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Regulation of estrogen receptor alpha gene mediated by promoter B responsible for its enhanced expressionin human breast cancer.

机译:启动子B介导的雌激素受体α基因的调控导致其在人乳腺癌中的表达增强。

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摘要

We have previously reported that transcription from a distal promoter (promoter B) of the estrogen receptor alpha (ERalpha) gene is responsible for the increased expression of ERalpha in human breast carcinomas. This paper first characterized the promoter B region in terms of transient transfection experiments with luciferase using MCF-7 cells. Gradual deletions from the 5'-end of promoter B resulted in a decrease in promoter activity corresponding to the deleted lengths; a deletion of 39 bp in a non-coding exon 1a, drastically diminished the activity, indicating existence of an important cis -element. Furthermore, electrophoretic mobility shift assay and subsequent mutational analysis indicated that this element containing nucleotide sequence CTGGAAAG forms a specific DNA-protein complex. This element was capable of transactivating a heterogeneous SV40 promoter in MCF-7 cells, confirming that the element is a transcriptional enhancer; the trans -acting factor binding to the element was named ERBF-1 (estrogen receptor promoter B associated factor-1). The ERBF-1 was exclusively expressed in those cells expressing ERalpha mRNA transcribed from promoter B. Our findings indicate that ERBF-1 plays an important role in the expression of the ERalpha gene transcribed from promoter B, which is selectively utilized in breast cancer.
机译:我们以前曾报道过,从雌激素受体α(ERalpha)基因的远端启动子(启动子B)转录是导致人乳腺癌中ERalpha表达增加的原因。本文首先通过使用MCF-7细胞的荧光素酶瞬时转染实验来表征启动子B区。从启动子B的5'末端逐渐缺失导致与缺失的长度相对应的启动子活性的降低。在非编码外显子1a中39bp的缺失大大降低了活性,表明存在重要的顺式元件。此外,电泳迁移率变动分析和随后的突变分析表明,该含有核苷酸序列CTGGAAAG的元件形成了特定的DNA-蛋白质复合物。该元件能够在MCF-7细胞中激活异质SV40启动子,从而证实该元件是转录增强子。与该元素结合的反式作用因子称为ERBF-1(雌激素受体启动子B相关因子-1)。 ERBF-1仅在表达从启动子B转录的ERalpha mRNA的细胞中表达。我们的发现表明ERBF-1在从启动子B转录的ERalpha基因的表达中起重要作用,该基因被选择性地用于乳腺癌。

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