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骨髓基质细胞在纳米粗糙钛铝钒表面产生的生长因子通过 BMP2 信号途径将骨髓间充质干细胞编程为成骨细胞。

Growth factors produced by bone marrow stromal cells on nanoroughened titanium-aluminum-vanadium surfaces program distal MSCs into osteoblasts via BMP2 signaling.

机构信息

Department of Biomedical Engineering, Virginia Commonwealth University, Richmond, Virgina, USA.

Department of Periodontology, University of Texas Health Science Center at San Antonio, San Antonio, Texas, USA.

出版信息

J Orthop Res. 2021 Sep;39(9):1908-1920. doi: 10.1002/jor.24869. Epub 2020 Oct 12.

Abstract

Statement of Clinical Significance: There remains the need to develop materials and surfaces that can increase the rate of implant osseointegration. Though osteoanabolic agents, like bone morphogenetic protein (BMP), can provide signaling for osteogenesis, the appropriate design of implants can also produce an innate cellular response that may reduce or eliminate the need to use additional agents to stimulate bone formation. Studies show that titanium implant surfaces that mimic the physical properties of osteoclast resorption pits regulate cellular responses of bone marrow stromal cells (MSCs) by altering cell morphology, transcriptomes, and local factor production to increase their differentiation into osteoblasts without osteogenic media supplements required for differentiation of MSCs on tissue culture polystyrene (TCPS). The goal of this study was to determine how cells in contact with biomimetic implant surfaces regulate the microenvironment around these surfaces in vitro. Two different approaches were used. First, unidirectional signaling was assessed by treating human MSCs grown on TCPS with conditioned media from MSC cultures grown on Ti6Al4V biomimetic surfaces. In the second set of studies, bidirectional signaling was assessed by coculturing MSCs grown on mesh inserts that were placed into culture wells in which MSCs were grown on the biomimetic Ti6Al4V substrates. The results show that biomimetic Ti6Al4V surface properties induce MSCs to produce factors within 7 days of culture that stimulate MSCs not in contact with the surface to exhibit an osteoblast phenotype via endogenous BMP2 acting in a paracrine signaling manner.

摘要

临床意义声明

仍需要开发能够提高植入物骨整合率的材料和表面。尽管骨形态发生蛋白 (BMP) 等成骨剂可以为成骨提供信号,但植入物的适当设计也可以产生固有细胞反应,从而减少或消除使用额外的成骨剂来刺激骨形成的必要性。研究表明,模仿破骨细胞吸收陷窝物理特性的钛植入物表面通过改变细胞形态、转录组和局部因子产生来调节骨髓基质细胞 (MSCs) 的细胞反应,从而增加其分化为成骨细胞的能力,而无需分化组织培养聚苯乙烯 (TCPS) 上的 MSC 所需的成骨介质。本研究的目的是确定与仿生植入物表面接触的细胞如何在体外调节这些表面周围的微环境。采用了两种不同的方法。首先,通过用从在仿生 Ti6Al4V 表面上生长的 MSC 培养物中获得的条件培养基处理在 TCPS 上生长的人 MSC,评估单向信号传导。在第二组研究中,通过将生长在网格插入物上的 MSC 进行共培养来评估双向信号传导,将网格插入物放置在培养孔中,MSC 生长在仿生 Ti6Al4V 基底上。结果表明,仿生 Ti6Al4V 表面特性诱导 MSC 在培养的 7 天内产生因子,这些因子通过内源性 BMP2 以旁分泌信号方式刺激未与表面接触的 MSC 表现出成骨细胞表型。

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