Department of Pathology and Molecular Medicine, Queen's University, Kingston, Ontario, Canada.
Blood. 2010 Nov 4;116(18):3645-52. doi: 10.1182/blood-2009-12-261131. Epub 2010 Aug 9.
We have studied the effect of a 13-bp deletion in the promoter of the von Willebrand factor (VWF) gene in a patient with type 1 von Willebrand disease. The index case has a VWF:Ag of 0.49 IU/mL and is heterozygous for the deletion. The deletion is located 48 bp 5' of the transcription start site, and in silico analysis, electrophoretic mobility shift assays, and chromatin immunoprecipitation studies all predict aberrant binding of Ets transcription factors to the site of the deletion. Transduction of reporter gene constructs into blood outgrowth endothelial cells showed a 50.5% reduction in expression with the mutant promoter (n = 16, P < .001). A similar 40% loss of transactivation was documented in transduced HepG2 cells. A similar marked reduction of transgene expression was shown in the livers of mice injected with the mutant promoter construct (n = 8, P = .003). Finally, in studies of BOEC mRNA, the index case showed a 4.6-fold reduction of expression of the VWF transcript associated with the deletion mutation. These studies show that the 13-bp deletion mutation alters the binding of Ets (and possibly GATA) proteins to the VWF promoter and significantly reduces VWF expression, thus playing a central pathogenic role in the type 1 von Willebrand disease phenotype in the index case.
我们研究了 1 型血管性血友病患者中血管性血友病因子 (VWF) 基因启动子中 13 个碱基对缺失的影响。该指数病例的 VWF:Ag 为 0.49 IU/mL,且为该缺失的杂合子。该缺失位于转录起始位点的 5'侧 48 个碱基对处,计算机分析、电泳迁移率变动分析和染色质免疫沉淀研究均预测 Ets 转录因子异常结合到缺失部位。将报告基因构建体转导到血外生内皮细胞中,发现突变启动子的表达降低了 50.5%(n = 16,P <.001)。在转导的 HepG2 细胞中也记录到类似的 40%转录激活丧失。在注射突变启动子构建体的小鼠肝脏中,也显示出类似的显著降低的转基因表达(n = 8,P =.003)。最后,在 BOEC mRNA 的研究中,该指数病例显示与缺失突变相关的 VWF 转录物的表达降低了 4.6 倍。这些研究表明,13 个碱基对缺失突变改变了 Ets(和可能的 GATA)蛋白与 VWF 启动子的结合,并显著降低了 VWF 的表达,从而在该指数病例的 1 型血管性血友病表型中发挥了核心致病作用。