Tissue Engineering of Functional Trileaflet Heart Valves From Human Marrow Stromal Cells

Circulation: Journal of the American Heart Association Pub Date : 2002-09-24 DOI:10.1161/01.CIR.0000032872.55215.05

S. Hoerstrup, A. Kadner, S. Melnitchouk, A. Trojan, K. Eid, Jay Tracy, R. Sodian, J. Visjager, S. Kolb, J. Grunenfelder, G. Zund, M. Turina

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引用次数: 259

Abstract

BackgroundWe previously demonstrated the successful tissue engineering and implantation of functioning autologous heart valves based on vascular-derived cells. Human marrow stromal cells (MSC) exhibit the potential to differentiate into multiple cell-lineages and can be easily obtained clinically. The feasibility of creating tissue engineered heart valves (TEHV) from MSC as an alternative cell source, and the impact of a biomimetic in vitro environment on tissue differentiation was investigated. Methods and ResultsHuman MSC were isolated, expanded in culture, and characterized by flow-cytometry and immunohistochemistry. Trileaflet heart valves fabricated from rapidly bioabsorbable polymers were seeded with MSC and grown in vitro in a pulsatile-flow-bioreactor. Morphological characterization included histology and electron microscopy (EM). Extracellular matrix (ECM)-formation was analyzed by immunohistochemistry, ECM protein content (collagen, glycosaminoglycan) and cell proliferation (DNA) were biochemically quantified. Biomechanical evaluation was performed using Instron™. In all valves synchronous opening and closing was observed in the bioreactor. Flow-cytometry of MSC pre-seeding was positive for ASMA, vimentin, negative for CD 31, LDL, CD 14. Histology of the TEHV-leaflets demonstrated viable tissue and ECM formation. EM demonstrated cell elements typical of viable, secretionally active myofibroblasts (actin/myosin filaments, collagen fibrils, elastin) and confluent, homogenous tissue surfaces. Collagen types I, III, ASMA, and vimentin were detected in the TEHV-leaflets. Mechanical properties of the TEHV-leaflets were comparable to native tissue. ConclusionGeneration of functional TEHV from human MSC was feasible utilizing a biomimetic in vitro environment. The neo-tissue showed morphological features and mechanical properties of human native-heart-valve tissue. The human MSC demonstrated characteristics of myofibroblast differentiation.

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人骨髓基质细胞三叶心脏瓣膜的组织工程研究

我们之前已经成功地展示了基于血管来源细胞的组织工程和植入功能正常的自体心脏瓣膜。人骨髓基质细胞(MSC)表现出分化为多种细胞系的潜力，在临床上很容易获得。研究了以间充质干细胞作为替代细胞来源制备组织工程心脏瓣膜(tev)的可行性，以及体外仿生环境对组织分化的影响。方法与结果分离人间充质干细胞，培养扩增，用流式细胞术和免疫组织化学对其进行鉴定。用可快速生物吸收的聚合物制备三叶心脏瓣膜，并在体外脉冲流生物反应器中植入MSC。形态学表征包括组织学和电子显微镜。免疫组织化学分析细胞外基质(ECM)的形成，生化定量细胞外基质蛋白(胶原、糖胺聚糖)含量和细胞增殖(DNA)。使用Instron™进行生物力学评价。在生物反应器中观察到所有阀门的同步开启和关闭。流式细胞术检测MSC预接种ASMA、vimentin阳性，cd31、LDL、cd14阴性。tev小叶的组织学显示有活力的组织和ECM的形成。电镜显示有活力的、分泌活跃的肌成纤维细胞(肌动蛋白/肌球蛋白丝、胶原原纤维、弹性蛋白)和融合的、均匀的组织表面的典型细胞成分。在tev小叶中检测到ⅰ型、ⅲ型胶原蛋白、ASMA和波形蛋白。tev -小叶的力学性能与天然组织相当。结论利用体外仿生环境从人骨髓间充质干细胞生成功能tev是可行的。新组织具有人类天然心脏瓣膜组织的形态特征和力学特性。人间充质干细胞表现出肌成纤维细胞分化的特征。

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Circulation: Journal of the American Heart Association

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