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Co-cultures of Glioma Stem Cells and Primary Neurons, Astrocytes, Microglia, and Endothelial Cells for Investigation of Intercellular Communication in the Brain

机译:胶质瘤干细胞与原代神经元,星形胶质细胞,小胶质细胞和内皮细胞的共培养物,用于研究大脑中的细胞间通讯

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摘要

Intercellular communication within complex biological and pathological systems via extracellular vesicles (EVs) and secreted factors is a highly attractive area of research. However, cell models enabling investigation of such communication in vitro are limited. Commonly utilized is the supplementation of hyper-concentrated EVs or other extracellular factors to the recipient cell cultures. This approach requires purification of the secreted complexes and is confounded by the contamination of media components. Two-chamber co-cultures of donor and recipient cells separated by a pore membrane may represent a more physiological and better-controlled system for the investigation of intercellular communication. Yet, distinct culture conditions for different neural cell types often make them incompatible for co-culturing. Here we optimized short-term co-cultures of patient-derived low-passage glioma-initiating stem cells with normal cells of the brain microenvironment, such as primary neurons, astrocytes, microglia, and brain endothelial cells. We demonstrate the culture compatibility of these cell types and internalization of glioma-derived extracellular RNA by the normal recipient cells. The presented protocols are valuable for the investigation of intercellular communication between glioma brain tumor and cells of its microenvironment, including but not limited to the EVs-mediated communication.RESEARCH IN CONTEXTCell-to-cell communication is essential in normal physiology and implicated in disease; however, experimental systems for its modeling in vitro are limited. Particularly, the investigation of communication between brain tumors and normal cells of the brain microenvironment has been challenged by the lack of adequate culture models. Here we developed co-cultures of glioma stem cells with various types of normal brain cells, including primary neurons, astrocytes, microglia, and brain endothelial cells, and demonstrated their utility for the study of intercellular communication. Detection of proposed markers in the recipient cells confirmed RNA transfer in these co-cultures.
机译:通过细胞外囊泡(EV)和分泌因子在复杂的生物和病理系统内进行细胞间通讯是一个非常有吸引力的研究领域。但是,能够研究这种体外通讯的细胞模型是有限的。通常使用的是将高浓度电动汽车或其他细胞外因子补充到受体细胞培养物中。该方法需要纯化分泌的复合物,并且由于培养基成分的污染而混淆。供体和受体细胞被孔膜分隔的两腔共培养可能代表了一种更生理和更好控制的系统,用于研究细胞间的通讯。但是,针对不同神经细胞类型的不同培养条件通常会使它们不适合共培养。在这里,我们优化了患者来源的低通道神经胶质瘤起始干细胞与大脑微环境的正常细胞(例如原代神经元,星形胶质细胞,小胶质细胞和脑内皮细胞)的短期共培养。我们证明了这些细胞类型的培养相容性和正常受体细胞对神经胶质瘤来源的细胞外RNA的内在化。所提出的方案对于研究神经胶质瘤脑肿瘤与其微环境细胞之间的细胞间通讯具有重要价值,包括但不限于电动汽车介导的通讯。细胞间通讯在正常生理中是必不可少的,并且与疾病有关。但是,体外建模的实验系统是有限的。特别地,由于缺乏适当的培养模型,对脑肿瘤与脑微环境正常细胞之间的通讯研究受到了挑战。在这里,我们开发了神经胶质瘤干细胞与各种类型的正常脑细胞(包括原代神经元,星形胶质细胞,小胶质细胞和脑内皮细胞)的共培养物,并证明了它们在细胞间通讯研究中的实用性。在受体细胞中提议的标记物的检测证实了这些共培养物中的RNA转移。

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