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A Highly Efficient Multifunctional Tandem Affinity Purification Approach Applicable to Diverse Organisms

机译:一种高效的多功能串联亲和纯化方法适用于多种生物

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摘要

Determining the localization, binding partners, and secondary modifications of individual proteins is crucial for understanding protein function. Several tags have been constructed for protein localization or purification under either native or denaturing conditions, but few tags permit all three simultaneously. Here, we describe a multifunctional tandem affinity purification (MAP) method that is both highly efficient and enables protein visualization. The MAP tag utilizes affinity tags inserted into an exposed surface loop of mVenus offering two advantages: (1) mVenus fluorescence can be used for protein localization or FACS-based selection of cell lines; and (2) spatial separation of the affinity tags from the protein results in high recovery and reduced variability between proteins. MAP purification was highly efficient in multiple organisms for all proteins tested. As a test case, MAP combined with liquid chromatography-tandem MS identified known and new candidate binding partners and modifications of the kinase Plk1. Thus the MAP tag is a new powerful tool for determining protein modification, localization, and interactions.
机译:确定单个蛋白质的定位,结合伴侣和二级修饰对于理解蛋白质功能至关重要。已经构建了几种标签用于天然或变性条件下的蛋白质定位或纯化,但是很少有标签同时允许全部三个。在这里,我们描述了一种多功能串联亲和纯化(MAP)方法,该方法既高效又可以实现蛋白质可视化。 MAP标签利用插入mVenus暴露的表面环中的亲和标签提供了两个优点:(1)mVenus荧光可用于蛋白质定位或基于FACS的细胞系选择; (2)亲和标签与蛋白质的空间分离导致蛋白质的高回收率和降低的变异性。对于所有测试的蛋白质,MAP纯化在多种生物中均非常有效。作为测试案例,MAP与液相色谱串联质谱联用鉴定了已知的和新的候选结合配偶体以及激酶Plk1的修饰。因此,MAP标签是确定蛋白质修饰,定位和相互作用的新的强大工具。

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