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首页> 外文期刊>European Biophysics Journal >Cell adhesion monitoring using a quartz crystal microbalance: comparative analysis of different mammalian cell lines.
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Cell adhesion monitoring using a quartz crystal microbalance: comparative analysis of different mammalian cell lines.

机译:使用石英晶体微量天平监测细胞粘附:不同哺乳动物细胞系的比较分析。

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摘要

The quartz crystal microbalance (QCM) has been widely accepted as a sensitive technique to follow adsorption processes in gas as well as in liquid environments. However, there are only a few reports about the use of this technique to monitor the attachment and spreading of mammalian cells onto a solid support in culture. Using a QCM-setup we investigated the time course of cell attachment and spreading as a function of seeding density for three widespread and frequently used cell lines (MDCK strains I and II and Swiss 3T3-fibroblasts). Results were found to be in good agreement with the geometrical properties of the individual cell types. The shifts of the resonance frequency associated with confluent cell layers on top of the quartz resonators were found to be dependent on the cell species [MDCK-I: (320 +/- 20) Hz; MDCK-II: (530 +/- 25) Hz; 3T3: (240 +/- 15) Hz] reflecting their individual influence on the shear oscillation of the resonator. These findings are discussed with respect to the basic models of materials in contact with an oscillating quartz resonator. We furthermore showed by inhibition-assays using soluble RGD-related peptides, that only specific, integrin mediated cell adhesion is detected using this QCM approach, whereas the sole presence of the cellular body in close vicinity to the resonator surface is barely detectable.
机译:石英晶体微天平(QCM)已被广泛接受为在气体以及液体环境中跟踪吸附过程的灵敏技术。但是,关于使用该技术监测哺乳动物细胞在培养中固相支持物上的附着和扩散的报道很少。使用QCM设置,我们调查了三种广泛使用的常用细胞系(MDCK I和II菌株以及Swiss 3T3-成纤维细胞)的细胞附着和扩散随播种密度变化的时间过程。发现结果与单个细胞类型的几何特性非常吻合。发现与石英谐振器顶部的汇合的细胞层相关的谐振频率的变化取决于细胞的种类[MDCK-1:(320 +/- 20)Hz; MSCK-1:(320 +/- 20)Hz;和(MDCK-1)。 MDCK-II:(530 +/- 25)Hz; 3T3:(240 +/- 15)Hz]反映了它们对谐振器剪切振荡的单独影响。关于与振荡石英谐振器接触的材料的基本模型讨论了这些发现。我们还通过使用可溶性RGD相关肽的抑制试验表明,使用这种QCM方法只能检测到特异性的整合素介导的细胞粘附,而几乎无法检测到共振器表面附近唯一的细胞体。

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