Optimizing a 3D model system for molecular manipulation of tenogenesis

被引:14
|
作者
Chien, Chun [1 ]
Pryce, Brian [2 ]
Tufa, Sara F. [2 ]
Keene, Douglas R. [2 ]
Huang, Alice H. [1 ]
机构
[1] Icahn Sch Med Mt Sinai, Dept Orthopaed, 1 Gustave Levy Pl,Box 1188, New York, NY 10029 USA
[2] Shriners Hosp Children, Microimaging Ctr, Portland, OR 97201 USA
关键词
Tendon biology; tendon tissue engineering; mouse embryonic fibroblasts; TGF signaling; Smad signaling; MESENCHYMAL STEM-CELLS; TENDON-LIKE TISSUE; IN-VITRO; MECHANICAL STIMULATION; DIFFERENTIATION; GROWTH; REPAIR; GENE; PROGENITORS; CONSTRUCTS;
D O I
10.1080/03008207.2017.1383403
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Purpose: Tendon injuries are clinically challenging due to poor healing. A better understanding of the molecular events that regulate tendon differentiation would improve current strategies for repair. The mouse model system has been instrumental to tendon studies and several key molecules were initially established in mouse. However, the study of gene function has been limited by the absence of a standard in vitro tendon system for efficiently testing multiple mutations, physical manipulations, and mis-expression. The purpose of this study is therefore to establish such a system.Methods: We adapted an existing design for generating three-dimensional (3D) tendon constructs for use with mouse progenitor cells harboring the ScxGFP tendon reporter and the Rosa26-TdTomato Cre reporter. Using these cells, we optimized the parameters for construct formation, inducing tenogenesis via transforming growth factor-2 (TGF2), and genetic recombination via an adenovirus encoding Cre recombinase. Finally, for proof of concept, we used Smad4 floxed cells and tested the robustness of the system for gene knockdown.Results: We found that TGF2 treatment induced a tenogenic phenotype depending on the timing of initiation. Addition of TGF2 after 3D tensioning enhanced tendon differentiation. Interestingly, while TGF2-induced proliferation depended on Smad4, tenogenic parameters such as ScxGFP expression and fibril diameter were independent of Smad4.Conclusions: Our results demonstrate the feasibility of this optimized system for harnessing the power of mouse genetics for in vitro applications.
引用
收藏
页码:295 / 308
页数:14
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