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人类腺苷脱氨酶基因第一个内含子中存在复杂调控序列的证据。

Evidence for a complex regulatory array in the first intron of the human adenosine deaminase gene.

作者信息

Aronow B, Lattier D, Silbiger R, Dusing M, Hutton J, Jones G, Stock J, McNeish J, Potter S, Witte D

机构信息

Division of Basic Science Research, Children's Hospital Medical Center, Cincinnati, Ohio.

出版信息

Genes Dev. 1989 Sep;3(9):1384-400. doi: 10.1101/gad.3.9.1384.

DOI:10.1101/gad.3.9.1384
PMID:2606352
Abstract

Adenosine deaminase (ADA) is expressed ubiquitously by diverse mammalian cells and tissues but at levels that vary according to tissue and species. In humans, the thymus exhibits levels of the enzyme up to 100-fold higher than most other tissues. Using transgenic mice, we identified human ADA gene regulatory domains. Up to 3.7 kb of 5'-flanking and first exon DNA from the human ADA gene failed to promote the expression of a chloramphenicol acetyl transferase (CAT) reporter gene in an efficient, reproducible, or tissue-appropriate manner in transgenic mice. However, when 12.8 kb of DNA from the first intron of the human ADA gene was placed 3' of CAT-coding and -processing sequences, transgenic mice reproducibly expressed CAT activity in most tissues, with profoundly high levels in the thymus. DNase I hypersensitivity studies demonstrated that among transgenic mouse tissues, human thymus, and a variety of human cell lines, a region of the intron 4-10 kb downstream of the first exon exhibited an array of hypersensitive sites that varied according to tissue and cell type. Deletion of this region from the gene construction eliminated high-level expression in transgenic mice. In transfection-transient expression assays, the 12.8-kb intron fragment exhibited enhancer activity in several cell types. A 1.3-kb fragment encompassing two of the hypersensitive sites exhibited some of these activities. The results of these studies suggest that the diverse pattern of human ADA gene expression is determined, in part, by a cluster of cis-regulatory elements contained within its large first intron.

摘要

腺苷脱氨酶(ADA)在多种哺乳动物细胞和组织中普遍表达,但其表达水平因组织和物种而异。在人类中,胸腺中该酶的水平比大多数其他组织高100倍。利用转基因小鼠,我们鉴定出了人类ADA基因的调控区域。来自人类ADA基因的长达3.7 kb的5'侧翼和第一个外显子DNA未能在转基因小鼠中以高效、可重复或组织特异性的方式促进氯霉素乙酰转移酶(CAT)报告基因的表达。然而,当将来自人类ADA基因第一个内含子的12.8 kb DNA置于CAT编码和加工序列的3'端时,转基因小鼠在大多数组织中可重复表达CAT活性,在胸腺中的表达水平极高。DNase I超敏性研究表明,在转基因小鼠组织、人类胸腺和多种人类细胞系中,第一个外显子下游4 - 10 kb的内含子区域表现出一系列根据组织和细胞类型而变化的超敏位点。从基因构建中删除该区域消除了转基因小鼠中的高水平表达。在转染-瞬时表达试验中,12.8 kb的内含子片段在几种细胞类型中表现出增强子活性。一个包含两个超敏位点的1.3 kb片段表现出其中一些活性。这些研究结果表明,人类ADA基因表达的多样化模式部分由其大的第一个内含子中包含的一组顺式调控元件决定。

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Genes Dev. 1989 Sep;3(9):1384-400. doi: 10.1101/gad.3.9.1384.
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