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Protein-DNA interactions associated with the onset of testis-specific expression of the mammalian Pgk-2 gene.

机译:蛋白-DNA相互作用与哺乳动物Pgk-2基因的睾丸特异性表达的开始有关。

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摘要

We have identified difference in protein-DNA interactions associated with the promoter of the mammalian spermatogenesis-specific Pgk-2 gene in expressing and nonexpressing cells, using a band shift assay. We compared DNA-binding activities in nuclear protein extracts from expressing adult testis cells versus nonexpressing prepuberal testis cells and nonexpressing somatic cells. One or two DNA-binding activities were found to be uniquely associated with the expressed state of Pgk-2, while a third appears to be associated with the nonexpressed state. All three of these activities map to a region within the first 40 bp upstream from the core promoter of this gene. The Pgk-2 core promoter lacks a TATA box but contain a GC box and a CAAT box. We show that the GC box binds the ubiquitous transcription factor Sp1 and that the CAAT box binds CTF-1, both of which are present in extracts from all three tissue types tested. These results suggest that tissue-specific transcription of the Pgk-2 gene is associated with changes in protein-DNA interactions occurring within a 40-bp enhancer region and that different arrays of protein-DNA interactions in this region are associated with the actively expressed state of the Pgk-2 gene in spermatocytes and spermatids and with the terminally repressed state of Pgk-2 in somatic cells.
机译:我们已经使用带移分析鉴定了在表达和非表达细胞中与哺乳动物精子发生特异性Pgk-2基因启动子相关的蛋白质-DNA相互作用中的差异。我们比较了表达成人睾丸细胞与不表达青春期前睾丸细胞和不表达体细胞的核蛋白提取物中的DNA结合活性。发现一种或两种DNA结合活性与Pgk-2的表达状态唯一相关,而第三种似乎与未表达的状态相关。所有这三个活动都映射到该基因核心启动子上游前40 bp内的区域。 Pgk-2核心启动子缺少TATA框,但包含GC框和CAAT框。我们显示,GC盒结合了无处不在的转录因子Sp1,而CAAT盒结合了CTF-1,两者都存在于所有三种测试的组织提取物中。这些结果表明Pgk-2基因的组织特异性转录与40 bp增强子区域内发生的蛋白质-DNA相互作用的变化有关,并且该区域中蛋白质-DNA相互作用的不同阵列与活跃表达状态有关精子细胞和精子细胞中Pgk-2基因的表达,在体细胞中具有Pgk-2的终末抑制状态。

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