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奇努克鲑(Oncorhynchus tschawytscha)促性腺激素IIβ亚基基因中雌激素反应元件的功能分析

Functional analysis of estrogen-responsive elements in chinook salmon (Oncorhynchus tschawytscha) gonadotropin II beta subunit gene.

作者信息

Liu D, Xiong F, Hew C L

机构信息

Research Institute, Hospital for Sick Children, Toronto, Ontario, Canada.

出版信息

Endocrinology. 1995 Aug;136(8):3486-93. doi: 10.1210/endo.136.8.7628385.

DOI:10.1210/endo.136.8.7628385
PMID:7628385
Abstract

The salmon gonadotropin II gene regulates ovulation and spawning. Analysis of the 5' flanking sequence of the hormone-specific beta-subunit of salmon gonadotropin II (sGTHII beta) gene reveals the presence of several presumptive estrogen-responsive elements (ERE). The participation of ERE in the control of sGTHII beta gene transcription was examined by the transient expression of sGTHII beta gene promoter-chloramphenicol acetyltransferase chimeric DNA constructs in HeLa cells, with the cotransfection of a rainbow trout estrogen receptor expression vector. Three ERE have been identified: the proximal ERE [pERE, at -267 base pair (bp) from the transcription start site], the distal ERE (dERE, at -2698 bp, three GGTCA motifs each separated by exactly 31 bp), and the half-ERE (1/2ERE, at -157 bp as a GGTCA motif), respectively. The pERE (TGTCAATCTGACC) represents a novel but less effective variation of the consensus ERE (cERE). The dERE is a unique estrogen-induced enhancer. It requires the participation of the pERE to be functional and the enhancer activity of pERE and dERE is promoter specific. The contribution of 1/2ERE is minor and is not cell-type specific. The activation of the ERE in the sGTHII beta gene and the synergistic cooperation between the dERE and pERE by estradiol-17 beta is dose dependent. DNA sequences in the vicinity of the ERE decreases their hormone responsiveness and the synergism between dERE and pERE. These negative regions may contribute to the quiescent endocrine state of the sGTHII beta gene during the regressive phase of the reproductive cycle in teleost.

摘要

鲑鱼促性腺激素II基因调控排卵和产卵。对鲑鱼促性腺激素II(sGTHIIβ)激素特异性β亚基的5'侧翼序列分析显示存在几个假定的雌激素反应元件(ERE)。通过在HeLa细胞中瞬时表达sGTHIIβ基因启动子-氯霉素乙酰转移酶嵌合DNA构建体,并共转染虹鳟鱼雌激素受体表达载体,研究了ERE在sGTHIIβ基因转录控制中的作用。已鉴定出三个ERE:近端ERE [pERE,位于转录起始位点-267碱基对(bp)处]、远端ERE(dERE,位于-2698 bp处,每个GGTCA基序相隔正好31 bp)和半ERE(1/2ERE,位于-157 bp处,为一个GGTCA基序)。pERE(TGTCAATCTGACC)代表共有ERE(cERE)的一种新的但效果较差的变体。dERE是一种独特的雌激素诱导增强子。它需要pERE的参与才能发挥功能,并且pERE和dERE的增强子活性具有启动子特异性。1/2ERE的作用较小且不具有细胞类型特异性。17β-雌二醇对sGTHIIβ基因中ERE的激活以及dERE和pERE之间的协同作用是剂量依赖性的。ERE附近的DNA序列会降低它们的激素反应性以及dERE和pERE之间的协同作用。这些负性区域可能有助于硬骨鱼生殖周期退化阶段sGTHIIβ基因的静止内分泌状态。

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