负载 LPS-hUCMSC-sEV 的支架可促进 hDPSCs 的骨/牙源性分化和血管生成潜能

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-08-30 DOI:10.1016/j.tice.2024.102549
Jingjie Zeng , Huidan Deng , Quanjie Li , Jingyi Kang , Yu Wu
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引用次数: 0

摘要

目的 牙本质-牙髓复合体的形成决定了牙髓治疗的成败。人脐带间充质干细胞衍生的细胞外小泡(hUCMSC-sEVs)似乎具有更强的抗炎、促进牙髓干细胞(hDPSCs)增殖和迁移的作用。此外,脂多糖(LPS)预处理可增强细胞外囊泡的抗炎作用。经 LPS 预处理的 hUCMSC-sEVs 有可能通过招募 hDPSCs 来再生牙本质-牙髓复合体。本文旨在开发负载 LPS 预处理 hUCMSC-sEVs 的海绵胶原/自组装肽纳米纤维支架(CS/SAPNS)复合支架(CS/SAPNS-sEVs),并评估 hUCMSC-sEVs 的释放特性以及该复合支架对 hDPSCs 成骨/成髓分化和血管生成潜能的影响。方法将经 LPS 预处理的 hUCMSC-sEVs(LPS-hUCMSC-sEVs)与自组装肽水凝胶混合并负载到海绵胶原上,得到 CS/SAPNS-sEVs。利用 BCA 检测、纳米颗粒分析、透射电子显微镜和激光共聚焦显微镜研究了负载在 CS/SAPNS 上的 LPS-hUCMSC-sEVs 的特性。通过 ALP 染色和茜素红染色分析了 hDPSCs 的骨/牙源性分化能力。结果CS/SAPNS可控制LPS-hUCMSC-sEVs释放7天,并保持其结构的完整性。CS/SAPNS-sEVs 促进了 hDPSCs 中钙化结节的沉积以及成骨/牙生成因子和血管生成因子的表达。结论CS/SNAPS 可用作 LPS-hUCMSC-sEVs 的支架,CS/SAPNS-sEVs 可通过激活 NF-κB 通路促进 hDPSCs 的成骨/成牙分化并增强其血管生成潜能。
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Scaffold loaded LPS-hUCMSC-sEVs promote Osteo/odontogenic differentiation and angiogenic potential of hDPSCs

Objective

The formation of dentin-pulp complex determines the success of vital pulp therapy. Human umbilical cord mesenchymal stem cell-derived small extracellular vesicles (hUCMSC-sEVs) appeared to have stronger effect in anti-inflammatory and promoting the proliferation and migration of human dental pulp stem cells (hDPSCs). Moreover, Lipopolysaccharides (LPS) pretreatment can enhance the rapeutic potency of extracellular vesicles. LPS pretreatment hUCMSC-sEVs have the potential to regenerate the dentin-pulp complex by recruiting hDPSCs. This paper aims to develop collagen sponge/self-assembling peptide nanofiber scaffold (CS/SAPNS) composite scaffold loaded with LPS pretreatment hUCMSC-sEVs (CS/SAPNS-sEVs), and assess the release characteristics of hUCMSC-sEVs and the effect of this composite scaffold on osteo/odontogenic differentiation and angiogenic potential in hDPSCs.

Methods

LPS pretreatment hUCMSC-sEVs (LPS-hUCMSC-sEVs) were mixed with self-assembling peptide hydrogel and loaded onto collagen sponge to obtain the CS/SAPNS-sEVs. BCA assay, nanoparticle analysis, transmission electron microscopy and laser confocal microscopy were used to investigate the characteristics of LPS-hUCMSC-sEVs loaded on CS/SAPNS. Osteo/odontogenic differentiation ability of hDPSCs were analyzed by ALP stainning, alizarin red staining. RT-PCR and Western blot analysis were performed to confirm the levels of osteo/odontogenic factors and angiogenic factors, and the involvement of NF-κB pathway was verified by immunocytochemical staining and Western blot analysis.

Results

CS/SAPNS could control LPS-hUCMSC-sEVs release for 7 days and keep their structural integrity. CS/SAPNS-sEVs promoted deposition of calcified nodules and expression of osteogenic/odontogenic and angiogenic factors in hDPSCs. On the contrary, inhibition of the NF-κB pathway down-regulated the expression of CS/SAPNS-sEVs-regulated osteo/odontogenic and angiogenic factors.

Conclusion

CS/SNAPS could be used as scaffold for LPS-hUCMSC-sEVs, and CS/SAPNS-sEVs may promote osteo/odontogenic differentiation and enhance the angiogenic potential of hDPSCs through activating the NF-κB pathway.

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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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