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Identification and Functional Characterization of Cis-Regulatory Elements Controlling Expression of the Porcine ADRB2 Gene

机译:控制猪ADRB2基因表达的顺式调控元件的鉴定和功能表征

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The beta-2 adrenergic receptor (beta-2 AR) modulates metabolic processes in skeletal muscle, liver, and adipose tissue in response to catecholamine stimulation. We showed previously that expression of the porcine beta-2 AR gene (ADRB2) is affected by cis-regulatory polymorphisms. These are most likely responsible for the association of ADRB2 with economically relevant muscle-related traits in pigs. The present study focused on characterization of promoter elements involved in basal transcriptional regulation of the porcine ADRB2 in different cell types to aid identification of its cis-regulatory polymorphisms. Based on in silico analysis, luciferase reporter gene assays and gel shift assays were performed using COS-7, HepG2, C2C12, and 3T3-L1 cells. Deletion mapping of the 5′ flanking region (-1324 to +33) of ADRB2 revealed the region between -307 and -269 to be the minimal promoter, including regulatory elements essential for the basal transcriptional activity in all four tested cell types. Directly upstream (-400 to -323) we identified an important enhancer element required for maximal promoter activity. In silico analysis and gel shift assays revealed that this GC-rich element harbors two evolutionarily conserved binding sites of Sp1, a constitutive transcriptional activator. Significant transcriptional activation of the porcine ADRB2 promoter was demonstrated by overexpression of Sp1. Our results demonstrate, for the first time, an important role of Sp1 and of the responsive enhancer element in the regulation of ADRB2 expression. Polymorphisms located in this domain of the porcine ADRB2 promoter represent candidate causal cis-regulatory variants.
机译:响应儿茶酚胺刺激,β-2肾上腺素能受体(β-2AR)调节骨骼肌,肝脏和脂肪组织中的代谢过程。我们以前表明猪β2 AR基因(ADRB2)的表达受到顺式调节多态性的影响。这些很可能是造成ADRB2与猪中与经济相关的肌肉相关性状的关联的原因。本研究集中于在不同细胞类型中参与猪ADRB2的基础转录调控的启动子元件的表征,以帮助鉴定其顺式调控多态性。基于计算机分析,使用COS-7,HepG2,C2C12和3T3-L1细胞进行了萤光素酶报告基因测定和凝胶位移测定。对ADRB2的5'侧翼区域(-1324至+33)的缺失作图揭示了-307至-269之间的区域是最小启动子,包括所有四种测试细胞类型中基础转录活性必不可少的调节元件。在上游(-400至-323)处,我们确定了启动子最大活性所需的重要增强子元件。在计算机分析和凝胶位移分析中发现,这种富含GC的元件带有两个进化上保守的组成型转录激活因子Sp1的结合位点。 Sp1的过表达证明了猪ADRB2启动子的显着转录激活。我们的结果首次证明了Sp1和响应性增强子在ADRB2表达调节中的重要作用。猪ADRB2启动子的这个结构域中的多态性代表候选因果顺式调节变体。

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