组织特异性细胞外基质增强骨骼肌前体细胞扩增和分化,有望应用于细胞治疗。
Tissue-Specific Extracellular Matrix Enhances Skeletal Muscle Precursor Cell Expansion and Differentiation for Potential Application in Cell Therapy.
作者信息
Zhang Deying, Zhang Yong, Zhang Yuanyuan, Yi Hualin, Wang Zhan, Wu Rongpei, He Dawei, Wei Guanghui, Wei Shicheng, Hu Yun, Deng Junhong, Criswell Tracy, Yoo James, Zhou Yu, Atala Anthony
机构信息
1 Department of Urology, Children's Hospital of Chongqing Medical University , Ministry of Education Key Laboratory of Child Development and Disorders, Chongqing, China .
2 Wake Forest Institute for Regenerative Medicine , Wake Forest School of Medicine, Winston-Salem, North Carolina.
出版信息
Tissue Eng Part A. 2017 Aug;23(15-16):784-794. doi: 10.1089/ten.TEA.2016.0489.
Skeletal muscle precursor cells (MPCs) are considered a key candidate for cell therapy in the treatment of skeletal muscle dysfunction due to injury, disease, or age. However, expansion of a sufficient number of functional skeletal muscle cells in vitro from a small tissue biopsy has been challenging due to changes in phenotypic expression of these cells under traditional culture conditions. Thus, the aim of the study was to develop a better culture system for the expansion and myo-differentiation of MPCs that could further be used for therapy. For this purpose, we developed an ideal method of tissue decellularization and compared the ability of different matrices to support MPC growth and differentiation. Porcine-derived skeletal muscle and liver and kidney extracellular matrix (ECM) were generated by decellularization methods consisting of distilled water, 0.2 mg/mL DNase, or 5% fetal bovine serum. Acellular matrices were further homogenized, dissolved, and combined with a hyaluronic acid-based hydrogel decorated with heparin (ECM-HA-HP). The cell proliferation and myogenic differentiation capacity of human MPCs were assessed when grown on gel alone, ECM, or each ECM-HA-HP substrate. Human MPC proliferation was significantly enhanced when cultured on the ECM-HA-HP substrates compared to the other substrates tested, with the greatest proliferation on the muscle ECM-HA-HP (mECM-HA-HP) substrate. The number of differentiated myotubes was significantly increased on the mECM-HA-HP substrate compared to the other gel-ECM substrates, as well as the numbers of MPCs expressing specific myogenic cell markers (i.e., myosin, desmin, myoD, and myf5). In conclusion, skeletal mECM-HA-HP as a culture substrate provided an optimal culture microenvironment potentially due to its similarity to the in vivo environment. These data suggest a potential use of skeletal muscle-derived ECM gel for the expansion and differentiation of human MPCs for cell-based therapy for skeletal muscle dysfunction.
骨骼肌前体细胞(MPCs)被认为是细胞疗法治疗因损伤、疾病或衰老导致的骨骼肌功能障碍的关键候选细胞。然而,由于这些细胞在传统培养条件下表型表达的变化,从小组织活检中在体外扩增足够数量的功能性骨骼肌细胞一直具有挑战性。因此,本研究的目的是开发一种更好的培养系统,用于MPCs的扩增和肌分化,以便进一步用于治疗。为此,我们开发了一种理想的组织去细胞化方法,并比较了不同基质支持MPCs生长和分化的能力。通过由蒸馏水、0.2mg/mL脱氧核糖核酸酶或5%胎牛血清组成的去细胞化方法生成猪源骨骼肌、肝脏和肾脏细胞外基质(ECM)。脱细胞基质进一步匀浆、溶解,并与用肝素修饰的基于透明质酸的水凝胶(ECM-HA-HP)混合。当人MPCs在单独的凝胶、ECM或每种ECM-HA-HP底物上生长时,评估其细胞增殖和肌源性分化能力。与其他测试底物相比,当在ECM-HA-HP底物上培养时,人MPCs的增殖显著增强,在肌肉ECM-HA-HP(mECM-HA-HP)底物上增殖最大。与其他凝胶-ECM底物相比,在mECM-HA-HP底物上分化的肌管数量显著增加,以及表达特定肌源性细胞标志物(即肌球蛋白、结蛋白、肌分化蛋白和肌因子5)的MPCs数量也显著增加。总之,骨骼肌mECM-HA-HP作为培养底物可能由于其与体内环境的相似性而提供了最佳的培养微环境。这些数据表明骨骼肌衍生的ECM凝胶在用于人MPCs的扩增和分化以用于骨骼肌功能障碍的基于细胞的治疗方面具有潜在用途。
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