具有不同 Hox 基因表达谱的两种干细胞来源在软骨分化过程中对氯化钴处理的可塑性比较

Biology Pub Date : 2024-07-24 DOI:10.3390/biology13080560
S. Khajeh, V. Razban, Y. Naeimzadeh, Elham Nadimi, R. Asadi-Golshan, Zahra Heidari, Tahereh Talaei-Khozani, Farzaneh Dehghani, Z. Mostafavi-Pour, M. Shirali
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引用次数: 0

摘要

关节软骨的自我修复能力有限,是治愈损伤的一大挑战。虽然间充质干/基质细胞(MSCs)是一种很有前景的组织再生方法,但选择合适细胞来源的标准仍未确定。为了提出一种分子标准,我们采用两步方案,在三维颗粒中将Hox表达阴性的牙髓干细胞(DPSCs)和Hox基因表达活跃的骨髓间充质基质细胞(BMSCs)向软骨细胞分化。通过形态学、组织化学、免疫组织化学和生物化学实验,探讨了间充质干细胞对氯化钴(CoCl2)(一种缺氧模拟剂)预处理的反应,以评估软骨分化的效率。预处理后的 DPSC 颗粒显示胶原蛋白 II 和糖胺聚糖(GAGs)水平明显升高,肥大标记物胶原蛋白 X 水平降低。虽然预处理没有改变两种细胞类型的 ALP 特异性活性,但与 BMSCs 颗粒相比,DPSCs 分化颗粒中的 ALP 特异性活性明显较低。这些结果可以解释为,与 BMSCs 相比,DPSCs 具有更高的可塑性,表明其独特的分子特征(包括负 Hox 表达模式)有助于促进软骨分化潜能。因此,DPSCs可被视为未来软骨细胞疗法的理想候选者。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Plasticity Comparison of Two Stem Cell Sources with Different Hox Gene Expression Profiles in Response to Cobalt Chloride Treatment during Chondrogenic Differentiation
The limited self-repair capacity of articular cartilage is a challenge for healing injuries. While mesenchymal stem/stromal cells (MSCs) are a promising approach for tissue regeneration, the criteria for selecting a suitable cell source remain undefined. To propose a molecular criterion, dental pulp stem cells (DPSCs) with a Hox-negative expression pattern and bone marrow mesenchymal stromal cells (BMSCs), which actively express Hox genes, were differentiated towards chondrocytes in 3D pellets, employing a two-step protocol. The MSCs’ response to preconditioning by cobalt chloride (CoCl2), a hypoxia-mimicking agent, was explored in an assessment of the chondrogenic differentiation’s efficiency using morphological, histochemical, immunohistochemical, and biochemical experiments. The preconditioned DPSC pellets exhibited significantly elevated levels of collagen II and glycosaminoglycans (GAGs) and reduced levels of the hypertrophic marker collagen X. No significant effect on GAGs production was observed in the preconditioned BMSC pellets, but collagen II and collagen X levels were elevated. While preconditioning did not modify the ALP specific activity in either cell type, it was notably lower in the DPSCs differentiated pellets compared to their BMSCs counterparts. These results could be interpreted as demonstrating the higher plasticity of DPSCs compared to BMSCs, suggesting the contribution of their unique molecular characteristics, including their negative Hox expression pattern, to promote a chondrogenic differentiation potential. Consequently, DPSCs could be considered compelling candidates for future cartilage cell therapy.
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