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Genetic characterization of a mammalian protein-protein interaction domain by using a yeast reverse two-hybrid system.

机译:通过使用酵母反向两杂交系统的哺乳动物蛋白质-蛋白质相互作用域的遗传表征。

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摘要

Many biological processes rely upon protein-protein interactions. Hence, detailed analysis of these interactions is critical for their understanding. Due to the complexities involved, genetic approaches are often needed. In yeast and phage, genetic characterizations of protein complexes are possible. However, in multicellular organisms, such characterizations are limited by the lack of powerful selection systems. Herein we describe genetic selections that allow single amino acid changes that disrupt protein-protein interactions to be selected from large libraries of randomly generated mutant alleles. The strategy, based on a yeast reverse two-hybrid system, involves a first-step negative selection for mutations that affect interaction, followed by a second-step positive selection for a subset of these mutations that maintain expression of full-length protein (two-step selection). We have selected such mutations in the transcription factor E2F1 that affect its ability to heterodimerize with DP1. The mutations obtained identified a putative helix in the marked box, a region conserved among E2F family members, as an important determinant for interaction. This two-step selection procedure can be used to characterize any interaction domain that can be tested in the two-hybrid system.
机译:许多生物学过程依赖于蛋白质-蛋白质相互作用。因此,对这些相互作用的详细分析对于理解它们至关重要。由于涉及的复杂性,经常需要遗传方法。在酵母和噬菌体中,蛋白质复合物的遗传表征是可能的。但是,在多细胞生物中,由于缺乏强大的选择系统,这种表征受到限制。在本文中,我们描述了允许从破坏随机等位基因的大型文库中选择破坏蛋白质与蛋白质相互作用的单个氨基酸变化的遗传选择。该策略基于酵母反向双杂交系统,涉及对影响相互作用的突变进行第一步负选择,然后对这些突变的子集进行第二步正选择,以保持全长蛋白的表达(两个步骤选择)。我们已经在转录因子E2F1中选择了影响其与DP1异源二聚化能力的突变。获得的突变在标记的框(E2F家族成员之间保守的区域)中识别出推定的螺旋,是相互作用的重要决定因素。此两步选择过程可用于表征可在双混合系统中测试的任何交互作用域。

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