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在海鲷中存在两种不同的催乳素受体,它们具有不同的组织分布模式、信号转导途径以及甾体激素对基因表达的调控。

The presence of two distinct prolactin receptors in seabream with different tissue distribution patterns, signal transduction pathways and regulation of gene expression by steroid hormones.

作者信息

Huang Xigui, Jiao Baowei, Fung Chun Kit, Zhang Yong, Ho Walter K K, Chan Chi Bun, Lin Haoran, Wang Deshou, Cheng Christopher H K

机构信息

Key Laboratory of Eco-environments in Three Gorges Reservoir Region (Ministry of Education), Key Laboratory of Aquatic Science of Chongqing, School of Life Science, Southwest University, Chongqing 400715, China.

出版信息

J Endocrinol. 2007 Aug;194(2):373-92. doi: 10.1677/JOE-07-0076.

Abstract

Two prolactin receptors (PRLRs) encoded by two different genes were identified in the fugu and zebrafish genomes but not in the genomes of other vertebrates. Subsequently, two cDNA sequences corresponding to two PRLRs were identified in black seabream and Nile tilapia. Phylogenetic analysis of PRLR sequences in various vertebrates indicated that the coexistence of two PRLRs in a single species is a unique phenomenon in teleosts. Both PRLRs in teleosts (the classical one named as PRLR1, the newly identified one as PRLR2) resemble the long-form mammalian PRLRs. However, despite their overall structural similarities, the two PRLR subtypes in fish share very low amino acid similarities (about 30%), mainly due to differences in the intracellular domain. In particular, the Box 2 region and some intracellular tyrosine residues are missing in PRLR2. Tissue distribution study by real-time PCR in black seabream (sb) revealed that both receptors (sbPRLR1 and sbPRLR2) are widely expressed in different tissues. In gill, the expression level of sbPRLR2 is much higher than that of sbPRLR1. In the intestine, the expression of sbPRLR1 is higher than that of sbPRLR2. The expression levels of both receptors are relatively low in most other tissues, with sbPRLR1 generally higher than sbPRLR2. The sbPRLR1 and sbPRLR2 were functionally expressed in cultured human embryonic kidney 293 cells. Both receptors can activate the beta-casein and c-fos promoters; however, only sbPRLR1 but not sbPRLR2 can activate the Spi promoter upon receptor stimulation in a ligand-specific manner. These results indicate that both receptors share some common functions but are distinctly different from each other in mobilizing post-receptor events. When challenged with different steroid hormones, the two PRLRs exhibited very different gene expression patterns in the seabream kidney. The sbPRLR1 expression was up-regulated by estradiol and cortisol, whereas testosterone had no significant effect. For sbPRLR2, its expression was down-regulated by estradiol and testosterone, while cortisol exerted no significant effect. The 5'-flanking regions of the sbPRLR1 and sbPRLR2 genes were cloned and the promoter activities were studied in transfected GAKS cells in the absence or presence of different steroid hormones. The results of the promoter studies were in general agreement with the in vivo hormonal regulation of gene expression results. The sbPRLR1 gene promoter activity was activated by estradiol and cortisol, but not by testosterone. In contrast, the sbPRLR2 gene promoter activity was inhibited by estradiol, cortisol, and testosterone.

摘要

在河豚和斑马鱼基因组中鉴定出了由两个不同基因编码的两种催乳素受体(PRLR),但在其他脊椎动物基因组中未发现。随后,在黑鲷和尼罗罗非鱼中鉴定出了与两种PRLR相对应的两个cDNA序列。对各种脊椎动物中PRLR序列的系统发育分析表明,单一物种中两种PRLR的共存是硬骨鱼中的独特现象。硬骨鱼中的两种PRLR(经典的一种命名为PRLR1,新鉴定的一种为PRLR2)类似于哺乳动物的长形式PRLR。然而,尽管它们在整体结构上相似,但鱼类中的两种PRLR亚型氨基酸相似性非常低(约30%),主要是由于细胞内结构域的差异。特别是,PRLR2中缺少Box 2区域和一些细胞内酪氨酸残基。通过实时PCR对黑鲷(sb)进行的组织分布研究表明,两种受体(sbPRLR1和sbPRLR2)在不同组织中广泛表达。在鳃中,sbPRLR2的表达水平远高于sbPRLR1。在肠道中,sbPRLR1的表达高于sbPRLR2。在大多数其他组织中,两种受体的表达水平相对较低,sbPRLR1通常高于sbPRLR2。sbPRLR1和sbPRLR2在培养的人胚肾293细胞中进行了功能表达。两种受体都可以激活β-酪蛋白和c-fos启动子;然而,在受体刺激后,只有sbPRLR1而不是sbPRLR2能够以配体特异性方式激活Spi启动子。这些结果表明,两种受体具有一些共同功能,但在启动受体后事件方面明显不同。当用不同的类固醇激素刺激时,两种PRLR在黑鲷肾脏中表现出非常不同的基因表达模式。sbPRLR1的表达受到雌二醇和皮质醇的上调,而睾酮没有显著影响。对于sbPRLR2,其表达受到雌二醇和睾酮的下调,而皮质醇没有显著影响。克隆了sbPRLR1和sbPRLR2基因的5'侧翼区域,并在转染的GAKS细胞中研究了在有无不同类固醇激素存在下的启动子活性。启动子研究的结果与基因表达的体内激素调节结果总体一致。sbPRLR1基因启动子活性受到雌二醇和皮质醇的激活,但不受睾酮的激活。相反,sbPRLR2基因启动子活性受到雌二醇、皮质醇和睾酮的抑制。

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