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应用于微流控芯片中的切变应力导致主动脉瓣间质细胞表型转化。

Phenotype Transformation of Aortic Valve Interstitial Cells Due to Applied Shear Stresses Within a Microfluidic Chip.

机构信息

Department of Chemical Engineering, Texas Tech University, Lubbock, TX, 79409, USA.

Department of Mechanical Engineering, Texas Tech University, Lubbock, TX, 79409, USA.

出版信息

Ann Biomed Eng. 2017 Oct;45(10):2269-2280. doi: 10.1007/s10439-017-1871-z. Epub 2017 Jun 15.

Abstract

Despite valvular heart diseases constituting a significant medical problem, the acquisition of information describing their pathophysiology remains difficult. Due to valvular size, role and location within the body, there is a need for in vitro systems that can recapitulate disease onset and progression. This study combines the development of an in vitro model and its application in the mechanical stimulation of valvular cell transformation. Specifically, porcine aortic valvular interstitial cells (PAVIC) were cultured on polydimethylsiloxane microfluidic devices with or without exposure to shear stresses. Mechanobiological responses of valvular interstitial cells were evaluated at shear stresses ranging from 0 to 4.26 dyn/cm. When flow rates were higher than 0.78 dyn/cm, cells elongated and aligned with the flow direction. In addition, we found that shear stress enhanced the formation of focal adhesions and up-regulated PAVIC transformation, assessed by increased expression of α-smooth muscle actin and transforming growth factor β. This study reveals a link between the action of shear forces, cell phenotype transformation and focal adhesion formation. This constitutes the first step towards the development of co-cultures (interstitial-endothelial cells) on organ-on-a-chip devices, which will enable studies of the signaling pathways regulating force-induced valvular degeneration in microtissues and potential discovery of valvular degeneration therapies.

摘要

尽管瓣膜性心脏病是一个重大的医学问题,但获取描述其病理生理学的信息仍然很困难。由于瓣膜的大小、在体内的作用和位置,需要有能够重现疾病发生和进展的体外系统。本研究结合了体外模型的开发及其在瓣膜细胞转化的机械刺激中的应用。具体来说,猪主动脉瓣膜间质细胞(PAVIC)在有无剪切力作用下培养在聚二甲基硅氧烷微流控装置上。在 0 至 4.26 dyn/cm 的剪切应力范围内评估瓣膜间质细胞的力学生物学反应。当流速高于 0.78 dyn/cm 时,细胞伸长并沿流动方向排列。此外,我们发现剪切力增强了细胞黏附斑的形成,并通过增加α-平滑肌肌动蛋白和转化生长因子β的表达来上调 PAVIC 转化。本研究揭示了剪切力作用、细胞表型转化和黏附斑形成之间的联系。这是朝着在器官芯片设备上进行间质-内皮细胞共培养发展迈出的第一步,这将使我们能够研究调节微组织中力诱导的瓣膜退化的信号通路,并有可能发现瓣膜退化的治疗方法。

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