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多重免疫沉淀流式细胞术(Multiplex IP-FCM):评估多蛋白复合物中生理蛋白-蛋白相互作用的原理和指南。

Multiplex IP-FCM (immunoprecipitation-flow cytometry): Principles and guidelines for assessing physiologic protein-protein interactions in multiprotein complexes.

机构信息

Mayo Clinic College of Medicine, Department of Immunology, Rochester, MN, USA.

出版信息

Methods. 2012 Feb;56(2):154-60. doi: 10.1016/j.ymeth.2011.09.005. Epub 2011 Sep 16.

Abstract

There is significant interest in the development of methods with the potential to increase access to 'the interactome' for both experimental and clinical applications. Immunoprecipitation detected by flow cytometry (IP-FCM) is a robust, biochemical method that can be used for measuring physiologic protein-protein interactions (PPI) in multiprotein complexes (MPC) with high sensitivity. Because it is based on antibody-mediated capture of protein complexes onto microspheres, IP-FCM is potentially compatible with a multiplex platform that could allow simultaneous assessment of many physiologic PPI. Here, we consider the principles of ambient analyte conditions (AAC) and inter-bead independence, and provide a template set of experiments showing how to convert singleplex IP-FCM to multiplex IP-FCM, including assays to confirm the validity of the experimental conditions for data acquisition. We conclude that singleplex IP-FCM can be successfully upgraded to multiplex format, and propose that the unique strengths of multiplex IP-FCM make it a method that is likely to facilitate the acquisition of new PPI data from primary cell sources.

摘要

人们对开发具有潜在用途的方法很感兴趣,这些方法可能有助于在实验和临床应用中获取“相互作用组”。通过流式细胞术检测的免疫沉淀(IP-FCM)是一种强大的生化方法,可用于测量多蛋白复合物(MPC)中生理蛋白-蛋白相互作用(PPI),具有高灵敏度。由于它基于抗体介导的将蛋白质复合物捕获到微球上,因此 IP-FCM 可能与可同时评估许多生理 PPI 的多路复用平台兼容。在这里,我们考虑环境分析物条件(AAC)和珠间独立性的原理,并提供了一组实验模板,展示了如何将单重 IP-FCM 转换为多重 IP-FCM,包括用于确认数据采集实验条件有效性的测定法。我们得出结论,单重 IP-FCM 可以成功升级为多重格式,并且提出了多重 IP-FCM 的独特优势,使其成为一种可能有助于从原代细胞来源获取新的 PPI 数据的方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5ae9/3261325/0f82db97d602/nihms329807f1.jpg

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