Feng Z M, Wu A Z, Chen C L
Population Council, New York, New York 10021.
Endocrinology. 1995 Mar;136(3):947-55. doi: 10.1210/endo.136.3.7867604.
We and others have shown that the inhibin/activin beta B-subunit gene is expressed differently in the gonads. Two species of 4.8- and 3.7-kilobase (kb) beta B-subunit messenger RNA (mRNA) with equal concentrations were identified in the testis, whereas 1 predominant 4.8-kb and a minor 3.7-kb mRNA were observed in the ovary. In this study, we analyzed the structures of these 2 mRNAs in rat testis and showed that both 4.8- and 3.7-kb beta B-subunit mRNAs were terminated at the region proximal to 2.2 kb down-stream from the translation stop codon. However, only 4.8-kb mRNA could be detected when RNA probes prepared from the 5'-region 1 kb up-stream from the translation start site were used for Northern blot analysis. Our observations suggested that the 2 heterogeneously sized beta B-subunit mRNAs are transcribed from different initiation sites. Transcription of the 4.8-kb mRNA was initiated at 3 adjacent nucleotides, GGA, 1.1 kb up-stream from the translation start codon ATG, whereas multiple transcription initiation sites spreading over 150 nucleotides upstream from the ATG codon were previously identified for 3.7-kb mRNA. Neither of the 2 transcripts contained TATA and CAAT boxes in their promoters. The 5'-flanking DNAs required for transcription of the 4.8- and 3.7-kb mRNA were examined by their ability to induce transient expression of the chloramphenicol acetyltransferase (CAT) gene in MA-10 Leydig tumor cells. A marked increase in CAT activity was detected when the 5'-flanking DNA for the 4.8- or 3.7-kb transcript was progressively shortened from its 5'-end. Maximal CAT activity was observed when -409 and -139 basepair beta B-subunit DNA up-stream from the 4.8- and 3.7-kb transcription initiation site, respectively, were fused to the CAT gene, suggesting the presence of a negative regulatory element(s) at the up-stream regions of these promoters. Although putative AP-2 sites were identified, treatment of the transfected cells with cAMP and/or phorbol 12-myristate 13-acetate did not apparently change CAT activity driven by either the 4.8- or 3.7-kb promoter. Our results concluded that 1) the two inhibin/activin beta B-subunit mRNAs were transcribed from different initiation sites; 2) both promoters may be controlled by up-stream negative regulatory elements; and 3) neither of these promoters is responsive to cAMP and/or phorbol esters under the conditions employed.
我们和其他研究人员已表明,抑制素/激活素βB亚基基因在性腺中的表达存在差异。在睾丸中鉴定出两种浓度相等的4.8千碱基(kb)和3.7 kb的βB亚基信使核糖核酸(mRNA),而在卵巢中观察到1种主要的4.8 kb和1种次要的3.7 kb mRNA。在本研究中,我们分析了大鼠睾丸中这两种mRNA的结构,结果显示4.8 kb和3.7 kb的βB亚基mRNA均在翻译终止密码子下游2.2 kb附近区域终止。然而,当使用从翻译起始位点上游1 kb的5'区域制备的RNA探针进行Northern印迹分析时,仅能检测到4.8 kb的mRNA。我们的观察结果表明,这两种大小不同的βB亚基mRNA是从不同的起始位点转录而来的。4.8 kb mRNA的转录起始于翻译起始密码子ATG上游1.1 kb处的3个相邻核苷酸GGA,而先前已确定3.7 kb mRNA的多个转录起始位点分布在ATG密码子上游150个核苷酸范围内。这两种转录本在其启动子中均不包含TATA盒和CAAT盒。通过它们在MA-10睾丸间质细胞瘤细胞中诱导氯霉素乙酰转移酶(CAT)基因瞬时表达的能力,检测了4.8 kb和3.7 kb mRNA转录所需的5'侧翼DNA。当从其5'端逐渐缩短4.8 kb或3.7 kb转录本的5'侧翼DNA时,检测到CAT活性显著增加。当分别将4.8 kb和3.7 kb转录起始位点上游-409和-139碱基对的βB亚基DNA与CAT基因融合时,观察到最大的CAT活性,这表明在这些启动子的上游区域存在负调控元件。尽管鉴定出了假定的AP-2位点,但用环磷酸腺苷(cAMP)和/或佛波酯12-肉豆蔻酸酯13-乙酸酯处理转染细胞后,由4.8 kb或3.7 kb启动子驱动的CAT活性并未明显改变。我们的结果表明:1)两种抑制素/激活素βB亚基mRNA是从不同的起始位点转录而来;2)两种启动子可能受上游负调控元件控制;3)在所采用的条件下,这些启动子均对cAMP和/或佛波酯无反应。
