Development of a cell culture system loading cyclic mechanical strain to chondrogenic cells

Mechanical stimulation is considered to be one of the major epigenetic factors regulating the metabolism, proliferation, survival and differentiation of cells in the skeletal tissues. It is generally accepted that the cytoskeleton can undergo remodeling in response to mechanical stimuli such as tens...

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Published in:Journal of biotechnology 2008-01, Vol.133 (2), p.231-238
Main Authors: Masuda, Taisuke, Takahashi, Ichiro, Anada, Takahisa, Arai, Fumihito, Fukuda, Toshio, Takano-Yamamoto, Teruko, Suzuki, Osamu
Format: Article
Language:English
Subjects:
Cell Culture Techniques - methods
Cell Line
Chondrocytes - metabolism
Chondrogenic cell
Collagen Type II - genetics
Collagen Type II - metabolism
Compressive Strength
Culture system
Dimethylpolysiloxanes - metabolism
Finite element modeling (FEM)
Gene Expression Regulation
Mechanical strain
Mechanical stress
Polydimethylsiloxane (PDMS)
Stress, Mechanical
Tensile Strength
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Summary:Mechanical stimulation is considered to be one of the major epigenetic factors regulating the metabolism, proliferation, survival and differentiation of cells in the skeletal tissues. It is generally accepted that the cytoskeleton can undergo remodeling in response to mechanical stimuli such as tensile strain or fluid flow. Mechanically induced cell deformation is one of the possible mechanotransduction pathways by which chondrocytes sense and respond to changes in their mechanical environment. Mechanical strain has a variety of effects on the structure and function of their cells in the skeletal tissues, such as chondrocytes, osteoblasts and fibroblasts. However, little is known about the effect of the quality and quantity of mechanical strain and the timing of mechanical loading on the differentiation of these cells. The present study was designed to investigate the effect of the deformation of chondrogenic cells, and cyclic compression using a newly developed culture device, by analyzing mechanobiological response to the differentiating chondrocytes. Cyclic compression between 0 and 22% strains, at 23 μHz was loaded on chondrogenic cell line ATDC5 by seeding in a mass mode on PDMS membrane, assuming direct transfer of cyclic deformation from the membrane to the cells at the same frequency. The compressive strain, induced within the membrane, was characterized based on the analysis of the finite element modeling (FEM). The results showed that the tensile strain inhibits the chondrogenic differentiation of ATDC5 cells, whereas the compressive strain enhances the chondrogenic differentiation, suggesting that the differentiation of the chondrogenic cells could be controlled by the amount and the mode of strain. In conclusion, we have developed a unique strain loading culture system to analyze the effect of various types of mechanical stimulation on various cellular activities.
ISSN:0168-1656
1873-4863
DOI:10.1016/j.jbiotec.2007.08.007