Voraberger G, Schäfer R, Stratowa C
Ernst Boehringer Institut, Bender & Co., Vienna, Austria.
J Immunol. 1991 Oct 15;147(8):2777-86.
Human intercellular adhesion molecule-1 (ICAM-1), a specific ligand for the lymphocyte function-associated Ag-1 (LFA-1), plays an important role in leukocyte-endothelial cell interactions. It is induced by proinflammatory cytokines such as IL-1, TNF-alpha, or IFN-gamma. However, little is known concerning the intracellular regulatory mechanisms which trigger ICAM-1 up-regulation. In order to study potential regulatory elements involved in ICAM-1 induction we have cloned the human ICAM-1 gene and 5 kb of its 5'-regulatory region. The sequence of the cDNA was found to be distributed over seven exons separated by six introns, whereby each of the five extracellular Ig-like domains of ICAM-1 is encoded by its own exon. The upstream sequence harbors a number of sequence motifs implicated in the regulation and expression of eukaryotic genes, including binding sites for the transcription factors SP-1, AP-1, and NF-kB. Primer extension and S1 nuclease analysis revealed two transcription initiation sites 319 bp and 41 bp upstream of the translation start site. Consensus TATA boxes were found at the expected positions about 25 bp upstream of both start sites. Reverse transcriptase polymerase chain reaction showed differential use of the two TATA boxes in A549 and HS913T cells. Both RNA seem to code for the same for of ICAM-1 protein. For regulation studies a 1.3-kb EcoRI/SalI fragment of the 5'-flanking region was used to promote transcription of a linked luciferase reporter gene in transient-transfection assays in A549 and HS913T cells. Treatment of A549 cells with IL-1 or TNF-alpha resulted in a two- or fourfold increase in luciferase activity. Furthermore, a sixfold induction could be achieved after treatment with the phorbol ester PMA. In contrast, agents that increase intracellular cAMP levels did not induce luciferase activity. Northern blot analysis was used to investigate the kinetics of ICAM-1 mRNA synthesis upon induction with TNF-alpha and PMA. These data suggest that the up-regulation of ICAM-1 by cytokines occurs at least partly at the transcriptional level. Deletion analysis of the 1.3-kb fragment of the 5'-flanking region revealed sequences responsible for promotion and inhibition of transcription. In particular, two functionally distinct regions have been characterized: a short fragment containing an NF-kB binding site has been shown to function as an activator, followed immediately downstream by a sequence acting as a silencer element. Therefore, ICAM-1 gene expression seems to be modulated by multiple cis-acting elements.
人细胞间黏附分子-1(ICAM-1)是淋巴细胞功能相关抗原-1(LFA-1)的特异性配体,在白细胞与内皮细胞的相互作用中起重要作用。它由促炎细胞因子如白细胞介素-1、肿瘤坏死因子-α或干扰素-γ诱导产生。然而,关于触发ICAM-1上调的细胞内调节机制知之甚少。为了研究参与ICAM-1诱导的潜在调节元件,我们克隆了人ICAM-1基因及其5'调控区的5kb片段。发现cDNA序列分布在7个外显子上,由6个内含子分隔,其中ICAM-1的5个细胞外免疫球蛋白样结构域各自由一个外显子编码。上游序列含有许多与真核基因调控和表达相关的序列基序,包括转录因子SP-1、AP-1和NF-κB的结合位点。引物延伸和S1核酸酶分析揭示了两个转录起始位点,分别位于翻译起始位点上游319bp和41bp处。在两个起始位点上游约25bp的预期位置发现了共有TATA盒。逆转录聚合酶链反应显示,在A549和HS913T细胞中,两个TATA盒的使用存在差异。两种RNA似乎都编码相同形式的ICAM-1蛋白。为了进行调控研究,在A549和HS913T细胞的瞬时转染实验中,使用5'侧翼区的1.3kb EcoRI/SalI片段来促进连接的荧光素酶报告基因的转录。用白细胞介素-1或肿瘤坏死因子-α处理A549细胞后,荧光素酶活性增加了两倍或四倍。此外,用佛波酯PMA处理后可实现六倍的诱导。相反,增加细胞内cAMP水平的试剂不会诱导荧光素酶活性。用Northern印迹分析研究了用肿瘤坏死因子-α和PMA诱导后ICAM-1 mRNA合成的动力学。这些数据表明,细胞因子对ICAM-1的上调至少部分发生在转录水平。对5'侧翼区1.3kb片段的缺失分析揭示了负责促进和抑制转录的序列。特别是,已鉴定出两个功能不同的区域:一个含有NF-κB结合位点的短片段已被证明起激活剂作用,紧接着下游是一个作为沉默元件的序列。因此,ICAM-1基因的表达似乎受多个顺式作用元件的调节。
