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人类5-脂氧合酶激活蛋白(FLAP)的基因特征与启动子分析

Gene characterization and promoter analysis of the human 5-lipoxygenase-activating protein (FLAP).

作者信息

Kennedy B P, Diehl R E, Boie Y, Adam M, Dixon R A

机构信息

Department of Molecular Biology, Merck Frosst Center for Therapeutic Research, Pointe Claire-Dorval, Quebec, Canada.

出版信息

J Biol Chem. 1991 May 5;266(13):8511-6.

PMID:1673682
Abstract

The human gene for the recently identified 5-lipoxy-genase-activating protein (FLAP) has been cloned. The gene was isolated from two different genomic libraries and is contained within four overlapping bacteriophage clones. The gene spans greater than 31 kilobases and consists of five small exons and four large introns. Southern blot analysis of human genomic DNA suggests the presence of a single FLAP gene per haploid genome. A restriction site polymorphism was identified in intron II of the gene. This restriction fragment length polymorphism appears to be present in the normal population at a fairly high frequency. The transcription initiation site was located, at an adenine residue, 74 base pairs upstream of the ATG initiation codon. Examination of the sequence of the gene 5' to the mRNA start site revealed the presence of a possible TATA box (TGTAAT) 22 base pairs upstream and potential AP-2 and glucocorticoid receptor binding sites. Functional analysis of the FLAP gene promoter was assayed by transient transfection of mouse P388D1 cells (macrophage) and human HepG2 cells (hepatoma) with 5'-flanking sequences of the FLAP gene fused upstream of the chloramphenicol acetyltransferase reporter gene. Expression in the mouse macrophage cell line of the various FLAP gene promoter constructs revealed both tissue specificity and enhancer-like activities whereas in the hepatoma cell line only a minimum level of activity was obtained.

摘要

最近发现的5-脂氧合酶激活蛋白(FLAP)的人类基因已被克隆。该基因是从两个不同的基因组文库中分离出来的,包含在四个重叠的噬菌体克隆中。该基因跨度超过31千碱基,由五个小外显子和四个大内含子组成。对人类基因组DNA的Southern印迹分析表明,单倍体基因组中存在单个FLAP基因。在该基因的内含子II中鉴定出一个限制性位点多态性。这种限制性片段长度多态性在正常人群中似乎以相当高的频率存在。转录起始位点位于ATG起始密码子上游74个碱基对处的一个腺嘌呤残基处。对基因5'端至mRNA起始位点序列的检查发现,在其上游22个碱基对处存在一个可能的TATA盒(TGTAAT)以及潜在的AP-2和糖皮质激素受体结合位点。通过将FLAP基因的5'侧翼序列与氯霉素乙酰转移酶报告基因上游融合,对小鼠P388D1细胞(巨噬细胞)和人类HepG2细胞(肝癌细胞)进行瞬时转染,分析FLAP基因启动子的功能。各种FLAP基因启动子构建体在小鼠巨噬细胞系中的表达显示出组织特异性和类似增强子的活性,而在肝癌细胞系中仅获得最低水平的活性。

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