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双轴细胞刺激:一项力学验证。

Biaxial cell stimulation: A mechanical validation.

作者信息

Bieler F H, Ott C E, Thompson M S, Seidel R, Ahrens S, Epari D R, Wilkening U, Schaser K D, Mundlos S, Duda G N

机构信息

Julius Wolff Institut and Center for Musculoskeletal Surgery, Berlin/Brandenburg Center for Regenerative Therapies, Charité - Universitätsmedizin Berlin, 13353 Berlin, Germany.

出版信息

J Biomech. 2009 Aug 7;42(11):1692-6. doi: 10.1016/j.jbiomech.2009.04.013. Epub 2009 May 15.

Abstract

To analyse mechanotransduction resulting from tensile loading under defined conditions, various devices for in vitro cell stimulation have been developed. This work aimed to determine the strain distribution on the membrane of a commercially available device and its consistency with rising cycle numbers, as well as the amount of strain transferred to adherent cells. The strains and their behaviour within the stimulation device were determined using digital image correlation (DIC). The strain transferred to cells was measured on eGFP-transfected bone marrow-derived cells imaged with a fluorescence microscope. The analysis was performed by determining the coordinates of prominent positions on the cells, calculating vectors between the coordinates and their length changes with increasing applied tensile strain. The stimulation device was found to apply homogeneous (mean of standard deviations approx. 2% of mean strain) and reproducible strains in the central well area. However, on average, only half of the applied strain was transferred to the bone marrow-derived cells. Furthermore, the strain measured within the device increased significantly with an increasing number of cycles while the membrane's Young's modulus decreased, indicating permanent changes in the material during extended use. Thus, strain magnitudes do not match the system readout and results require careful interpretation, especially at high cycle numbers.

摘要

为了分析在特定条件下拉伸加载产生的力传导,已开发出各种用于体外细胞刺激的装置。这项工作旨在确定一种市售装置膜上的应变分布及其随循环次数增加的一致性,以及传递给贴壁细胞的应变量。使用数字图像相关技术(DIC)确定刺激装置内的应变及其行为。在用荧光显微镜成像的eGFP转染骨髓来源细胞上测量传递给细胞的应变。通过确定细胞上突出位置的坐标、计算坐标之间的向量及其随施加拉伸应变增加的长度变化来进行分析。发现刺激装置在中心孔区域施加均匀(标准偏差平均值约为平均应变的2%)且可重复的应变。然而,平均而言,仅一半的施加应变传递给了骨髓来源细胞。此外,装置内测量的应变随循环次数增加而显著增加,而膜的杨氏模量降低,表明在长期使用过程中材料发生了永久性变化。因此,应变大小与系统读数不匹配,结果需要仔细解读,尤其是在高循环次数时。

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