Cardiovascular Innovation Institute, University of Louisville, Louisville, Kentucky 40202, USA.
Tissue Eng Part C Methods. 2013 Apr;19(4):307-15. doi: 10.1089/ten.TEC.2012.0311. Epub 2013 Jan 4.
The three-dimensional culture of blood vessel wall cells now permits the construction of a human blood vessel mimic (BVM). Previous studies have used the human BVM as a tool to perform in vitro testing of medical devices and imaging instrumentation. The purpose of the current study was to enhance this technology through both the elimination of animal serum and the modification of scaffold properties in human BVM preparation. Additionally, BVMs were implanted with vascular stents to observe a potential cellular response to the devices in a serum-free environment. Serum-free culture of human adipose-derived stromal vascular fraction (SVF) cells was accomplished through sequential adaptation from a serum-supplemented medium. The adipose-derived SVF serves as a source of both human endothelium and human smooth muscle cells. Utilizing established pressure-sodding technologies, these cells were incorporated into the luminal surface of either expanded polytetrafluoroethylene (ePTFE) tubular scaffolds or electrospun poly(l-lactide-co-caprolactone) scaffolds, and the resulting constructs were cultivated in a perfusion bioreactor using a serum-free medium. Histological analysis of BVMs created using ePTFE scaffolds indicated that a complete lining of cells had formed on the inner surfaces of the grafts. Vessel mimics were also established under serum-free conditions on the highly porous electrospun tubes, resulting in cellularization throughout the scaffold wall in addition to inner and outer surfaces. Neither endothelial cells nor smooth muscles cells were identified among the mesenchymal cells present in each type of BVM. Bare metal stents were deployed within the electrospun BVMs, and after bioreactor perfusion, scanning electron microscopy and nuclear-specific bisbenzimide staining confirmed the presence of cells on stent surfaces. The outcomes of this study support the hypothesis that BVMs developed using serum-free conditions are affected by scaffold variations and exhibit tissue growth over implanted medical devices. Ultimately, employing serum-free methods could lead to controlled, reproducible BVM production and interpretable, human-specific results in studies of device-tissue interaction, toxicity, and other vascular phenomena; however, comparisons to in vivo biological responses and incorporation of defined blood vessel cells will be critical to validating the serum-free BVM as an appropriate device testing alternative.
血管壁细胞的三维培养现在允许构建人类血管模拟物(BVM)。以前的研究使用人类 BVM 作为工具,对医疗器械和成像仪器进行体外测试。本研究的目的是通过消除动物血清和修饰人 BVM 制备中的支架特性来增强这项技术。此外,将血管支架植入 BVM 中,以观察无血清环境下对设备的潜在细胞反应。通过从补充有血清的培养基中进行连续适应,实现了无血清培养人脂肪来源的基质血管部分(SVF)细胞。脂肪来源的 SVF 是人类内皮细胞和人类平滑肌细胞的来源。利用已建立的压力接种技术,将这些细胞整合到膨胀聚四氟乙烯(ePTFE)管状支架或电纺聚(L-丙交酯-共-己内酯)支架的管腔表面,然后将所得构建体在无血清培养基中使用灌注生物反应器进行培养。使用 ePTFE 支架构建的 BVM 的组织学分析表明,移植物的内表面已经形成了完整的细胞层。在高度多孔的电纺管中也在无血清条件下建立了血管模拟物,除了内表面和外表面之外,还在支架壁的整个范围内实现了细胞化。在每种类型的 BVM 中存在的间充质细胞中,既没有鉴定出内皮细胞也没有平滑肌细胞。裸金属支架被部署在电纺 BVM 内,在生物反应器灌注后,扫描电子显微镜和核特异性双苯并眯唑染色证实支架表面存在细胞。这项研究的结果支持了这样的假设,即使用无血清条件开发的 BVM 受到支架变化的影响,并在植入的医疗器械上表现出组织生长。最终,采用无血清方法可能会导致可控制的、可重复的 BVM 生产,并在设备-组织相互作用、毒性和其他血管现象的研究中获得可解释的、人类特异性的结果;然而,与体内生物反应的比较以及定义的血管细胞的纳入对于验证无血清 BVM 作为一种合适的设备测试替代方法至关重要。
