单倍型对内皮NO合成酶启动子效率的特异性影响:吸烟可改变

Jian Wang, D. Dudley, Xing-li Wang
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引用次数: 143

摘要

内皮NO合成酶(eNOS)基因的T-786C启动子和27-bp重复内含子4多态性与各种eNOS相关的表型变化不一致。我们探索了这种不一致的分子机制。我们构建了pGL3荧光素酶报告载体,方法是在荧光素酶编码区5 '端插入一个在- 786 bp处含有T或C核苷酸的eNOS启动子片段,在荧光素酶基因3 '端插入一个含有5x或4×27-bp重复序列的eNOS内含子4。T启动子的转录效率低于C启动子(5×27-bp为增强子时为15.7±1.0%比83.3±5.8%,P <0.01; 4×27bp为增强子时为37.6±4.7%比58.9±7.5%,P <0.01)。烟草提取物处理显著提高了T启动子的转录效率(1.7倍,P <0.01),但降低了C启动子的转录效率(10% ~ 15%)。迁移迁移试验显示27 bp重复片段与内皮细胞核蛋白提取物正结合。我们的研究证明了27 bp重复序列在eNOS启动子功能中的顺式作用,以及由- 786 bp和eNOS基因内含子4的DNA变异决定的单倍型特异性表达模式,该模式也可以通过吸烟改变。
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Haplotype-Specific Effects on Endothelial NO Synthase Promoter Efficiency: Modifiable by Cigarette Smoking
The T–786C promoter and 27-bp repeat intron 4 polymorphisms in the endothelial NO synthase (eNOS) gene have been inconsistently associated with various eNOS-related phenotypic changes. We explored molecular mechanisms underlying the inconsistency. We constructed pGL3 luciferase reporter vectors by inserting an eNOS promoter fragment containing either T or C nucleotide at −786 bp at the 5′ end of the luciferase coding region and eNOS intron 4 containing either 5× or 4×27-bp repeats at the 3′ end of the luciferase gene. The transcription efficiency in the T promoter was lower than in the C promoter (15.7±1.0% vs 83.3±5.8%, P <0.01 when 5×27-bp was an enhancer and 37.6±4.7% vs 58.9±7.5%, P <0.01 when 4×27bp was an enhancer). Although cigarette smoking extracts treatment increased the transcription efficiency significantly in the T promoter (1.7-fold, P <0.01), it reduced the C promoter efficiency (by 10% to 15%). A mobility shift assay revealed positive binding of the 27-bp repeat fragment with endothelial cell nuclear protein extracts. Our study demonstrates a cis-acting role of the 27-bp repeats in eNOS promoter function and a haplotype-specific expression pattern determined by DNA variants at −786 bp and intron 4 of the eNOS gene that is also modifiable by cigarette smoking.
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