A comprehensive strategy to identify stoichiometric membrane protein interactomes.

Avanti Gokhale, Patricia Perez-Cornejo, Charity Duran, H Criss Hartzell, Victor Faundez
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引用次数: 11

Abstract

There are numerous experimental approaches to identify the interaction networks of soluble proteins, but strategies for the identification of membrane protein interactomes remain limited. We discuss in detail the logic of an experimental design that led us to identify the interactome of a membrane protein of complex membrane topology, the calcium activated chloride channel Anoctamin 1/Tmem16a (Ano1). We used covalent chemical stabilizers of protein-protein interactions combined with magnetic bead immuno-affinity chromatography, quantitative SILAC mass-spectrometry and in silico network construction. This strategy led us to define a putative Ano1 interactome from which we selected key components for functional testing. We propose a combination of procedures to narrow down candidate proteins interacting with a membrane protein of interest for further functional studies.

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鉴定化学计量膜蛋白相互作用组的综合策略。
有许多实验方法来鉴定可溶性蛋白的相互作用网络,但鉴定膜蛋白相互作用组的策略仍然有限。我们详细讨论了实验设计的逻辑,使我们确定了复杂膜拓扑的膜蛋白的相互作用组,钙活化的氯离子通道Ano1 /Tmem16a (Ano1)。我们使用蛋白-蛋白相互作用的共价化学稳定剂,结合磁珠免疫亲和层析、定量SILAC质谱和硅网络构建。这个策略使我们定义了一个假定的Ano1交互组,从中我们选择了用于功能测试的关键组件。我们提出了一系列的程序来缩小候选蛋白与感兴趣的膜蛋白相互作用的范围,以进行进一步的功能研究。
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