Witkowska-Zimny Malgorzata, Wrobel Edyta, Mrowka Piotr
Department of Biophysics and Human Physiology, Medical University of Warsaw, Poland.
Folia Histochem Cytobiol. 2014;52(4):297-307. doi: 10.5603/FHC.a2014.0031. Epub 2014 Nov 17.
The formation and maintenance of tissues is regulated by various signals triggered by biological, chemical, and physical factors. Data increasingly confirm that matrix or tissue elasticity plays an influential role in regulating numerous cell functions. The aim of the present study was to better understand the regulation of cellular differentiation by mechanical cues. We studied the influence of matrix stiffness on the osteodifferentiation of two cell lineages characterized by different responses: mesenchymal stromal/stem cells isolated from the Wharton's jelly of the umbilical cord (UC-MSCs) with strong stiffness-dependent responses; and bone-derived cells (BDCs), which are insensitive to changes in matrix rigidity. The study also aimed to delineate how matrix stiffness affects intracellular signaling through focal adhesion kinase (FAK) activity—one of the key components in integrin-mediated signaling pathways.
The effect of substrate stiffness on the expression of α2, α5, and β1 integrin was studied using real time PCR and Western blot using cells cultured in an osteogenic medium on tunable polyacrylamide gels coated with type I collagen, with elasticities corresponding to Young's moduli of 1.46 kPa and 26.12 kPa. FAK activity was monitored using ELISA assays.
We demonstrate for the first time the changes in the expression of α2, α5, and β1 integrin subunits in perinatal stem cells and in adult osteoblast precursor cells during in vitro osteogenic differentiation on surfaces characterized by different stiffness. We found that matrix rigidity significantly affects the osteogenic differentiation of UC-MSCs through α2 integrin-mediated mechanotransduction events, though not through the α5 integrin subunit. In BDCs, there were no significant changes in the expression levels of the tested protein associated with varying stiffness.
Our results provide evidence that matrix rigidity affects the osteogenic differentiation of UC-MSCs via mechanotransduction events mediated by α2 integrin subunits.
组织的形成和维持受生物、化学及物理因素触发的各种信号调节。越来越多的数据证实,基质或组织弹性在调节众多细胞功能中发挥着重要作用。本研究的目的是更好地理解机械信号对细胞分化的调节作用。我们研究了基质硬度对两种具有不同反应特征的细胞谱系骨分化的影响:从脐带华通氏胶中分离的间充质基质/干细胞(UC-MSCs),其对硬度有强烈依赖性反应;以及骨源性细胞(BDCs),其对基质刚度变化不敏感。该研究还旨在阐明基质硬度如何通过粘着斑激酶(FAK)活性影响细胞内信号传导,FAK活性是整合素介导的信号通路中的关键成分之一。
使用实时PCR和蛋白质印迹法研究了底物硬度对在涂有I型胶原蛋白的可调聚丙烯酰胺凝胶上培养于成骨培养基中的细胞α2、α5和β1整合素表达的影响,这些凝胶的弹性对应于杨氏模量为1.46 kPa和26.12 kPa。使用酶联免疫吸附测定法监测FAK活性。
我们首次证明了围产期干细胞和成体成骨细胞前体细胞在体外成骨分化过程中,在具有不同硬度的表面上α2、α5和β1整合素亚基表达的变化。我们发现,基质刚度通过α2整合素介导的机械转导事件显著影响UC-MSCs的成骨分化,但不通过α5整合素亚基。在BDCs中,与不同刚度相关的测试蛋白表达水平没有显著变化。
我们的结果提供了证据,表明基质刚度通过α2整合素亚基介导的机械转导事件影响UC-MSCs的成骨分化。
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