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首页> 外文期刊>Frontiers in Cardiovascular Medicine >Stem Cell Cytoskeletal Responses to Pulsatile Flow in Heart Valve Tissue Engineering Studies
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Stem Cell Cytoskeletal Responses to Pulsatile Flow in Heart Valve Tissue Engineering Studies

机译:在心脏瓣膜组织工程研究中干细胞对搏动流的细胞骨架反应

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Heart valve replacement options remain exceedingly limited for pediatric patients because they cannot accommodate somatic growth. To overcome this shortcoming, heart valve tissue engineering using human bone marrow stem cells (HBMSCs) has been considered a potential solution to the treatment of critical congenital valvular defects. The mechanical environments during in vitro culture are key regulators of progenitor cell fate. Here, we report on alterations in HBMSCs, specifically in their actin cytoskeleton and their nucleus under fluid-induced shear stresses of relevance to heart valves. HBMSCs were seeded in microfluidic channels and were exposed to the following conditions: pulsatile shear stress (PSS), steady shear stress (SS), and no flow controls (n = 4/group). Changes to the actin filament structure were monitored and subsequent gene expression was evaluated. A significant increase (p < 0.05) in the number of actin filaments, filament density and angle (between 30° and 84°), and conversely a significant decrease (p < 0.05) in the length of the filaments were observed when the HBMSCs were exposed to PSS for 48 h compared to SS and no flow conditions. No significant differences in nuclear shape were observed among the groups (p > 0.05). Of particular relevance to valvulogenesis, klf2a, a critical gene in valve development, was significantly expressed only by the PSS group (p < 0.05). We conclude that HBMSCs respond to PSS by alterations to their actin filament structure that are distinct from SS and no flow conditions. These changes coupled with the subsequent gene expression findings suggest that at the cellular level, the immediate effect of PSS is to initiate a unique set of quantifiable cytoskeletal events (increased actin filament number, density and angle, but decrease in filament length) in stem cells, which could be useful in the fine-tuning of in vitro protocols in heart valve tissue engineering.
机译:对于小儿患者,心脏瓣膜置换术仍然非常受限制,因为它们不能适应体细胞的生长。为了克服这个缺点,使用人骨髓干细胞(HBMSC)的心脏瓣膜组织工程被认为是治疗关键先天性瓣膜缺损的潜在解决方案。体外培养过程中的机械环境是祖细胞命运的关键调节器。在这里,我们报道了在流体诱导的与心脏瓣膜相关的切应力作用下,HBMSCs,特别是肌动蛋白细胞骨架和细胞核的改变。 HBMSCs接种在微流体通道中,并暴露于以下条件:搏动剪切应力(PSS),稳态剪切应力(SS)和无流量控制(n = 4 /组)。监测肌动蛋白丝结构的变化,并评估随后的基因表达。当HBMSCs出现时,肌动蛋白细丝的数目,细丝密度和角度(在30°和84°之间)显着增加(p <0.05),相反,细丝长度显着减少(p <0.05)。与SS和无流动条件相比,暴露于PSS 48小时。各组之间未观察到核形状的显着差异(p> 0.05)。与瓣膜形成特别相关的是,瓣膜发育中的关键基因klf2a仅由PSS组显着表达(p <0.05)。我们得出的结论是,HBMSC通过改变其肌动蛋白丝结构来应对PSS,这不同于SS,并且没有流动条件。这些变化以及随后的基因表达发现表明,在细胞水平上,PSS的即时作用是引发干细胞中独特的一组可量化的细胞骨架事件(肌动蛋白丝数,密度和角度增加,但丝长度减少) ,这可能有助于微调心脏瓣膜组织工程中的体外方案。

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