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本文引用的文献

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Three-dimensional quantification of cellular traction forces and mechanosensing of thin substrata by fourier traction force microscopy.利用傅里叶牵引力显微镜对细胞牵引力和薄基底的机械感知进行三维定量。
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Coordination of satellite cell activation and self-renewal by Par-complex-dependent asymmetric activation of p38α/β MAPK.Par 复合物依赖性 p38α/β MAPK 的不对称激活协调卫星细胞的激活和自我更新。
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Building muscle: molecular regulation of myogenesis.肌肉生长:成肌分化的分子调控。
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Mechanical derivation of functional myotubes from adipose-derived stem cells.从脂肪干细胞中机械衍生出功能性肌管。
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Fibroblast polarization is a matrix-rigidity-dependent process controlled by focal adhesion mechanosensing.成纤维细胞极化是一个由黏着斑机械感知控制的依赖于细胞外基质硬度的过程。
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Small molecule inhibition of RISC loading.小分子抑制 RISCs 的加载。
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通过黏着斑蛋白的机械转导调控干细胞分化。

In situ mechanotransduction via vinculin regulates stem cell differentiation.

机构信息

Department of Bioengineering, University of California, San Diego, La Jolla, California, USA.

出版信息

Stem Cells. 2013 Nov;31(11):2467-77. doi: 10.1002/stem.1490.

DOI:10.1002/stem.1490
PMID:23897765
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3833960/
Abstract

Human mesenchymal stem cell (hMSC) proliferation, migration, and differentiation have all been linked to extracellular matrix stiffness, yet the signaling pathway(s) that are necessary for mechanotransduction remain unproven. Vinculin has been implicated as a mechanosensor in vitro, but here we demonstrate its ability to also regulate stem cell behavior, including hMSC differentiation. RNA interference-mediated vinculin knockdown significantly decreased stiffness-induced MyoD, a muscle transcription factor, but not Runx2, an osteoblast transcription factor, and impaired stiffness-mediated migration. A kinase binding accessibility screen predicted a cryptic MAPK1 signaling site in vinculin which could regulate these behaviors. Indeed, reintroduction of vinculin domains into knocked down cells indicated that MAPK1 binding site-containing vinculin constructs were necessary for hMSC expression of MyoD. Vinculin knockdown does not appear to interfere with focal adhesion assembly, significantly alter adhesive properties, or diminish cell traction force generation, indicating that its knockdown only adversely affected MAPK1 signaling. These data provide some of the first evidence that a force-sensitive adhesion protein can regulate stem cell fate.

摘要

人源间充质干细胞(hMSC)的增殖、迁移和分化都与细胞外基质的硬度有关,但机械转导所需的信号通路仍未得到证实。 vinculin 已被证明是体外的机械感受器,但在这里我们证明了它也能够调节干细胞行为,包括 hMSC 的分化。RNA 干扰介导的 vinculin 敲低显著降低了刚度诱导的肌肉转录因子 MyoD,但不降低成骨细胞转录因子 Runx2,并且削弱了刚度诱导的迁移。激酶结合可及性筛选预测 vinculin 中存在一个隐藏的 MAPK1 信号位点,可调节这些行为。事实上,将 vinculin 结构域重新引入敲低的细胞中表明,含有 MAPK1 结合位点的 vinculin 结构域对于 hMSC 中 MyoD 的表达是必需的。vinculin 敲低似乎不会干扰焦点粘连的组装,不会显著改变粘附特性,也不会减少细胞牵引力的产生,这表明其敲低仅对 MAPK1 信号产生不利影响。这些数据提供了一些首次证据表明,力敏黏附蛋白可以调节干细胞命运。