Department of Pediatric Dentistry, School and Hospital of Stomatology, China Medical University, Shenyang, China.
Liaoning Province Key Laboratory of Oral Disease, Shenyang, China.
Int Endod J. 2024 Sep;57(9):1279-1292. doi: 10.1111/iej.14099. Epub 2024 Jun 3.
To evaluate the role of biomimetic pulp scaffolds derived from the extracellular matrix derived of stem cells from human exfoliated deciduous teeth (SHED-ECM-PS) in promoting pulp-dentine complex regeneration.
SHED-ECM-PS was prepared through cell aggregation and decellularization techniques. Histological and immunofluorescence analyses, scanning electron microscopy, and DNA quantification assays were used to characterize the SHED-ECM-PS. Additionally, a tooth slice implantation model was established to evaluate the effects of SHED-ECM-PS on regeneration of the pulp-dentine complex in vivo. Extraction medium for SHED-ECM-PS was prepared, and its effect on bone marrow mesenchymal stem cells (BMMSCs) was assessed in vitro. Cell counting kit-8 and Ki-67 staining assays were performed to determine cell proliferation. The rate of apoptosis was evaluated by flow cytometry. Wound healing and transwell assays were conducted to evaluate cell migration. Alizarin red S staining was performed to examine mineralized nodule formation. Western blotting was used to detect the expression of osteogenic and odontogenic markers. The results were analysed using an independent two-tailed Student's t-test. p < .05 was considered statistically significant.
SHED-ECM-PS was successfully constructed, exhibiting a striped dental pulp-like shape devoid of nuclear structures or DNA components, and rich in fibronectin, collagen I, DMP1 and DSPP. Notably, SHED-ECM-PS showed no impact on the proliferation or apoptosis of BMMSCs. Histological analysis revealed that dental pulp fibroblasts formed an interwoven mesh in the root canal, and angiogenesis was observed in the SHED-ECM-PS group. Moreover, a continuous, newly formed tubular dentine layer with polarized odontoblast-like cells was observed along the inner wall of the root canal. SHED-ECM-PS promoted the migration, polar alignment and mineralized nodule formation of BMMSCs and specifically elevated the expression levels of odontogenic markers, but not osteogenic markers, compared with the control group in vitro.
SHED-ECM-PS exhibited no cytotoxicity and promoted pulp-dentine complex regeneration in vivo as well as cell migration and odontogenic differentiation of BMMSCs in vitro. These findings provide evidence that SHED-ECM-PS, as a novel biological scaffold, has the potential to improve the outcomes of REPs.
评估来源于人脱落乳牙干细胞细胞外基质的仿生牙髓支架(SHED-ECM-PS)在促进牙髓-牙本质复合体再生中的作用。
通过细胞聚集和去细胞化技术制备 SHED-ECM-PS。通过组织学和免疫荧光分析、扫描电子显微镜和 DNA 定量分析来表征 SHED-ECM-PS。此外,建立了牙切片植入模型,以评估 SHED-ECM-PS 在体内对牙髓-牙本质复合体再生的影响。制备 SHED-ECM-PS 的提取介质,并在体外评估其对骨髓间充质干细胞(BMMSCs)的作用。通过细胞计数试剂盒-8 和 Ki-67 染色测定来确定细胞增殖。通过流式细胞术评估细胞凋亡率。通过伤口愈合和 Transwell 测定来评估细胞迁移。通过茜素红 S 染色来检测矿化结节形成。通过 Western blot 检测成骨和成牙本质标志物的表达。使用独立的双尾学生 t 检验分析结果。p<.05 被认为具有统计学意义。
成功构建了 SHED-ECM-PS,其呈现出无核结构或 DNA 成分的条纹状牙髓样形状,富含纤维连接蛋白、胶原 I、DMP1 和 DSPP。值得注意的是,SHED-ECM-PS 对 BMMSCs 的增殖或凋亡没有影响。组织学分析显示,牙髓成纤维细胞在根管内形成交织的网状结构,并且在 SHED-ECM-PS 组中观察到血管生成。此外,沿着根管内壁观察到连续的、新形成的具有极化成牙本质样细胞的管状牙本质层。SHED-ECM-PS 促进了 BMMSCs 的迁移、极性排列和矿化结节形成,并在体外特异性地上调了成牙本质标志物的表达水平,而不是成骨标志物的表达水平,与对照组相比。
SHED-ECM-PS 无细胞毒性,可促进体内牙髓-牙本质复合体的再生以及体外 BMMSCs 的细胞迁移和成牙本质分化。这些发现为 SHED-ECM-PS 作为一种新型生物支架有可能改善再生牙本质的疗效提供了证据。
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