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原代神经元培养与瞬时转染

Primary Neuronal Culture and Transient Transfection.

作者信息

Tseng Shun-Cheng, Chen Peng-Tzu, Hwang Eric

机构信息

Department of Orthopedic Surgery, Changhua Christian Hospital, Changhua, Taiwan.

Department of Biological Science and Technology, National Yang Ming Chiao Tung University, Hsinchu, Taiwan.

出版信息

Bio Protoc. 2025 Jan 20;15(2):e5169. doi: 10.21769/BioProtoc.5169.

Abstract

Primary neuronal culture and transient transfection offer a pair of crucial tools for neuroscience research, providing a controlled environment to study the behavior, function, and interactions of neurons in vitro. These cultures can be used to investigate fundamental aspects of neuronal development and plasticity, as well as disease mechanisms. There are numerous methods of transient transfection, such as electroporation, calcium phosphate precipitation, or cationic lipid transfection. In this protocol, we used electroporation for neurons immediately before plating and cationic lipid transfection for neurons that have been cultured for a few days in vitro. In our experience, the transfection efficiency of electroporation can be as high as 30%, and cationic lipid transfection has an efficiency of 1%-2%. While cationic lipid transfection has much lower efficiency than electroporation, it does offer the advantage of a higher expression level. Therefore, these transfection methods are suitable for different stages of neurons and different expression requirements. Key features • Culture of primary neurons from the CNS. • Electroporation for freshly isolated neurons in suspension. • Cationic lipid transfection for adherent neurons.

摘要

原代神经元培养和瞬时转染为神经科学研究提供了一对关键工具,为在体外研究神经元的行为、功能和相互作用提供了一个可控环境。这些培养物可用于研究神经元发育和可塑性的基本方面以及疾病机制。有多种瞬时转染方法,如电穿孔、磷酸钙沉淀或阳离子脂质转染。在本方案中,我们在铺板前立即对神经元使用电穿孔,对已在体外培养数天的神经元使用阳离子脂质转染。根据我们的经验,电穿孔的转染效率可高达30%,阳离子脂质转染的效率为1%-2%。虽然阳离子脂质转染的效率远低于电穿孔,但它确实具有表达水平较高的优势。因此,这些转染方法适用于神经元的不同阶段和不同的表达要求。关键特性• 从中枢神经系统培养原代神经元。• 对悬浮的新鲜分离神经元进行电穿孔。• 对贴壁神经元进行阳离子脂质转染。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a761/11769751/0d8bb191d151/BioProtoc-15-2-5169-g001.jpg

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