Resnick N, Collins T, Atkinson W, Bonthron D T, Dewey C F, Gimbrone M A
Department of Pathology, Brigham and Women's Hospital, Boston, MA.
Proc Natl Acad Sci U S A. 1993 May 15;90(10):4591-5. doi: 10.1073/pnas.90.10.4591.
The endothelial lining of blood vessels is constantly exposed to fluid mechanical forces generated by flowing blood. In vitro application of fluid shear stresses to cultured endothelial cells influences the expression of multiple genes, as reflected by changes in their steady-state mRNA levels. We have utilized the B chain of platelet-derived growth factor (PDGF-B) as a model to investigate the mechanisms of shear-stress-induced gene regulation in cultured bovine aortic endothelial cells (BAECs). Northern blot analysis revealed elevated endogenous PDGF-B transcript levels in BAECs, after exposure to a physiological level of laminar shear stress (10 dynes/cm2; 1 dyne = 100 mN) for 4 h. A transfected reporter gene, consisting of a 1.3-kb fragment of the human PDGF-B promoter coupled to chloramphenicol acetyltransferase (CAT), indicated a direct effect on transcriptional activity. Transfection of a series of PDGF-B-CAT deletion mutants led to the characterization of a cis-acting component within the PDGF-B promoter that was necessary for shear-stress responsiveness. In gel-shift assays, overlapping oligonucleotide probes of this region formed several protein-DNA complexes with nuclear extracts prepared from both static and shear-stressed BAECs. A 12-bp component (CTCTCAGAGACC) was identified that formed a distinct pattern of complexes with nuclear proteins extracted from shear-stressed BAECs. This shear-stress-responsive element does not encode binding sites for any known transcription factor but does contain a core binding sequence (GAGACC), as defined by deletion mutation in gel-shift assays. Interestingly, this putative transcription factor binding site is also present in the promoters of certain other endothelial genes, including tissue plasminogen activator, intercellular adhesion molecule 1, and transforming growth factor beta 1, that also are induced by shear stress. Thus, the expression of PDGF-B and other pathophysiologically relevant genes in vascular endothelium appears to be regulated, in part, by shear-stress-induced transcription factors interacting with a common promoter element.
血管的内皮衬里不断受到流动血液产生的流体机械力的作用。在体外将流体剪切应力施加于培养的内皮细胞会影响多个基因的表达,这可通过其稳态mRNA水平的变化反映出来。我们利用血小板衍生生长因子(PDGF - B)的B链作为模型,来研究培养的牛主动脉内皮细胞(BAECs)中剪切应力诱导的基因调控机制。Northern印迹分析显示,在暴露于生理水平的层流剪切应力(10达因/平方厘米;1达因 = 100毫牛顿)4小时后,BAECs中内源性PDGF - B转录本水平升高。一个由人PDGF - B启动子的1.3千碱基片段与氯霉素乙酰转移酶(CAT)组成的转染报告基因表明对转录活性有直接影响。一系列PDGF - B - CAT缺失突变体的转染导致了对PDGF - B启动子内一个顺式作用元件的表征,该元件对于剪切应力反应性是必需的。在凝胶迁移分析中,该区域的重叠寡核苷酸探针与从静态和剪切应力处理的BAECs制备的核提取物形成了几种蛋白质 - DNA复合物。鉴定出一个12碱基的成分(CTCTCAGAGACC),它与从剪切应力处理的BAECs中提取的核蛋白形成了独特的复合物模式。这个剪切应力反应元件不编码任何已知转录因子的结合位点,但确实包含一个核心结合序列(GAGACC),这是通过凝胶迁移分析中的缺失突变确定的。有趣的是,这个假定的转录因子结合位点也存在于某些其他内皮基因的启动子中,包括组织纤溶酶原激活剂、细胞间粘附分子1和转化生长因子β1,这些基因也由剪切应力诱导。因此,血管内皮中PDGF - B和其他病理生理相关基因的表达似乎部分受剪切应力诱导的转录因子与一个共同启动子元件相互作用的调控。
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