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通过补体耗竭来消耗特定细胞群体。

Depletion of specific cell populations by complement depletion.

作者信息

Dittel Bonnie N

机构信息

BloodCenter of Wisconsin, Blood Research Institute, USA.

出版信息

J Vis Exp. 2010 Feb 5(36):1487. doi: 10.3791/1487.

DOI:10.3791/1487
PMID:20139864
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2816978/
Abstract

The purification of immune cell populations is often required in order to study their unique functions. In particular, molecular approaches such as real-time PCR and microarray analysis require the isolation of cell populations with high purity. Commonly used purification strategies include fluorescent activated cell sorting (FACS), magnetic bead separation and complement depletion. Of the three strategies, complement depletion offers the advantages of being fast, inexpensive, gentle on the cells and a high cell yield. The complement system is composed of a large number of plasma proteins that when activated initiate a proteolytic cascade culminating in the formation of a membrane-attack complex that forms a pore on a cell surface resulting in cell death(1). The classical pathway is activated by IgM and IgG antibodies and was first described as a mechanism for killing bacteria. With the generation of monoclonal antibodies (mAb), the complement cascade can be used to lyse any cell population in an antigen-specific manner. Depletion of cells by the complement cascade is achieved by the addition of complement fixing antigen-specific antibodies and rabbit complement to the starting cell population. The cells are incubated for one hour at 37 degrees C and the lysed cells are subsequently removed by two rounds of washing. MAb with a high efficiency for complement fixation typically deplete 95-100% of the targeted cell population. Depending on the purification strategy for the targeted cell population, complement depletion can be used for cell purification or for the enrichment of cell populations that then can be further purified by a subsequent method.

摘要

为了研究免疫细胞群体的独特功能,常常需要对其进行纯化。特别是,诸如实时PCR和微阵列分析等分子方法需要分离高纯度的细胞群体。常用的纯化策略包括荧光激活细胞分选(FACS)、磁珠分离和补体耗竭。在这三种策略中,补体耗竭具有快速、廉价、对细胞温和且细胞产量高的优点。补体系统由大量血浆蛋白组成,这些蛋白被激活后会引发蛋白水解级联反应,最终形成膜攻击复合物,该复合物在细胞表面形成孔道,导致细胞死亡(1)。经典途径由IgM和IgG抗体激活,最初被描述为一种杀死细菌的机制。随着单克隆抗体(mAb)的产生,补体级联反应可用于以抗原特异性方式裂解任何细胞群体。通过向起始细胞群体中添加补体固定抗原特异性抗体和兔补体来实现通过补体级联反应耗尽细胞。将细胞在37℃下孵育1小时,随后通过两轮洗涤去除裂解的细胞。具有高效补体固定能力的单克隆抗体通常可耗尽95-100%的目标细胞群体。根据目标细胞群体的纯化策略,补体耗竭可用于细胞纯化或用于富集细胞群体,然后可通过后续方法进一步纯化。

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