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Development of an optimized protocol for primary culture of smooth muscle cells from rat thoracic aortas

机译:开发用于大鼠胸主动脉平滑肌细胞原代培养的优化方案

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Primary culture of smooth muscle cells has been widely used as a valuable tool to study the molecular mechanisms underlying atherosclerosis and restenosis. Currently, tissue explants and enzymatic digestion methods are frequently applied to produce smooth muscle cells. Explants method is time consuming, usually taking several weeks. The enzymatic digestion method requires large amounts of proteolytic enzymes to generate enough cells for cardiovascular research. The present study reports an optimized method by combining both techniques to obtain high purity smooth muscle cells. The cultured cells exhibited the characteristic “hills and valleys” growth pattern as observed by phase contrast microscopy and showed α-SM-actin positive staining by indirect immunocytochemistry and immunofluorescence. Purity of the cells is guaranteed by the lack of von Willebrand Factor immunoreactivity. Finally, the cultured cells well proliferate on oxidized-LDL stimulation, suggesting the practical utility of this new method.
机译:平滑肌细胞的原代培养已广泛用作研究动脉粥样硬化和再狭窄的分子机制的有价值的工具。当前,组织外植体和酶消化方法经常用于产生平滑肌细胞。外植体方法耗时,通常需要数周时间。酶消化方法需要大量的蛋白水解酶才能产生足够的细胞用于心血管研究。本研究报告了一种通过结合两种技术以获得高纯度平滑肌细胞的优化方法。通过相差显微镜观察,培养的细胞表现出特征性的“丘陵和山谷”生长模式,并通过间接免疫细胞化学和免疫荧光显示α-SM-肌动蛋白阳性染色。缺乏von Willebrand因子免疫反应性可确保细胞纯度。最后,培养的细胞在氧化的LDL刺激下能很好地增殖,表明该新方法的实用性。

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