肌肉增强子因子2对猪肌肉生长抑制素启动子活性的调节

肌肉生长抑制素(Myostatin,Mstn)是转化生长因子-β超家族的成员,在哺乳动物的骨骼肌生长和分化过程中起负调控作用,其转录调控受到多个基因的影响,其中肌肉增强子因子2(MEF2)是重要的调控因子之一。因此,对猪Mstn启动子上MEF2位点及其作用方式的探讨具有重要意义。首先,通过PCR方法扩增了猪Mstn基因上游1 969 kb的启动子序列,利用生物信息学方法分析该序列包含3个MEF2的结合位点;其次,采用逐步删除的方法获得5个长度不等的启动子,用荧光素酶报告系统评估了它们在小鼠成肌细胞C2C12中的活性。其次,转入含有MEF2结合位点的启动子片段和MEF2C表达载体,可以显著增强启动子活性2～6倍,高表达另一亚型MEF2A则启动子活性没有明显改变。最后,转入MEF2C表达载体,用实时定量PCR和Western blotting方法检测Mstn的转录和蛋白水平的变化,结果发现mRNA升高了2～4倍;在肌管细胞中,蛋白翻译水平也有显著升高。这些结果显示,MEF2C可以通过激活Mstn参与猪肌肉生长和发育阶段的调节。研究为Mstn基因的转录调控提供了有效的作用靶点和效应分子,为进一步探讨Mstn的功能调控提供了一种新的思路。     

Cloning and sequence analysis of myostatin promoter in sheep.

To better understand the structure and function of the myostatin's gene promoter region in sheep, we cloned and sequenced a 1.517 kb fragment containing the 5'-regulatory region of the sheep myostatin gene (GenBank accession number is AY918121). The promoter sequence consists of three TATA boxes, one CAAT box, and eight putative E-boxes. Some putative muscle growth response elements for Octamer-binding factor 1(Octamer), Activator protein 1(AP1), Growth factor independence 1 zinc finger protein (Gfi-1B), Myocyte enhancer factor 2 (MEF2), Muscle-specific Mt binding site (MTBF), Glucocorticoid response elements (GRE) and Progesterone receptor binding site (PRE) were detected. Some of the motifs are conserved as compared to with that in the goat, bovine and porcine myostatin promoters. However, some differences were also found.     

The myostatin gene is a downstream target gene of basic helix-loop-helix transcription factor MyoD

Myostatin is a negative regulator of myogenesis, and inactivation of myostatin leads to heavy muscle growth. Here we have cloned and characterized the bovine myostatin gene promoter. Alignment of the upstream sequences shows that the myostatin promoter is highly conserved during evolution. Sequence analysis of 1.6 kb of the bovine myostatin gene upstream region revealed that it contains 10 E-box motifs (E1 to E10), arranged in three clusters, and a single MEF2 site. Deletion and mutation analysis of the myostatin gene promoter showed that out of three important E boxes (E3, E4, and E6) of the proximal cluster, E6 plays a significant role in the regulation of a reporter gene in C(2)C(12) cells. We also demonstrate by band shift and chromatin immunoprecipitation assay that the E6 E-box motif binds to MyoD in vitro and in vivo. Furthermore, cotransfection experiments indicate that among the myogenic regulatory factors, MyoD preferentially up-regulates myostatin promoter activity. Since MyoD expression varies during the myoblast cell cycle, we analyzed the myostatin promoter activity in synchronized myoblasts and quiescent "reserve" cells. Our results suggest that myostatin promoter activity is relatively higher during the G(1) phase of the cell cycle, when MyoD expression levels are maximal. However, in the reserve cells, which lack MyoD expression, a significant reduction in the myostatin promoter activity is observed. Taken together, these results suggest that the myostatin gene is a downstream target gene of MyoD. Since the myostatin gene is implicated in controlling G(1)-to-S progression of myoblasts, MyoD could be triggering myoblast withdrawal from the cell cycle by regulating myostatin gene expression.