Floryanzia Sydney, Lee Seoyoung, Nance Elizabeth
Department of Chemical Engineering, University of Washington, Seattle, WA, 98195, USA.
Department of Bioengineering, University of Washington, Seattle, WA, 98195, USA.
J Biol Eng. 2024 Jul 11;18(1):39. doi: 10.1186/s13036-024-00434-3.
There is significant interest in isolating cells of the blood-brain barrier (BBB) for use in in vitro screening of therapeutics and analyzing cell specific roles in neurovascular pathology. Primary brain cells play an advantageous role in BBB models; however, isolation procedures often do not produce cells at high enough yields for experiments. In addition, although numerous reports provide primary cell isolation methods, the field is lacking in documentation and detail of expected morphological changes that occur throughout culturing and there are minimal troubleshooting resources. Here, we present simplified, robust, and reproducible methodology for isolating astrocytes, pericytes, and endothelial cells, and demonstrate several morphological benchmarks for each cell type throughout the process and culture timeframe. We also analyze common considerations for developing neurovascular cell isolation procedures and recommend solutions for troubleshooting.
The presented methodology isolated astrocytes, pericytes, and endothelial cells and enabled cell attachment, maturation, and cell viability. We characterized milestones in cell maturation over 12 days in culture, a common timeline for applications of these cell types in BBB models. Phase contrast microscopy was used to show initial cell plating, attachment, and daily growth of isolated cells. Confocal microscopy images were analyzed to determine the identity of cell types and changes to cell morphology. Nuclear staining was also used to show the viability and proliferation of glial cells at four time points. Astrocyte branches became numerous and complex with increased culture time. Microglia, oligodendrocytes, and neurons were present in mixed glial cultures for 12 days, though the percentage of microglia and neurons expectedly decreased after passaging, with microglia demonstrating a less branched morphology.
Neurovascular cells can be isolated through our optimized protocols that minimize cell loss and encourage the adhesion and proliferation of isolated cells. By identifying timepoints of viable glia and neurons within an astrocyte-dominant mixed culture, these cells can be used to evaluate drug targeting, uptake studies, and response to pathological stimulus in the neurovascular unit.
分离血脑屏障(BBB)细胞用于治疗药物的体外筛选以及分析细胞在神经血管病理中的特定作用备受关注。原代脑细胞在血脑屏障模型中发挥着有利作用;然而,分离程序往往无法产生足够高产量的细胞用于实验。此外,尽管有许多报道提供了原代细胞分离方法,但该领域缺乏关于整个培养过程中预期形态变化的记录和细节,并且故障排除资源极少。在此,我们提出了一种简化、稳健且可重复的方法来分离星形胶质细胞、周细胞和内皮细胞,并展示了每种细胞类型在整个过程和培养时间范围内的几个形态学基准。我们还分析了开发神经血管细胞分离程序的常见注意事项并推荐故障排除解决方案。
所提出的方法分离出了星形胶质细胞、周细胞和内皮细胞,并实现了细胞附着、成熟和细胞活力。我们对培养12天内细胞成熟的里程碑进行了表征,这是这些细胞类型在血脑屏障模型中应用的常见时间线。相差显微镜用于显示分离细胞的初始接种、附着和每日生长情况。共聚焦显微镜图像用于分析细胞类型的身份和细胞形态的变化。核染色还用于显示胶质细胞在四个时间点的活力和增殖情况。随着培养时间的增加,星形胶质细胞的分支变得繁多且复杂。在混合胶质细胞培养物中,小胶质细胞、少突胶质细胞和神经元存在了12天,不过传代后小胶质细胞和神经元的百分比预计会下降,小胶质细胞的形态分支较少。
通过我们优化的方案可以分离神经血管细胞,该方案可最大限度减少细胞损失并促进分离细胞的黏附和增殖。通过确定星形胶质细胞占主导的混合培养物中存活的胶质细胞和神经元的时间点,这些细胞可用于评估药物靶向、摄取研究以及神经血管单元对病理刺激的反应。
Zotero 插件
