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从海洋鱼类真鲷中分析肌肉生长抑制素 2 启动子等位基因的结构和功能:具有很强的肌肉特异性启动子活性和转录后调控的证据。

Structural and functional analysis of myostatin-2 promoter alleles from the marine fish Sparus aurata: evidence for strong muscle-specific promoter activity and post-transcriptional regulation.

机构信息

Department of Marine Biology & Biotechnology, National Institute of Oceanography, Israel Oceanographic and Limnological Research, Tel-Shikmona, Haifa, Israel.

出版信息

Mol Cell Endocrinol. 2012 Sep 25;361(1-2):51-68. doi: 10.1016/j.mce.2012.03.017. Epub 2012 Mar 29.

DOI:10.1016/j.mce.2012.03.017
PMID:22483947
Abstract

Myostatin (MSTN) is a negative regulator of skeletal muscle growth. In contrast to mammals, fish possess at least two paralogs of MSTN: MSTN-1 and MSTN-2. In this study, we analyzed the structural-functional features of the four variants of Sparus aurata MSTN-2 5'-flanking region: saMSTN-2a, saMSTN-2as, saMSTN-2b and saMSTN-2c. In silico analysis revealed numerous putative cis regulatory elements including several E-boxes known as binding sites to myogenic transcription factors. Transient transfection experiments using non-muscle and muscle cell lines showed surprisingly high transcriptional activity in muscle cells, suggesting the presence of regulatory elements unique to differentiated myotubes. These observations were confirmed by in situ intramuscular injections of promoter DNA followed by reporter gene assays. Moreover, high promoter activity was found in differentiated neural cell, in agreement with MSTN-2 expression in brain. Progressive 5'-deletion analysis, using reporter gene assays, showed that the core promoter is located within the first -127 bp upstream of the ATG, and suggested the presence of regulatory elements that either repress or induce transcriptional activity. Transient transgenic zebrafish provided evidence for saMSTN-2 promoter ability to direct GFP expression to myofibers. Finally, our data shows that although no mature saMSTN-2 mRNA is observed in muscle; unspliced forms accumulate, confirming high level of transcription. In conclusion, our study shows for the first time that MSTN-2 promoter is a very robust promoter, especially in muscle cells.

摘要

肌肉生长抑制素 (MSTN) 是一种负调控骨骼肌生长的因子。与哺乳动物不同,鱼类至少拥有两种 MSTN 的 paralogs:MSTN-1 和 MSTN-2。在本研究中,我们分析了 Sparus aurata MSTN-2 5'侧翼区的四个变体:saMSTN-2a、saMSTN-2as、saMSTN-2b 和 saMSTN-2c 的结构功能特征。通过计算机分析,发现了许多可能的顺式调控元件,包括几个 E-box,这些是结合到肌源性转录因子的结合位点。使用非肌肉和肌肉细胞系进行的瞬时转染实验显示,肌肉细胞中的转录活性非常高,这表明存在仅存在于分化的肌管中的调控元件。这些观察结果通过肌肉内原位注射启动子 DNA 并进行报告基因分析得到了证实。此外,在分化的神经细胞中也发现了高启动子活性,这与大脑中 MSTN-2 的表达一致。使用报告基因分析的逐步 5'缺失分析表明,核心启动子位于 ATG 上游的第一个 -127bp 内,并且存在抑制或诱导转录活性的调控元件。瞬时转基因斑马鱼提供了证据,证明 saMSTN-2 启动子能够将 GFP 表达导向肌纤维。最后,我们的数据表明,尽管在肌肉中未观察到成熟的 saMSTN-2 mRNA;但未剪接的形式积累,证实了高水平的转录。总之,我们的研究首次表明,MSTN-2 启动子是一个非常强大的启动子,尤其是在肌肉细胞中。

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