从胎盘组织外植体中分离人绒毛滋养细胞的独特方法

Ashley Serjilus, D. Alcendor
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引用次数: 4

摘要

从原代胎盘组织中分离细胞滋养细胞可能成本高,耗时长,结果不一。在本文中,我们提供了一种简单、经济、有效的方法,可以使用常见的实验室用品来实现绒毛组织中细胞滋养细胞的一致体外分离。滋养层细胞群体是根据形态和表型来确定的,在培养之前及时从胎盘中提取绒毛节点,并通过视觉引导分离结外生物,选择性地捕获细胞滋养层细胞群体和传代培养。这种方法可以分离出不受其他胎盘细胞类型污染的细胞滋养细胞。分离细胞特异性细胞滋养层生物标志物细胞角蛋白7和人绒毛膜促性腺激素(HCG)染色阳性。继代培养的细胞生长到融合形成单层细胞,这种单层细胞可以在培养中传代,并随着时间的推移用于发育原代合体滋养细胞。这些原代细胞滋养细胞群可用于体外胎盘芯片模型,以更好地了解胎盘细胞生物学和功能,以及暴露于毒物和感染因子后的生理反应。该技术可用于从多个器官系统的不同组织中选择性地分离特定类型的细胞。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Unique method for human villous trophoblasts isolation from placental tissue explants
Isolation of cytotrophoblasts from primary placental tissue may be costly and time consuming with variable results. In this paper, we provide a simple, affordable, and efficient method that may performed using common laboratory supplies to achieve consistent in vitro isolation of cytotrophoblasts from villous tissue. Trophoblast populations are identified based on morphology and phenotyping, which employs the timely extraction of villous nodes from the placenta prior to cultivation and isolation of nodal outgrowth by visual guidance for selective capture of cytotrophoblast populations and subculture. This method allows for the isolation of cytotrophoblasts free of contamination with other placental cell types. Isolated cells stain positive for the specific cytotrophoblast biomarker cytokeratin 7 and Human Chorionic Gonadotropin (HCG). Subcultured cells grow to confluency to establish monolayers that may be passaged in culture and later used to develop primary syncytiotrophoblasts over time. These primary cytotrophoblast populations may be employed using in in vitro placenta-on-a chip models to better understand placental cell biology and function, as well as physiological responses after exposure to toxicants, and infectious agents. This technique may be modified for selective isolation of specific cell types within different tissues from multiple organ systems.
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