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通过流式细胞术对多蛋白复合物进行可视化分析。

Visualization of multiprotein complexes by flow cytometry.

作者信息

Schrum Adam G

机构信息

Mayo Clinic College of Medicine, Rochester, Minnesota.

出版信息

Curr Protoc Immunol. 2009 Nov;Chapter 5:5.9.1-5.9.14. doi: 10.1002/0471142735.im0509s87.

Abstract

Multiprotein complexes and other protein-protein interactions play important roles in virtually all cellular processes. Analysis of coimmunoprecipitation of protein complexes by flow cytometry (IP-FCM, or "the fly-p" method) provides a sensitive means to measure these interactions in the native/nondenatured state. First, immunoprecipitating antibodies are covalently coupled to polystyrene latex beads whose low autofluorescence is compatible with flow cytometry. These antibody-coupled beads are used to immunoprecipitate a specific protein (primary analyte) present in cell lysates. Finally, the protein complexes associated with the beads are probed with fluorochrome-conjugated antibodies specific for interaction partners, or secondary analytes, that may be associated with the primary analyte. The use of quantitative flow cytometric methodology can allow the semiquantitative fluorescence data generated to be converted into estimated numbers of co-associated molecules on the beads. The method represents a robust technique to assess native protein-protein interactions without requiring genetic engineering or large sample sizes.

摘要

多蛋白复合物和其他蛋白质-蛋白质相互作用几乎在所有细胞过程中都发挥着重要作用。通过流式细胞术分析蛋白质复合物的共免疫沉淀(IP-FCM,或“飞p”法)提供了一种在天然/非变性状态下测量这些相互作用的灵敏方法。首先,免疫沉淀抗体共价偶联到聚苯乙烯乳胶珠上,其低自发荧光与流式细胞术兼容。这些抗体偶联珠用于免疫沉淀细胞裂解物中存在的特定蛋白质(主要分析物)。最后,用针对可能与主要分析物相关的相互作用伙伴或次要分析物的荧光染料偶联抗体探测与珠子相关的蛋白质复合物。使用定量流式细胞术方法可以将产生的半定量荧光数据转换为珠子上共相关分子的估计数量。该方法是一种无需基因工程或大量样本即可评估天然蛋白质-蛋白质相互作用的强大技术。

相似文献

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Visualization of multiprotein complexes by flow cytometry.通过流式细胞术对多蛋白复合物进行可视化分析。
Curr Protoc Immunol. 2009 Nov;Chapter 5:5.9.1-5.9.14. doi: 10.1002/0471142735.im0509s87.
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Protein-Protein Interactions: Co-Immunoprecipitation.蛋白质-蛋白质相互作用:免疫共沉淀法
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