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鼠 Wnt1-CRE-Rosa 牙髓干细胞直接参与颅骨骨再生过程。

Mouse Wnt1-CRE-Rosa Dental Pulp Stem Cells Directly Contribute to the Calvarial Bone Regeneration Process.

机构信息

EA 2496 Orofacial Pathologies, Imagery, and Biotherapies, Dental School Faculty, University Paris Descartes, and Life Imaging Platform (PIV), Montrouge, France.

University Hospitals, AP-HP, Paris, France.

出版信息

Stem Cells. 2019 May;37(5):701-711. doi: 10.1002/stem.2973. Epub 2019 Mar 13.

DOI:10.1002/stem.2973
PMID:30674073
Abstract

Stem cells endowed with skeletogenic potentials seeded in specific scaffolds are considered attractive tissue engineering strategies for treating large bone defects. In the context of craniofacial bone, mesenchymal stromal/stem cells derived from the dental pulp (DPSCs) have demonstrated significant osteogenic properties. Their neural crest embryonic origin further makes them a potential accessible therapeutic tool to repair craniofacial bone. The stem cells' direct involvement in the repair process versus a paracrine effect is however still discussed. To clarify this question, we have followed the fate of fluorescent murine DPSCs derived from PN3 Wnt1-CRE- Rosa mouse molar (T-mDPSCs) during the repair process of calvaria bone defects. Two symmetrical critical defects created on each parietal region were filled with (a) dense collagen scaffolds seeded with T-mDPSCs, (b) noncellularized scaffolds, or (c) no scaffold. Mice were imaged over a 3-month period by microcomputed tomography to evaluate the extent of repair and by biphotonic microscopy to track T-mDPSCs. Histological and immunocytochemical analyses were performed in parallel to characterize the nature of the repaired tissue. We show that T-mDPSCs are present up to 3 months postimplantation in the healing defect and that they rapidly differentiate in chondrocyte-like cells expressing all the expected characteristic markers. T-mDPSCs further maturate into hypertrophic chondrocytes and likely signal to host progenitors that form new bone tissue. This demonstrates that implanted T-mDPSCs are able to survive in the defect microenvironment and to participate directly in repair via an endochondral bone ossification-like process. Stem Cells 2019;37:701-711.

摘要

具有成骨潜力的干细胞接种在特定支架中被认为是治疗大骨缺损的有吸引力的组织工程策略。在颅面骨的背景下,来源于牙髓的间充质基质/干细胞(DPSCs)表现出显著的成骨特性。它们的神经嵴胚胎起源进一步使它们成为修复颅面骨的潜在可行治疗工具。然而,干细胞是直接参与修复过程还是旁分泌效应仍存在争议。为了澄清这个问题,我们跟踪了来源于 PN3 Wnt1-CRE- Rosa 鼠磨牙(T-mDPSCs)的荧光鼠 DPSCs 在颅盖骨骨缺损修复过程中的命运。在每个顶骨区域创建两个对称的临界缺损,用(a)接种 T-mDPSCs 的致密胶原支架、(b)非细胞化支架或(c)无支架填充。通过微计算机断层扫描在 3 个月的时间内对小鼠进行成像,以评估修复程度,并通过双光子显微镜跟踪 T-mDPSCs。同时进行组织学和免疫细胞化学分析,以表征修复组织的性质。我们表明,T-mDPSCs 在植入后 3 个月内存在于愈合缺陷中,并且它们迅速分化为表达所有预期特征标志物的软骨细胞样细胞。T-mDPSCs 进一步成熟为肥大软骨细胞,并可能向宿主祖细胞发出信号,形成新的骨组织。这表明植入的 T-mDPSCs 能够在缺陷微环境中存活,并通过类似于软骨内骨化的过程直接参与修复。《干细胞》2019;37:701-711。

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