Sriraman Venkataraman, Richards JoAnne S
Department of Molecular and Cellular Biology, Baylor College of Medicine, One Baylor Place, Houston, TX 77030, USA.
Endocrinology. 2004 Feb;145(2):582-91. doi: 10.1210/en.2003-0963. Epub 2003 Oct 16.
The cysteine protease cathepsin L exhibits hormone-regulated expression during ovulation. In situ hybridization analyses of immature and pregnant mare serum gonadotropin-treated mouse and rat ovaries showed that cathepsin L expression in granulosa cells of small, growing follicles increased in periovulatory follicles after human chorionic gonadotropin stimulation. In the rat ovary, cathepsin L was also expressed in follicles with signs of atresia. To determine the molecular mechanisms that mediate the diverse regulation of this gene in granulosa cells, rat cathepsin L promoter-reporter constructs were analyzed by transient transfection assays in rat granulosa cells and EMSAs. A construct containing the transcriptional start site and -244 bp of upstream promoter sequence (-244/+33 bp) exhibited inducibility by forskolin, the phorbol ester phorbol myristate acetate, and an additive effect of both. Within this region, three functional specificity protein 1 (Sp1) sites, an overlapping early growth response protein-1 site, and a cAMP regulatory element-binding protein site were identified. Single or double mutants of the above-mentioned sites did not alter forskolin/phorbol myristate acetate inducibility of the promoter. Mutation of all three Sp1/specificity protein 3 (Sp3) sites, which also mutated the early growth response protein-1 site, reduced the promoter activation. Mutation of the cAMP regulatory element-binding protein site in the triple Sp1 mutant construct completely blocked the inducibility of the promoter. When these same constructs were transfected into MCF-7 human breast cancer cells or were cotransfected with an Sp1 expression vector in Drosophila SL2 cells, similar results were obtained. Collectively, the data document that three Sp1/specificity protein 3 binding GC-rich regions and a functional cAMP regulatory element constitute an important transcriptional regulatory complex for expression of the cathepsin L gene in rat granulosa cells.
半胱氨酸蛋白酶组织蛋白酶L在排卵过程中表现出激素调节的表达。对未成熟及经孕马血清促性腺激素处理的小鼠和大鼠卵巢进行原位杂交分析显示,人绒毛膜促性腺激素刺激后,小的生长卵泡颗粒细胞中的组织蛋白酶L表达在排卵前卵泡中增加。在大鼠卵巢中,组织蛋白酶L在有闭锁迹象的卵泡中也有表达。为了确定介导该基因在颗粒细胞中不同调节的分子机制,通过在大鼠颗粒细胞中的瞬时转染试验和电泳迁移率变动分析(EMSA)对大鼠组织蛋白酶L启动子 - 报告基因构建体进行了分析。一个包含转录起始位点和上游启动子序列 -244 bp(-244 / +33 bp)的构建体表现出对福斯可林、佛波酯肉豆蔻酸佛波醇酯的诱导性以及两者的相加效应。在该区域内,鉴定出三个功能性特异性蛋白1(Sp1)位点、一个重叠的早期生长反应蛋白 -1位点和一个cAMP反应元件结合蛋白位点。上述位点的单突变或双突变并未改变启动子对福斯可林/肉豆蔻酸佛波醇酯的诱导性。所有三个Sp1 /特异性蛋白3(Sp3)位点的突变,同时也使早期生长反应蛋白 -1位点发生突变,降低了启动子的活性。三重Sp1突变构建体中cAMP反应元件结合蛋白位点的突变完全阻断了启动子的诱导性。当将这些相同的构建体转染到MCF - 7人乳腺癌细胞中或与Sp1表达载体共转染到果蝇SL2细胞中时,获得了相似的结果。总体而言,数据表明三个富含GC的Sp1 /特异性蛋白3结合区域和一个功能性cAMP反应元件构成了大鼠颗粒细胞中组织蛋白酶L基因表达的重要转录调节复合体。
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