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The proangiogenic effects of extracellular vesicles secreted by dental pulp stem cells derived from periodontally compromised teeth

机译:牙髓牙髓干细胞分泌细胞外囊泡的致粒细胞囊泡源自牙周损伤牙齿

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摘要

Abstract Background Although dental pulp stem cells (DPSCs) isolated from periodontally compromised teeth (P-DPSCs) have been demonstrated to retain pluripotency and regenerative potential, their use as therapeutics remains largely unexplored. In this study, we investigated the proangiogenic effects of extracellular vesicles (EVs) secreted by P-DPSCs using in vitro and in vivo testing models. Methods Patient-matched DPSCs derived from periodontally healthy teeth (H-DPSCs) were used as the control for P-DPSCs. Conditioned media (CMs) derived from H-DPSCs and P-DPSCs (H-CM and P-CM), CMs derived from both cell types pretreated with the EV secretion blocker GW4869 (H-GW and P-GW), and EVs secreted by H-DPSCs and P-DPSCs (H-EVs and P-EVs) were prepared to test their proangiogenic effects on endothelial cells (ECs). Cell proliferation, migration, and tube formation were assessed using the Cell Counting Kit-8 (CCK-8), transwell/scratch wound healing, and Matrigel assays, respectively. Specifically, quantitative reverse transcriptase-polymerase chain reaction (qRT-PCR) and western blot analysis were used to examine the expression levels of angiogenesis-related genes/proteins in ECs in response to EV-based incubation. Finally, a full-thickness skin defect model was applied to test the effects of EVs on wound healing and new vessel formation. Results Both H-CM and P-CM promoted EC angiogenesis, but the proangiogenic effects were compromised when ECs were incubated in H-GW and P-GW, wherein the EV secretion was blocked by pretreatment with GW4869. In EV-based incubations, although both H-EVs and P-EVs were found to enhance the angiogenesis-related activities of ECs, P-EVs exerted a more robust potential to stimulate EC proliferation, migration, and tube formation. In addition, P-EVs led to higher expression levels of angiogenesis-related genes/proteins in ECs than H-EVs. Similarly, both P-EVs and H-EVs were found to accelerate wound healing and promote vascularization across skin defects in mice, but wounds treated with P-EVs resulted in a quicker healing outcome and enhanced new vessel formation. Conclusions The findings of the present study provide additional evidence that P-DPSCs derived from periodontally diseased teeth represent a potential source of cells for research and therapeutic use. Particularly, the proangiogenic effects of P-EVs suggest that P-DPSCs may be used to promote new vessel formation in cellular therapy and regenerative medicine.
机译:摘要背景虽然已经证明了从牙周损害的牙齿(P-DPSCs)中分离的牙髓干细胞(DPSC)来保持多能性和再生潜力,但它们作为治疗剂的使用仍然很大程度上是未开发的。在这项研究中,我们研究了在体外和体内测试模型中通过P-DPSCs分泌的细胞外囊泡(EVS)的致致囊泡效应。方法使用源自牙周健康牙齿(H-DPSC)的患者匹配的DPSC作为P-DPSC的对照。来自H-DPSCS和P-DPSCS(H-CM和P-CM)的调节培养基(CMS),CMS来自于用EV分泌阻断器GW4869(H-GW和P-GW)的电池类型,以及分泌的EVS通过H-DPSCS和P-DPSC(H-EVS和P-EV)制备在内皮细胞(ECS)上测试它们的常规效应。使用细胞计数试剂盒-8(CCK-8),Transwell /刮伤伤口愈合和基质胶测定来评估细胞增殖,迁移和管形成。具体地,定量逆转录酶聚合酶链反应(QRT-PCR)和Western印迹分析用于检查ECS中ECS中血管生成相关基因/蛋白的表达水平,响应于EV基孵育。最后,应用全厚的皮肤缺陷模型来测试EVS对伤口愈合和新血管形成的影响。结果H-CM和P-CM促进EC血管生成,但是当EC在H-GW和P-GW中孵育EC时,所述致剂作用受到损害,其中通过用GW4869预处理阻止了EV分泌。在EV基孵育中,虽然发现H-EVS和P-EV均得到增强ECS的血管生成相关活动,但P-EV施加更强大的刺激EC增殖,迁移和管形成。此外,P-EVS导致ECS中血管生成相关基因/蛋白的表达水平高于H-EVS。同样,发现P-eV和H-EV均在伤口愈合和促进小鼠皮肤缺陷的血管形成,但用P-EVS处理的伤口导致更快的愈合结果和增强的新血管形成。结论本研究的结果提供了额外的证据,即源自牙周病患者的P-DPSCs代表了用于研究和治疗用途的潜在细胞来源。特别是,P-EVS的常规效应表明P-DPSC可用于促进细胞疗法和再生医学中的新血管形成。

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