Saulnier-Blache J S, Yang Q, Sherlock J D, Lanier S M
Department of Pharmacology, Medical University of South Carolina, Charleston 29425, USA.
Mol Pharmacol. 1996 Dec;50(6):1432-42.
As an initial approach to define the regulatory elements and transcriptional factors that account for cell-restricted expression of the alpha2c-adrenergic receptor (AR) gene, we isolated and characterized the receptor gene and identified regions of the gene conferring cell-specific expression. A 4300-nucleotide (nt) fragment of the 5'-flanking region of the rat alpha2c-AR gene was isolated from a genomic library. The genomic sequence contained the uninterrupted sequence of the 5'-untranslated region of a previously isolated alpha2c-AR cDNA clone indicating the lack of introns in the 5' gene segment. RNase protection assays and/or RNA blot analysis indicated the expression of alpha2c-AR mRNA in rat brain but not in kidney or liver, which is consistent with the major expression of this gene in neuronal tissue. The 5' gene segment was used to identify sites of transcriptional initiation and promoter activity by RNase protection assays and transient transfection of reporter gene constructs. With the use of RNA probes progressively upstream of the translational start site, RNase protection assays with rat brain total RNA indicated multiple sites of transcriptional initiation within a approximately 70-nt span (-660 to -730 nt 5' to the translational start codon). The zone of transcriptional initiation was part of a larger GC-rich area of the 5' gene segment that is a characteristic of genes initiating transcripts at multiple sites. The promoter activity of this zone of transcriptional initiation and the influence of gene segments 5' to this area were addressed using chloramphenicol acetyl transferase reporter gene constructs. Transient transfection of reporter gene constructs indicated that a 96-nt gene fragment (-699/-603 relative to the translational start codon) was sufficient to direct transcription in the neuroblastoma X glioma hybrid cell line NG108-15, a cell line expressing the endogenous alpha2c-AR. Promoter activity was not observed in constructs lacking the zone of transcriptional initiation. The promoter segment was inactive when introduced into the rat glioma cell line C6B4, the rat submandibular cell line RSMT-A5, and the rat pancreatic beta cell line RIN-5AH, all of which do not express the endogenous alpha2c-AR gene. Upon incubation with nuclear extracts, a 129-nt fragment encompassing the promoter exhibited a gel mobility shift pattern that was specific for cells expressing the receptor protein and involved a nuclear protein that recognized a Sp1 oligonucleotide. These data indicate that a 96-nt gene promoter segment of the alpha2c-AR gene functions in a cell-type-specific manner.
作为确定负责α2c - 肾上腺素能受体(AR)基因细胞限制性表达的调控元件和转录因子的初步方法,我们分离并鉴定了该受体基因,并确定了赋予细胞特异性表达的基因区域。从基因组文库中分离出大鼠α2c - AR基因5' - 侧翼区域的一个4300个核苷酸(nt)的片段。该基因组序列包含先前分离的α2c - AR cDNA克隆的5' - 非翻译区的不间断序列,表明5'基因片段中不存在内含子。核糖核酸酶保护试验和/或RNA印迹分析表明α2c - AR mRNA在大鼠脑中表达,但在肾脏或肝脏中不表达,这与该基因在神经元组织中的主要表达一致。5'基因片段用于通过核糖核酸酶保护试验和报告基因构建体的瞬时转染来鉴定转录起始位点和启动子活性。使用在翻译起始位点上游逐渐延伸的RNA探针,用大鼠脑总RNA进行的核糖核酸酶保护试验表明在大约70 nt范围内(翻译起始密码子5'端 - 660至 - 730 nt)有多个转录起始位点。转录起始区是5'基因片段中一个更大的富含GC区域的一部分,这是在多个位点起始转录本的基因的特征。使用氯霉素乙酰转移酶报告基因构建体研究了该转录起始区的启动子活性以及该区域5'端基因片段的影响。报告基因构建体瞬时转染表明一个96 nt的基因片段(相对于翻译起始密码子为 - 699 / - 603)足以指导神经母细胞瘤X胶质瘤杂交细胞系NG108 - 15中的转录,该细胞系表达内源性α2c - AR。在缺乏转录起始区的构建体中未观察到启动子活性。当将启动子片段导入大鼠胶质瘤细胞系C6B4、大鼠下颌下细胞系RSMT - A5和大鼠胰腺β细胞系RIN - 5AH时,启动子片段均无活性,所有这些细胞系均不表达内源性α2c - AR基因。与核提取物孵育后,包含启动子的129 nt片段表现出凝胶迁移率变化模式,该模式对表达受体蛋白的细胞具有特异性,并且涉及一种识别Sp1寡核苷酸的核蛋白。这些数据表明α2c - AR基因的一个96 nt的基因启动子片段以细胞类型特异性方式发挥作用。
