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鉴定一种新型增强子元件,其介导在表皮生长因子或蛋白激酶C激活后基因表达的钙依赖性诱导。

Identification of a novel enhancer element mediating calcium-dependent induction of gene expression in response to either epidermal growth factor or activation of protein kinase C.

作者信息

Lenormand P, Pribnow D, Rodland K D, Magun B E

机构信息

Centre de Biochimie, Université de Nice, 06034 France.

出版信息

Mol Cell Biol. 1992 Jun;12(6):2793-803. doi: 10.1128/mcb.12.6.2793-2803.1992.

DOI:10.1128/mcb.12.6.2793-2803.1992
PMID:1588971
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC364474/
Abstract

The VL30 family of defective murine retroviruses consists of 100 to 200 members, of which fewer than 5% appear to be transcriptionally active. A genomic clone of the transcriptionally active VL30 element RVL-3 was identified and sequenced. Genetic analysis indicated that a triple-repeat sequence within the RVL-3 long terminal repeat is capable of functioning as an inducible enhancer element responding to a variety of agonists. In Rat-1 fibroblasts, the ability of the RVL-3 enhancer to mediate induction of gene expression from a heterologous promoter in response to either epidermal growth factor (EGF) or phorbol ester treatment required coelevation of intracellular calcium. Two CArG boxes present in the triple-repeat sequence appeared to exert a negative effect on gene expression, as mutation of these sequences elevated the basal level of expression observed without altering the fold induction in response to either EGF or protein kinase C activation. In the presence of these CArG elements, mutation of AP-1-like sites adjacent to the CArG elements significantly inhibited the ability of either EGF or phorbol esters to induce gene expression. The effect of mutating these AP-1-like sites was relieved by simultaneous mutation of the CArG sites, indicating that interactions among these sites modulate RVL-3 expression. Mutational analysis and gel mobility shift experiments have identified a third sequence within the VL30 triple-repeat element that is required for the induction of gene expression and serves as a binding site for nuclear proteins. Sequence comparisons indicate that this enhancer element has not been described previously.

摘要

有缺陷的鼠逆转录病毒VL30家族由100至200个成员组成,其中转录活跃的成员不到5%。已鉴定并测序了转录活跃的VL30元件RVL-3的基因组克隆。遗传分析表明,RVL-3长末端重复序列中的一个三重复序列能够作为一个可诱导的增强子元件,对多种激动剂作出反应。在大鼠-1成纤维细胞中,RVL-3增强子介导异源启动子基因表达诱导以响应表皮生长因子(EGF)或佛波酯处理的能力需要细胞内钙的共同升高。三重复序列中存在的两个CArG框似乎对基因表达产生负面影响,因为这些序列的突变提高了在不改变对EGF或蛋白激酶C激活的诱导倍数的情况下观察到的基础表达水平。在这些CArG元件存在的情况下,CArG元件附近的AP-1样位点的突变显著抑制了EGF或佛波酯诱导基因表达的能力。这些AP-1样位点突变的影响通过CArG位点的同时突变而得到缓解,表明这些位点之间的相互作用调节RVL-3的表达。突变分析和凝胶迁移率变动实验已经确定了VL30三重复元件内的第三个序列,该序列是基因表达诱导所必需的,并且作为核蛋白的结合位点。序列比较表明,这种增强子元件以前尚未被描述过。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4f3e/364474/e2829d9f9628/molcellb00028-0356-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4f3e/364474/2eed3780549f/molcellb00028-0355-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4f3e/364474/e2829d9f9628/molcellb00028-0356-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4f3e/364474/2eed3780549f/molcellb00028-0355-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4f3e/364474/e2829d9f9628/molcellb00028-0356-a.jpg

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