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Characterization of sINR, a strict version of the Initiator core promoter element.

机译:sINR(Initiator核心启动子元件的严格版本)的特征。

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The proximal promoter consists of binding sites for transcription regulators and a core promoter. We identified an overrepresented motif in the proximal promoter of human genes with an Initiator (INR) positional bias. The core of the motif fits the INR consensus but its sequence is more strict and flanked by additional conserved sequences. This strict INR (sINR) is enriched in TATA-less genes that belong to specific functional categories. Analysis of the sINR-containing DHX9 and ATP5F1 genes showed that the entire sINR sequence, including the strict core and the conserved flanking sequences, is important for transcription. A conventional INR sequence could not substitute for DHX9 sINR whereas, sINR could replace a conventional INR. The minimal region required to create the major TSS of the DHX9 promoter includes the sINR and an upstream Sp1 site. In a heterologous context, sINR substituted for the TATA box when positioned downstream to several Sp1 sites. Consistent with that the majority of sINR promoters contain at least one Sp1 site. Thus, sINR is a TATA-less-specific INR that functions in cooperation with Sp1. These findings support the idea that the INR is a family of related core promoter motifs.
机译:近端启动子由转录调节子的结合位点和核心启动子组成。我们在人类基因的近端启动子中发现了一个过度代表的基序,该基序具有启动子(INR)位置偏差。该基序的核心适合INR共有序列,但其序列更为严格,并侧翼有其他保守序列。这种严格的INR(sINR)富含属于特定功能类别的不含TATA的基因。对包含sINR的DHX9和ATP5F1基因的分析表明,整个sINR序列(包括严格的核心序列和保守的侧翼序列)对于转录非常重要。常规INR序列不能替代DHX9 sINR,而sINR可以替代常规INR。创建DHX9启动子的主要TSS所需的最小区域包括sINR和上游Sp1位点。在异源环境中,当位于几个Sp1位点的下游时,sINR代替了TATA盒。与大多数sINR启动子包含至少一个Sp1位点一致。因此,sINR是与Tap1协同工作的TATA特有的INR。这些发现支持了INR是相关的核心启动子基序家族的想法。

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