Trophoblast Cell Recovery from Angiogenesis-Tube Formation Assay for Differentiation Marker Expression Analysis.

IF 1.2 4区 综合性期刊 Q3 MULTIDISCIPLINARY SCIENCES Jove-Journal of Visualized Experiments Pub Date : 2024-11-08 DOI:10.3791/66454
Rodrigo Escalona-Rivano, Delia I Chiarello, Lorena Carvajal, Ivo Carrasco-Wong, Jaime A Gutiérrez
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Abstract

During placenta development, extravillous trophoblast (EVT) cells invade the maternal decidua to remodel the uterine spiral arteries by a process of mesenchymal to endothelial-like transition. Traditionally, this process is evaluated by an in vitro tube-formation assay, where the cells organize themselves into tube-like structures when seeded over a polymerized basement membrane preparation. Although several structural features can be measured in photomicrographs of the structures, to assess the real commitment of EVT to the endothelial-type phenotype, biochemical analysis of cell extracts is required. Scraping the cells from the culture dish to obtain RNA and/or protein extracts is not an alternative since the tube-like structures are severely contaminated by the bulk of proteins from the polymerized basement membrane. Thus, a strategy to separate the cells from the basement membrane proteins prior to the preparation of cell extracts is needed. Here, a simple, fast, and cost-effective method to recover the tube-like structures from the in vitro tube-formation assay and the subsequent analysis by biochemical techniques is presented. Tube-like structures formed by HTR8/SVneo cells, an EVT cell line, were liberated from the polymerized basement membrane by a short incubation with PBS supplemented with ethylenediaminetetraacetic acid (EDTA). After serial washes, a ready-to-use pellet of purified tube-like structures can be obtained. This pellet can be subsequently processed to obtain RNA and protein extracts. qPCR analysis evidenced the induced expression of VE-cadherin and alphav-integrin, two endothelial cell markers, in EVT-derived tube-like structures compared to control cells, which was consistent with the induction of the endothelial cell marker, CD31, evaluated by immunofluorescence. Western blot analysis of the tube-like structures' protein extracts revealed the overexpression of RECK in transfected HTR8/SVneo cells. Thus, this simple method allows to obtain cell extracts from the in vitro tube-formation assay for the subsequent analysis of RNAs and protein expression.

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滋养层细胞从血管生成中恢复--用于分化标记表达分析的试管形成试验
在胎盘发育过程中,绒毛外滋养层细胞(EVT)侵入母体蜕膜,通过间充质向内皮样转变的过程重塑子宫螺旋动脉。传统上,这一过程是通过体外管形成试验来评估的,即当细胞播种在聚合基底膜制备物上时,会自行组织成管状结构。虽然可以从结构的显微照片中测量出一些结构特征,但要评估 EVT 是否真正形成了内皮型表型,还需要对细胞提取物进行生化分析。从培养皿中刮取细胞以获得 RNA 和/或蛋白质提取物的方法并不可行,因为管状结构会受到来自聚合基底膜的大量蛋白质的严重污染。因此,需要一种策略,在制备细胞提取物之前将细胞与基底膜蛋白质分离。本文介绍了一种简单、快速且经济有效的方法,可从体外管状结构形成试验中回收管状结构,并随后通过生化技术进行分析。HTR8/SVneo 细胞(一种 EVT 细胞系)形成的管状结构通过与添加乙二胺四乙酸(EDTA)的 PBS 短时间孵育后从聚合基底膜中释放出来。经过连续洗涤后,可得到纯化的管状结构的即用颗粒。qPCR 分析表明,与对照细胞相比,在 EVT 衍生的管样结构中,VE-cadherin 和 alphav-integrin 这两种内皮细胞标记物的表达受到诱导,这与免疫荧光评估的内皮细胞标记物 CD31 的诱导相一致。管样结构蛋白提取物的 Western 印迹分析显示,转染的 HTR8/SVneo 细胞中 RECK 过表达。因此,这种简单的方法可以从体外管状结构实验中获得细胞提取物,用于随后的 RNA 和蛋白质表达分析。
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来源期刊
Jove-Journal of Visualized Experiments
Jove-Journal of Visualized Experiments MULTIDISCIPLINARY SCIENCES-
CiteScore
2.10
自引率
0.00%
发文量
992
期刊介绍: JoVE, the Journal of Visualized Experiments, is the world''s first peer reviewed scientific video journal. Established in 2006, JoVE is devoted to publishing scientific research in a visual format to help researchers overcome two of the biggest challenges facing the scientific research community today; poor reproducibility and the time and labor intensive nature of learning new experimental techniques.
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