Ngan E S, Cheng P K, Leung P C, Chow B K
Department of Zoology, University of Hong Kong, Hong Kong.
Endocrinology. 1999 Jun;140(6):2452-62. doi: 10.1210/endo.140.6.6759.
GnRH plays a pivotal role in regulating human reproductive functions. This hypothalamic peptide interacts with its receptor (GnRHR) on the pituitary gonadotropes to trigger the secretion of gonadotropins, which, in turn, regulates the release of sex steroids from the gonads. In light of the importance of GnRHR, the molecular mechanisms underlying the transcriptional regulation of the human GnRHR (hGnRHR) gene become a key issue in understanding human reproduction. In this report, the possible involvement of steriodogenic factor-1 (SF-1) as a key cell-specific regulator for hGnRHR gene expression was examined. By the transient luciferase reporter gene assays, the wild-type promoter, containing 2.3 kb ofthe hGnRHR gene 5'-flanking region relative to the ATG codon, was able to drive a 3.6 +/- 0.2-fold (P < 0.05) increase in luciferase activity in the mouse alphaT3-1 gonadotropes. Subsequent deletion analysis indicated that the most proximal 173 bp within the first exon of the gene, although not a promoter itself, contains a critical regulatory element(s) essential for the basal expression of the hGnRHR gene. The functional roles of the putative gonadotrope-specific elements (GSE; consensus 5'-CTG(A)/(T)CCTTG-3') residing at positions -5, -134, and -396 were studied by site-directed mutagenesis, and it was found that only the mutation at position -134 significantly reduced the promoter activity (80% reduction; P < 0.05). The attenuation effect of this GSE mutant was cell specific, as it was restricted to alphaT3-1 cells, but not to COS-7 and human ovarian adenocarcinoma (SKOV-3) cells. Competitive mobility shift assays using either alphaT3-1 nuclear extract or recombinant SF-1 protein clearly indicated that SF-1 is able to interact specifically with this GSE element positioned at -134. Using a SF-1 antibody that completely abrogated complex formation in the gel shift assays, the involvement of endogenous nuclear SF-1 was further evidenced. By competitive gel shift assays using oligoprimers with 2-bp scanning mutations, the sequences essential for the interaction with SF-1 were identified (5'-TTG(A)/(T)CCCTG-3', underlined sequences were important). To study the in vivo function of SF-1, vector directing expression of sense or antisense SF-1 messenger RNA (mRNA) was cotransfected with the hGnRHR promoter-luciferase construct into alphaT3-1, SKOV-3, and COS-7 cells. Overexpression of the SF-1 mRNA was able to enhance promoter activities in all of the cells tested. On the contrary, expression of the antisense SF-1 mRNA reduced the hGnRHR promoter activity only in alphaT3-1 cells, not in COS-7 or SKOV-3 cells. In summary, the data reported here provide conclusive evidence that SF-1 interacts with the GSE motif at position -134 within the first exon of the hGnRHR gene to mediate its cell-specific expression.
促性腺激素释放激素(GnRH)在调节人类生殖功能中起关键作用。这种下丘脑肽与垂体促性腺细胞上的受体(GnRHR)相互作用,触发促性腺激素的分泌,进而调节性腺中性类固醇的释放。鉴于GnRHR的重要性,人类GnRHR(hGnRHR)基因转录调控的分子机制成为理解人类生殖的关键问题。在本报告中,研究了类固醇生成因子-1(SF-1)作为hGnRHR基因表达的关键细胞特异性调节因子的可能参与情况。通过瞬时荧光素酶报告基因检测,相对于ATG密码子,包含hGnRHR基因5'侧翼区域2.3 kb的野生型启动子能够使小鼠αT3-1促性腺细胞中的荧光素酶活性增加3.6±0.2倍(P<0.05)。随后的缺失分析表明,该基因第一个外显子内最靠近近端的173 bp,虽然本身不是启动子,但包含hGnRHR基因基础表达所必需的关键调控元件。通过定点诱变研究了位于-5、-134和-396位置的假定促性腺细胞特异性元件(GSE;共有序列5'-CTG(A)/(T)CCTTG-3')的功能作用,发现只有-134位置的突变显著降低了启动子活性(降低80%;P<0.05)。这种GSE突变体的减弱作用具有细胞特异性,因为它仅限于αT3-1细胞,而不是COS-7细胞和人卵巢腺癌(SKOV-3)细胞。使用αT3-1核提取物或重组SF-1蛋白进行的竞争性迁移率变动分析清楚地表明,SF-1能够与位于-134的这个GSE元件特异性相互作用。使用在凝胶迁移分析中完全消除复合物形成的SF-1抗体,进一步证明了内源性核SF-1的参与。通过使用具有2 bp扫描突变的寡核苷酸引物进行竞争性凝胶迁移分析,确定了与SF-1相互作用所必需的序列(5'-TTG(A)/(T)CCCTG-3',下划线序列很重要)。为了研究SF-1的体内功能,将指导有义或反义SF-1信使RNA(mRNA)表达的载体与hGnRHR启动子-荧光素酶构建体共转染到αT3-1、SKOV-3和COS-7细胞中。SF-1 mRNA的过表达能够增强所有测试细胞中的启动子活性。相反,反义SF-1 mRNA的表达仅在αT3-1细胞中降低hGnRHR启动子活性,而在COS-7或SKOV-3细胞中则没有。总之,这里报告的数据提供了确凿的证据,即SF-1与hGnRHR基因第一个外显子中位于-134的GSE基序相互作用,以介导其细胞特异性表达。
