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A rapid two-step method for isolation of functional primary mouse hepatocytes: cell characterization and asialoglycoprotein receptor based assay development

机译:一种快速的两步法分离功能性原代小鼠肝细胞的方法:基于细胞特征和去唾液酸糖蛋白受体的测定方法的开发

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Primary mouse hepatocytes are an important tool in the biomedical research field for the assessment of hepatocyte function. Several methods for hepatocyte isolation have been published; however, many of these methods require extensive handling and can therefore compromise the viability and function of the isolated cells. Since one advantage of utilizing freshly isolated cells is to maintain an environment in which the cells are more comparable to their in vivo state, it is important to have robust methods that produce cells with high viability, good purity and that function in a similar manner to that in their in vivo state. Here we describe a modified two-step method for the rapid isolation and characterization of mouse primary hepatocytes that results in high yields of viable cells. The asialoglycoprotein receptor (ASGPR), which is one of the most abundant cell surface receptors on hepatocytes, was used to monitor the function of the isolated hepatocytes by demonstrating specific binding of its ligand using a newly developed flow cytometry based ligand-receptor binding assay. Also, an in vitro screening method for siRNA drug candidates was successfully developed utilizing freshly isolated hepatocytes with minimum culture time.
机译:小鼠原代肝细胞是生物医学研究领域中评估肝细胞功能的重要工具。已经公开了几种分离肝细胞的方法。但是,这些方法中的许多方法都需要大量处理,因此可能会损害分离细胞的活力和功能。由于利用新鲜分离的细胞的一个优势是维持一种环境,使细胞与其体内状态更具可比性,因此重要的是要有可靠的方法来生产具有高生存力,良好纯度并以与处于体内状态。在这里,我们描述了一种改良的两步法,可快速分离和鉴定小鼠原代肝细胞,从而获得高产率的活细胞。脱唾液酸糖蛋白受体(ASGPR)是肝细胞上最丰富的细胞表面受体之一,用于通过使用新开发的基于流式细胞仪的配体-受体结合测定法证明其配体的特异性结合来监测分离的肝细胞的功能。同样,利用新鲜培养的肝细胞以最少的培养时间成功开发了一种siRNA候选药物的体外筛选方法。

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