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黑腹果蝇乙醇脱氢酶基因幼虫表达所需顺式调控元件的鉴定

Identification of cis-regulatory elements required for larval expression of the Drosophila melanogaster alcohol dehydrogenase gene.

作者信息

Corbin V, Maniatis T

机构信息

Department of Biochemistry and Molecular Biology, Harvard University, Cambridge, Massachusetts 02138.

出版信息

Genetics. 1990 Mar;124(3):637-46. doi: 10.1093/genetics/124.3.637.

Abstract

The Alcohol dehydrogenase (Adh) genes of two distantly related species, Drosophila melanogaster and Drosophila mulleri, display similar, but not identical, patterns of tissue-specific expression in larvae and adults. The regulatory DNA sequences necessary for wild-type Adh expression in D. mulleri larvae were previously reported. In this paper we present an analysis of the DNA sequences necessary for wild-type Adh expression in D. melanogaster larvae. We show that transcription from the proximal promoter of the melanogaster Adh gene is regulated by a far upstream enhancer and two or more elements near the transcription start site. The enhancer is tissue specific and stimulates transcription to high levels in fat body and to lower levels in midgut and malpighian tubules whether linked to the proximal promoter or to a heterologous promoter. The enhancer activity localized to at least two discrete regions dispersed over more than 1.7 kb of DNA. Deletion of any one of these subregions reduces Adh transcription in all three larval tissues. Similarly, two regions immediately upstream of the proximal promoter start site are necessary for wild-type transcription levels in all three tissues. Thus, each of the identified regulatory elements is sufficient for low levels of Adh gene expression in all three larval tissues, but maximal levels of expression requires the entire set.

摘要

两个远缘物种——黑腹果蝇(Drosophila melanogaster)和穆勒果蝇(Drosophila mulleri)的乙醇脱氢酶(Adh)基因,在幼虫和成虫中表现出相似但不完全相同的组织特异性表达模式。先前已报道了穆勒果蝇幼虫中野生型Adh表达所需的调控DNA序列。在本文中,我们对黑腹果蝇幼虫中野生型Adh表达所需的DNA序列进行了分析。我们发现,黑腹果蝇Adh基因近端启动子的转录受一个远上游增强子和转录起始位点附近的两个或更多元件调控。该增强子具有组织特异性,无论与近端启动子相连还是与异源启动子相连,都能在脂肪体中刺激转录至高水平,而在中肠和马氏管中刺激转录至较低水平。增强子活性定位于分散在超过1.7 kb DNA上的至少两个离散区域。删除这些亚区域中的任何一个都会降低所有三种幼虫组织中的Adh转录。同样,近端启动子起始位点上游紧邻的两个区域对于所有三种组织中的野生型转录水平是必需的。因此,每个已鉴定的调控元件足以在所有三种幼虫组织中实现低水平的Adh基因表达,但最大表达水平需要整套元件。

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