首页> 外文期刊>Molecular and Cellular Endocrinology >Molecular characterization of prolactin receptor (cPRLR) gene in chickens: Gene structure, tissue expression, promoter analysis, and its interaction with chicken prolactin (cPRL) and prolactin-like protein (cPRL-L)
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Molecular characterization of prolactin receptor (cPRLR) gene in chickens: Gene structure, tissue expression, promoter analysis, and its interaction with chicken prolactin (cPRL) and prolactin-like protein (cPRL-L)

机译:鸡催乳激素受体(cPRLR)基因的分子表征:基因结构,组织表达,启动子分析及其与鸡催乳素(cPRL)和催乳素样蛋白(cPRL-L)的相互作用

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In this study, gene structure, tissue expression, and promoter usage of prolactin receptor (PRLR) and its interaction with prolactin (PRL) and the newly identified prolactin-like protein (PRL-L) were investigated in chickens. The results showed that (1) PRLR gene was found to consist of at least 25 exons by 5'-RACE and RT-PCR assays; (2) multiple PRLR 5'-UTR sequences different in exon composition were isolated from chicken liver or intestine by 5'-RACE and could be subdivided into type I and type II transcripts according to the first exon used (exon 1G or exon 1A); (3) PRLR Type I transcripts with exon 1G were detected to be predominantly expressed in adult kidney and small intestine by RT-PCR, implying their expression is likely controlled by a tissue-specific promoter (P1). By contrast, PRLR type II transcripts containing exon 1A are widely expressed in adult and embryonic tissues examined and their expression is controlled by a generic promoter (P2) near exon 1A, which was demonstrated to display promoter activities in cultured DF-1, HEK293 and LoVo cells by the dual-luciferase reporter assay; (4) Using a 5. ×. STAT5-luciferase reporter system, cPRLR expressed in HepG2 cells was shown to be activated by recombinant cPRL and cPRL-L via interaction with PRLR membrane-proximal ligand-binding domain, suggesting that like cPRL, cPRL-L is also a functional ligand of cPRLR. Collectively, characterization of cPRLR gene helps to elucidate the roles of PRLR and its ligands in birds and provides insights into the regulatory mechanisms of PRLR expression conserved in birds and mammals.
机译:在这项研究中,研究了鸡泌乳素受体(PRLR)的基因结构,组织表达和启动子用途,以及与催乳素(PRL)和新鉴定的催乳素样蛋白(PRL-L)的相互作用。结果表明:(1)通过5'-RACE和RT-PCR检测发现PRLR基因至少由25个外显子组成; (2)通过5'-RACE从鸡肝或肠中分离出多个外显子组成不同的PRLR 5'-UTR序列,并可以根据使用的第一个外显子(外显子1G或外显子1A)将其分为I型和II型转录本。 ; (3)RT-PCR检测到具有外显子1G的PRLR I型转录物主要在成人肾脏和小肠中表达,这表明它们的表达可能受组织特异性启动子(P1)的控制。相比之下,含有外显子1A的PRLR II型转录物在受检的成年和胚胎组织中广泛表达,其表达受到外显子1A附近的通用启动子(P2)的控制,该启动子在培养的DF-1,HEK293和DF1中显示出启动子活性。 LoVo细胞通过双荧光素酶报告基因检测; (4)使用5.×。 STAT5-荧光素酶报告系统显示,通过与PRLR膜近端配体结合域相互作用,重组cPRL和cPRL-L激活了HepG2细胞中表达的cPRLR,这表明cPRL-L也是cPRLR的功能性配体。总的来说,cPRLR基因的表征有助于阐明PRLR及其配体在鸟类中的作用,并为深入了解鸟类和哺乳动物中PRLR表达的调控机制提供了见识。

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