and show that the cloned gene is regulated by c-myc in vivo. We find that regulation by c-myc is mediated by sequences downstream of the transcriptional start site, whereas the promoter is constitutive and not regulated by c-myc. We have identified an enhancer element within the first intron that is sufficient to mediate a response to Myc and Max in transient transfection assays and to activation of estrogen receptor-Myc chimeras in vivo. We find that this element contains a consensus Myc-binding site (CACGTG). Disruption of this site abolishes the response to Myc and Max in both transient and stable assays. Mutants of either Myc or Max that are deficient for heterodimerization fail to regulate the prothymosin alpha gene, suggesting that a heterodimer between Myc and Max activates the prothymosin alpha gene. Our data define the prothymosin alpha gene as a bona fide target gene for c-myc.

摘要

在RAT1A成纤维细胞中,前胸腺素α基因的表达受原癌基因c-myc的转录调控。我们现已克隆出编码前胸腺素α的大鼠基因,并证明该克隆基因在体内受c-myc调控。我们发现,c-myc的调控是由转录起始位点下游的序列介导的,而启动子是组成型的,不受c-myc调控。我们在第一个内含子中鉴定出一个增强子元件,该元件在瞬时转染实验中足以介导对Myc和Max的应答,并在体内介导雌激素受体-Myc嵌合体的激活。我们发现该元件含有一个共有Myc结合位点(CACGTG)。在瞬时和稳定实验中,该位点的破坏均消除了对Myc和Max 的应答。不能进行异源二聚化的Myc或Max突变体无法调控前胸腺素α基因,这表明Myc和Max之间的异源二聚体激活了前胸腺素α基因。我们的数据将前胸腺素α基因定义为c-myc真正的靶基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1d66/358752/07881c092afa/molcellb00006-0336-a.jpg

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