David B. Beck, Roberto Bonasio
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引用次数: 2
Abstract
Identification of molecular interactions is paramount to understanding how cells function. Most available technologies rely on co-purification of a protein of interest and its binding partners. Therefore, they are limited in their ability to detect low-affinity interactions and cannot be applied to proteins that localize to difficult-to-solubilize cellular compartments. In vivo proximity labeling (IPL) overcomes these obstacles by covalently tagging proteins and RNAs based on their proximity in vivo to a protein of interest. In IPL, a heterobifunctional probe comprising a photoactivatable moiety and biotin is recruited by a monomeric streptavidin tag fused to a protein of interest. Following UV irradiation, candidate interacting proteins and RNAs are covalently biotinylated with tight spatial and temporal control and subsequently recovered using biotin as an affinity handle. Here, we describe experimental protocols to discover novel protein-protein and protein-RNA interactions using IPL. © 2017 by John Wiley & Sons, Inc.
光激活的体内接近标记
分子相互作用的鉴定对于理解细胞的功能是至关重要的。大多数可用的技术依赖于感兴趣的蛋白质及其结合伙伴的共同纯化。因此,它们检测低亲和力相互作用的能力有限,不能用于定位于难以溶解的细胞室的蛋白质。体内接近标记(IPL)通过基于蛋白质和rna在体内接近感兴趣的蛋白质的共价标记来克服这些障碍。在IPL中,由光激活片段和生物素组成的异双功能探针通过融合到感兴趣蛋白质上的单体链亲和素标签募集。在紫外线照射后,候选的相互作用蛋白和rna在严格的时空控制下被共价生物素化,随后以生物素作为亲和手柄进行恢复。在这里,我们描述了使用IPL发现新的蛋白质-蛋白质和蛋白质- rna相互作用的实验方案。©2017 by John Wiley &儿子,Inc。
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