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ROCK-TAZ 信号轴调控机械张力诱导的大鼠颅顶矢状缝间充质干细胞成骨分化。

ROCK-TAZ signaling axis regulates mechanical tension-induced osteogenic differentiation of rat cranial sagittal suture mesenchymal stem cells.

机构信息

Jiangsu Key Laboratory of Oral Diseases, Nanjing Medical University, Nanjing, China.

Department of Orthodontics, Affiliated Hospital of Stomatology, Nanjing Medical University, Nanjing, China.

出版信息

J Cell Physiol. 2020 Sep;235(9):5972-5984. doi: 10.1002/jcp.29522. Epub 2020 Jan 22.

Abstract

Mechanical force across sutures is able to promote suture osteogenesis. Orthodontic clinics often use this biological characteristic of sutures to treat congenital cranio-maxillofacial malformations. However, the underlying mechanisms still remain poorly understood. Craniofacial sutures provide a special growth source and support primary sites of osteogenesis. Here, we isolated rat sagittal suture cells (rSAGs), which had mesenchymal stem cell characteristics and differentiating abilities. Cells were then subjected to mechanical tension (5% elongation, 0.5 Hz; sinusoidal waveforms) showing that mechanical tension could enhance osteogenic differentiation but hardly affect proliferation of rSAGs. Besides, mechanical tension could increase Rho-associated kinase (ROCK) expression and enhance transcriptional coactivator with PDZ-binding motif (TAZ) nuclear translocation. Inhibiting ROCK expression could suppress tension-induced osteogenesis and block tension-induced upregulation of nuclear TAZ. In addition, our results indicated that TAZ had direct combination sites with runt-related transcription factor 2 (Runx2) in rSAGs, and knock-downed TAZ simultaneously decreased the expression of Runx2 no matter with or without mechanical tension. In summary, our findings demonstrated that the multipotency of rSAGs in vitro could give rise to early osteogenic differentiation under mechanical tension, which was mediated by ROCK-TAZ signal axis.

摘要

机械力可穿过缝线促进缝线成骨。正畸诊所常利用缝线的这一生物学特性来治疗先天性颅面畸形。然而,其潜在机制仍知之甚少。颅面缝线提供了特殊的生长源和主要成骨部位的支撑。在这里,我们分离了具有间充质干细胞特征和分化能力的大鼠矢状缝线细胞(rSAG)。然后对细胞施加机械张力(5%伸长率,0.5 Hz;正弦波),结果表明机械张力可以增强成骨分化,但几乎不影响 rSAG 的增殖。此外,机械张力可以增加 Rho 相关激酶(ROCK)的表达并增强转录共激活因子与 PDZ 结合基序(TAZ)的核易位。抑制 ROCK 表达可抑制张力诱导的成骨作用,并阻断张力诱导的核 TAZ 上调。此外,我们的结果表明,TAZ 在 rSAG 中与 runt 相关转录因子 2(Runx2)具有直接结合位点,并且无论有无机械张力,敲低 TAZ 均可同时降低 Runx2 的表达。总之,我们的研究结果表明,rSAG 在体外的多能性可在机械张力下引发早期成骨分化,这是由 ROCK-TAZ 信号轴介导的。

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