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Whole bone marrow cell culture: A convenient protocol for the in vitro expansion of endothelial progenitor cells

机译:全骨髓细胞培养:体外扩增内皮祖细胞的便捷方案

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摘要

The number and function of endothelial progenitor cells (EPCs) may be a predictive factor for the severity and outcome of cardiovascular disease. However, the manipulation of bone marrow mononuclear cell (BMMC) cultures for EPCs is an elaborate and difficult procedure in small experimental animals. The present study aimed to assess the feasibility of whole bone marrow cell (WBMC) culture for expanding EPCs in small experimental animals. C57BL/6 mice (age, 3–4 weeks; weight, 9.47±0.76 g) were used as the experimental animals, and WBMCs were isolated from the femora and tibiae and cultured in endothelial cell growth medium-2. A BMMC culture for EPCs was used as a control. EPC growth, phenotype and functions were assessed in vitro and in vivo. The results demonstrated that EPCs were easily obtained from a WBMC culture in vitro. The cells exhibited similar growth and biological characteristics when compared with the EPCs derived from the traditional BMMC culture system. Thus, the cells were able to simultaneously bind to lectin and cause phagocytosis of acetylated-low density lipoproteins. In addition, the cells exhibited high expression levels of cluster of differentiation 34 and fetal liver kinase 1, and possessed similar functional properties to BMMC-derived EPCs, including vascular network formation, proliferation, adhesion and migration abilities in vitro. Thus, WBMC-derived EPCs can improve the outcome of pulmonary vascular disease when transplanted into a monocrotaline-induced pulmonary hypertension mouse model. The results of the present study indicated that the WBMC culture system is a more convenient and effective method of obtaining and expanding EPCs compared with BMMC culture, with the advantage of a simplified procedure.
机译:内皮祖细胞(EPC)的数量和功能可能是心血管疾病严重程度和预后的预测因素。但是,在小型实验动物中,对EPC进行骨髓单核细胞(BMMC)培养的操作是一个复杂而困难的过程。本研究旨在评估全骨髓细胞(WBMC)培养在小型实验动物中扩展EPC的可行性。使用C57BL / 6小鼠(3-4周;体重9.47±0.76 g)作为实验动物,从股骨和胫骨中分离WBMC,并在内皮细胞生长培养基2中培养。用于EPC的BMMC培养用作对照。在体外和体内评估EPC的生长,表型和功能。结果表明,EPCs很容易从体外WBMC培养物中获得。与源自传统BMMC培养系统的EPC相比,这些细胞具有相似的生长和生物学特性。因此,细胞能够同时结合凝集素并引起乙酰化低密度脂蛋白的吞噬作用。另外,这些细胞表现出高表达水平的分化簇34和胎儿肝激酶1,并且具有与BMMC衍生的EPC相似的功能特性,包括体外的血管网形成,增殖,粘附和迁移能力。因此,当将WBMC衍生的EPC移植到单芥子碱诱导的肺动脉高压小鼠模型中时,可以改善肺血管疾病的预后。本研究结果表明,与BMMC培养相比,WBMC培养系统是一种更便捷,有效的获取和扩展EPC的方法,其优点是程序简化。

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