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Sexually dimorphic DNA demethylation in the promoter of the Slp (sex-limited protein) gene in mouse liver.

机译:小鼠肝脏中Slp(性别受限蛋白)基因启动子中的性二态性DNA去甲基化。

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摘要

Mouse Slp, a duplicate of the fourth complement component (C4) gene, exhibits EDTA-independent complement activity with a hepatic expression that is male specific. To provide an underlying mechanism for the male-specific expression, we have analyzed the promoter activity of the various 5'-flanking sequences and CpG demethylation of the Slp gene. Transient transfections using HepG2 cells indicate that the element TTCCGGGC (nt -124 to -117) regulates the promoter activity. Moreover, CpG at position -121 of this regulatory element is demethylated to a much higher degree in males than in females. This sexually dimorphic DNA demethylation is consistent with the male-specific expression of the Slp gene in DBA/2 males. The regulatory element binds to the different TTCCGGGC-specific nuclear proteins depending on the methylation of the CpG site. In contrast, the corresponding CpG at position -119 of the C4 gene, which is expressed in both males and females, is demethylated at equal and high levels in both sexes. We therefore propose that the DNA demethylation and methylation-sensitive transcription factors may be a part of the regulatory mechanism for the male-specific expression of the Slp gene.
机译:鼠Slp,第四补体成分(C4)基因的重复体,表现出EDTA依赖性补体活性,其肝表达是雄性特异性的。为了提供雄性特异性表达的潜在机制,我们分析了各种5'侧翼序列的启动子活性和Slp基因的CpG去甲基化。使用HepG2细胞进行的瞬时转染表明,元素TTCCGGGC(nt -124至-117)调节启动子活性。而且,该调节元件在-121位的CpG在男性中的脱甲基程度远高于在女性中。这种性二态性DNA去甲基化与DBA / 2雄性中Slp基因的雄性特异性表达相一致。取决于CpG位点的甲基化,调节元件结合不同的TTCCGGGC特异性核蛋白。相反,在雄性和雌性中都表达的C4基因的-119位相应的CpG在两个性别中均以相同和较高的水平去甲基化。因此,我们建议DNA脱甲基和甲基化敏感的转录因子可能是Slp基因的男性特异性表达调控机制的一部分。

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