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Msx2在哺乳动物肌管中的异位表达概括了两栖动物肌肉去分化的某些方面。

Ectopic expression of Msx2 in mammalian myotubes recapitulates aspects of amphibian muscle dedifferentiation.

作者信息

Yilmaz Atilgan, Engeler Rachel, Constantinescu Simona, Kokkaliaris Konstantinos D, Dimitrakopoulos Christos, Schroeder Timm, Beerenwinkel Niko, Paro Renato

机构信息

Department of Biosystems Science and Engineering, ETH Zürich, Mattenstrasse 26, Basel 4058, Switzerland.

Department of Biosystems Science and Engineering, ETH Zürich, Mattenstrasse 26, Basel 4058, Switzerland.

出版信息

Stem Cell Res. 2015 Nov;15(3):542-553. doi: 10.1016/j.scr.2015.09.012. Epub 2015 Sep 30.

DOI:10.1016/j.scr.2015.09.012
PMID:26468601
Abstract

In contrast to urodele amphibians and teleost fish, mammals lack the regenerative responses to replace large body parts. Amphibian and fish regeneration uses dedifferentiation, i.e., reversal of differentiated state, as a means to produce progenitor cells to eventually replace damaged tissues. Therefore, induced activation of dedifferentiation responses in mammalian tissues holds an immense promise for regenerative medicine. Here we demonstrate that ectopic expression of Msx2 in cultured mouse myotubes recapitulates several aspects of amphibian muscle dedifferentiation. We found that MSX2, but not MSX1, leads to cellularization of myotubes and downregulates the expression of myotube markers, such as MHC, MRF4 and myogenin. RNA sequencing of myotubes ectopically expressing Msx2 showed downregulation of over 500 myotube-enriched transcripts and upregulation of over 300 myoblast-enriched transcripts. MSX2 selectively downregulated expression of Ptgs2 and Ptger4, two members of the prostaglandin pathway with important roles in myoblast fusion during muscle differentiation. Ectopic expression of Msx2, as well as Msx1, induced partial cell cycle re-entry of myotubes by upregulating CyclinD1 expression but failed to initiate S-phase. Finally, MSX2-induced dedifferentiation in mouse myotubes could be recapitulated by a pharmacological treatment with trichostatin A (TSA), bone morphogenetic protein 4 (BMP4) and fibroblast growth factor 1 (FGF1). Together, these observations indicate that MSX2 is a major driver of dedifferentiation in mammalian muscle cells.

摘要

与有尾两栖动物和硬骨鱼不同,哺乳动物缺乏替换大型身体部位的再生反应。两栖动物和鱼类的再生利用去分化,即分化状态的逆转,作为产生祖细胞以最终替换受损组织的一种方式。因此,在哺乳动物组织中诱导激活去分化反应对再生医学具有巨大的前景。在这里,我们证明在培养的小鼠肌管中异位表达Msx2概括了两栖动物肌肉去分化的几个方面。我们发现,MSX2而非MSX1导致肌管细胞化,并下调肌管标记物如MHC、MRF4和肌细胞生成素的表达。对异位表达Msx2的肌管进行RNA测序显示,超过500个富含肌管的转录本下调,超过300个富含成肌细胞的转录本上调。MSX2选择性下调Ptgs2和Ptger4的表达,这两个前列腺素途径成员在肌肉分化过程中的成肌细胞融合中起重要作用。Msx2以及Msx1的异位表达通过上调细胞周期蛋白D1的表达诱导肌管部分重新进入细胞周期,但未能启动S期。最后,用曲古抑菌素A(TSA)、骨形态发生蛋白4(BMP4)和成纤维细胞生长因子1(FGF1)进行药物处理可以重现MSX2诱导的小鼠肌管去分化。总之,这些观察结果表明MSX2是哺乳动物肌肉细胞去分化的主要驱动因素。

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