Ramarao C S, Denker J M, Perez D M, Gaivin R J, Riek R P, Graham R M
Department of Heart and Hypertension Research, Cleveland Clinic Foundation, Ohio 44195.
J Biol Chem. 1992 Oct 25;267(30):21936-45.
alpha 1-Adrenergic receptors (ARs) are members of the guanine nucleotide-binding protein-coupled receptor superfamily. The genes for all ARs described thus far are intronless. We report here the cloning and the nucleotide sequence of the gene for the human alpha 1B-AR. It consists of two exons and a single large intron of at least 20 kilobases which interrupts the coding region at the end of the putative sixth transmembrane domain. The deduced amino acid sequence of the encoded receptor has a high degree of homology to the cloned hamster, rat, and dog alpha 1B-ARs. To characterize the encoded protein, a fusion gene constructed by splicing together exon 1 and exon 2 was expressed transiently in COS-1 cells. The transfected gene fusion product resulted in the production of an alpha 1B-AR with ligand binding characteristics indistinguishable from those of the expressed hamster alpha 1B cDNA. Evidence that the human alpha 1B-AR gene we have isolated is indeed transcribed is the finding of similar sized (2.8-kilobase) transcripts in human heart and other tissues by Northern blot analysis when either exon 1 or exon 2 is used as a probe. Moreover, using primers designed to span the exon 1/exon 2 boundary, a polymerase chain reaction product generated from single-stranded DNA prepared from human heart mRNA had the exact size and nucleotide sequence predicted for a transcript in which exon 1 is spliced to exon 2. The 5'-flanking region (924 base pairs (bp)) of exon 1 contains neither a TATA box nor a CAAT box but is high in GC content (70%) and contains several Sp1 binding sites (GC boxes), consistent with promoters described for housekeeping genes. The 5'-untranslated region also contains a putative cyclic AMP response element. Primer extension studies and RNase protection assays suggested that there are several potential transcription start sites in most tissues with a predominant site located 173 bp upstream from the translation start site. The 3'-flanking region contains a putative polyadenylation signal (ATTAAA) 492 bp downstream from the stop codon. The genomic organization of the human alpha 1B-AR with a single large intron interrupting its coding region differs from those of other ARs as well as muscarinic and 5-hydroxy-tryptamine receptors, which are intronless. The location of the intron in the human alpha 1B-AR gene is also unique among those members of the G-protein-coupled receptor family that do possess introns.(ABSTRACT TRUNCATED AT 400 WORDS)
α1 - 肾上腺素能受体(ARs)是鸟嘌呤核苷酸结合蛋白偶联受体超家族的成员。迄今为止所描述的所有ARs的基因都没有内含子。我们在此报告人类α1B - AR基因的克隆及核苷酸序列。它由两个外显子和一个至少20千碱基的大内含子组成,该内含子在假定的第六跨膜结构域末端中断编码区。所编码受体的推导氨基酸序列与克隆的仓鼠、大鼠和犬α1B - ARs具有高度同源性。为了表征所编码的蛋白质,通过将外显子1和外显子2拼接在一起构建的融合基因在COS - 1细胞中瞬时表达。转染的基因融合产物产生了一种α1B - AR,其配体结合特性与表达的仓鼠α1B cDNA的配体结合特性无法区分。我们分离的人类α1B - AR基因确实被转录的证据是,通过Northern印迹分析发现在人类心脏和其他组织中,当使用外显子1或外显子2作为探针时,存在大小相似(2.8千碱基)的转录本。此外,使用设计用于跨越外显子1 /外显子2边界的引物,从人类心脏mRNA制备的单链DNA产生的聚合酶链反应产物具有与外显子1剪接到外显子2的转录本预测的精确大小和核苷酸序列。外显子1的5' - 侧翼区域(924个碱基对(bp))既不包含TATA盒也不包含CAAT盒,但GC含量高(70%)且包含几个Sp1结合位点(GC盒),这与管家基因的启动子一致。5' - 非翻译区还包含一个假定的环磷酸腺苷反应元件。引物延伸研究和核糖核酸酶保护试验表明,大多数组织中有几个潜在的转录起始位点,主要位点位于翻译起始位点上游173 bp处。3' - 侧翼区域在终止密码子下游492 bp处包含一个假定的聚腺苷酸化信号(ATTAAA)。人类α1B - AR的基因组结构有一个大内含子中断其编码区,这与其他ARs以及毒蕈碱和5 - 羟色胺受体不同,后两者没有内含子。在确实具有内含子的G蛋白偶联受体家族成员中,人类α1B - AR基因内含子的位置也很独特。(摘要截断于400字)
