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鉴定小鼠Igf2基因座中的一个远端肌肉增强子。

Characterizing a distal muscle enhancer in the mouse Igf2 locus.

作者信息

Alzhanov Damir, Rotwein Peter

机构信息

Department of Biochemistry and Molecular Biology, Oregon Health & Science University, Portland, Oregon; and.

Department of Biochemistry and Molecular Biology, Oregon Health & Science University, Portland, Oregon; and Department of Biomedical Sciences, Paul L. Foster School of Medicine, Texas Tech University Health Sciences Center, El Paso, Texas

出版信息

Physiol Genomics. 2016 Feb;48(2):167-72. doi: 10.1152/physiolgenomics.00095.2015. Epub 2015 Dec 8.

Abstract

Insulin-like growth factor-2 (IGF2) is highly expressed in skeletal muscle and was identified as a quantitative trait locus for muscle mass. Yet little is known about mechanisms of its regulation in muscle. Recently, a DNA segment found ∼100 kb from the Igf2 gene was identified as a possible muscle transcriptional control element. Here we have developed an in vivo reporter system to assess this putative enhancer by substituting nuclear (n) EGFP for Igf2 coding exons in a bacterial artificial chromosome containing the mouse Igf2 - H19 chromosomal locus. After stable transfection into a mesenchymal stem cell line, individual clones were converted to myoblasts and underwent progressive muscle-specific gene expression and myotube formation in differentiation medium. Transgenic mRNA and nuclear-targeted enhanced green fluorescent protein were produced coincident with endogenous Igf2 mRNA, but only in lines containing an intact distal conserved DNA element. Our results show that a 294 bp DNA fragment containing two E-boxes is a necessary and sufficient long-range enhancer for induction of Igf2 gene transcription during skeletal muscle differentiation and provides a robust experimental platform for its further functional dissection.

摘要

胰岛素样生长因子2(IGF2)在骨骼肌中高表达,并且被确定为肌肉质量的一个数量性状位点。然而,其在肌肉中的调控机制却鲜为人知。最近,一个距离Igf2基因约100 kb的DNA片段被确定为一个可能的肌肉转录控制元件。在此,我们开发了一种体内报告系统,通过在包含小鼠Igf2 - H19染色体位点的细菌人工染色体中用核(n)EGFP替代Igf2编码外显子,来评估这个假定的增强子。在稳定转染到间充质干细胞系后,单个克隆被转化为成肌细胞,并在分化培养基中经历逐步的肌肉特异性基因表达和肌管形成。转基因mRNA和核靶向增强绿色荧光蛋白与内源性Igf2 mRNA同时产生,但仅在含有完整远端保守DNA元件的细胞系中。我们的结果表明,一个包含两个E盒的294 bp DNA片段是骨骼肌分化过程中诱导Igf2基因转录所必需且充分的长程增强子,并为其进一步的功能剖析提供了一个强大的实验平台。

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