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鉴定受Six1同源蛋白调控的进化保守功能性非编码元件。

Identification of an evolutionarily conserved, functional noncoding element regulated by Six1 homeoprotein.

作者信息

Jeong Yongsu, Oh Sangtaek

机构信息

Department of Genetic Engineering, College of Life Sciences and Graduate School of Biotechnology, Kyung Hee University, Yongin-si, Republic of Korea.

出版信息

Genes Genet Syst. 2010;85(3):233-40. doi: 10.1266/ggs.85.233.

DOI:10.1266/ggs.85.233
PMID:21041981
Abstract

Six1, which belongs to the sine oculis homeobox (Six) protein family, is an evolutionarily conserved transcription factor found in diverse organisms ranging from flatworms to humans. Six1 is expressed in various tissues including the nervous system during ontogenesis and has been implicated in cell differentiation, morphogenesis, and organogenesis of the ganglia and sensory placodes. However, the molecular mechanisms by which Six1 influences these events at the transcriptional level remain largely unknown. In this study, we used ChIP-Display to discover genomic regions occupied in vivo by Six1 homeoprotein in the developing mouse embryo. To validate Six1 occupancy at each of Six1-bound regions, ChIP - Quantitative PCR was performed using locus-specific primers, and it showed robust enrichment of the Six1-bound sequences. To address their regulatory potential, each of the Six1-bound sequences was cloned into a reporter cassette containing beta-globin minimal promoter and lacZ gene and assayed for enhancer activity in transgenic mouse embryos. One of the novel sequences, which was designated Six1-bound Regulatory Element 1 (SRE1), was sufficient to activate lacZ reporter expression in the cranial and spinal ganglia. Comparative genomic analysis identified SRE1 sequences from a number of vertebrate phyla. Transgenic embryos carrying SRE1 sequences from human, chicken and frog showed reporter expression in a pattern similar to that of mouse SRE1, indicating their functional conservation. Through mutational analysis, we further showed that a conserved binding site matching the consensus for Six1/2/4/5 is required for the SRE1 regulatory activity. These data suggest that SRE1 is a functionally conserved transcriptional enhancer regulated by Six1.

摘要

Six1属于眼无同源框(Six)蛋白家族,是一种在进化上保守的转录因子,存在于从扁虫到人类等多种生物中。Six1在个体发育过程中在包括神经系统在内的各种组织中表达,并与神经节和感觉基板的细胞分化、形态发生和器官发生有关。然而,Six1在转录水平上影响这些事件的分子机制仍 largely未知。在本研究中,我们使用ChIP-Display来发现发育中的小鼠胚胎中Six1同源蛋白在体内占据的基因组区域。为了验证Six1在每个Six1结合区域的占据情况,使用位点特异性引物进行了ChIP - 定量PCR,结果显示Six1结合序列有强烈的富集。为了研究它们的调控潜力,将每个Six1结合序列克隆到一个包含β-珠蛋白最小启动子和lacZ基因的报告盒中,并在转基因小鼠胚胎中检测增强子活性。其中一个新序列,被命名为Six1结合调控元件1(SRE1),足以在颅神经节和脊髓神经节中激活lacZ报告基因的表达。比较基因组分析确定了来自多个脊椎动物门的SRE1序列。携带人类、鸡和青蛙SRE1序列的转基因胚胎显示出与小鼠SRE1相似的报告基因表达模式,表明它们功能保守。通过突变分析,我们进一步表明,SRE1调控活性需要一个与Six1/2/4/5共识匹配的保守结合位点。这些数据表明,SRE1是一个受Six1调控的功能保守的转录增强子。

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