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Yeast two-hybrid detection of integrase-host factor interactions.

机译:酵母整合酶-宿主因子相互作用的两杂交检测。

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摘要

Here we describe methods developed based on systematic yeast two-hybrid screenings that allowed us to identify several binding partners of HIV-1 integrase. We have developed an efficient strategy to perform large comprehensive screenings with different highly complex cDNA libraries derived both random- and oligo-dT primed reactions. A very efficient mating procedure was used for screening in yeast, allowing genetic saturation of positive clones. This importantly leads with confidence to the determination of the regions within the participating proteins responsible for the interactions. Several additional tools were used that allowed us to assess the specificity of the interactions detected, including rebound screens with cellular co-factors as baits performed against a library of random fragments of HIV-1 proviral DNA. For some of the identified cell factors, we have generated and characterized loss of affinity mutants of integrase, which, when combined with viral functional assays, validated the involvement of human lens epithelium-derived growth factor (LEDGF/p75) in the integration step of the HIV-1 replication cycle. All tolled, our studies identified LEDGF/p75, Transportin-SR2 (TNPO3), von Hippel-Lindau binding protein 1 (VBP1), and sucrose non-fermenting 5 (SNF5) as cellular binding partners of HIV-1 integrase.
机译:在这里,我们描述了基于系统的酵母双杂交筛选开发的方法,该筛选使我们能够鉴定HIV-1整合酶的几个结合配偶体。我们已经开发出一种有效的策略,可以使用衍生自随机和寡聚dT引发反应的不同高度复杂的cDNA文库进行大型综合筛选。使用非常有效的交配程序筛选酵母,从而使阳性克隆遗传饱和。重要的是,这有信心地导致参与蛋白相互作用区域的确定。使用了几种其他工具,这些工具使我们能够评估检测到的相互作用的特异性,包括针对针对HIV-1前病毒DNA的随机片段库进行诱饵进行的具有细胞辅助因子的反弹筛查。对于某些已鉴定的细胞因子,我们已经产生并鉴定了整合酶亲和突变体的损失,将其与病毒功能测定结合使用时,验证了人晶状体上皮来源的生长因子(LEDGF / p75)参与了整合酶的整合步骤。 HIV-1复制周期。我们所有的研究都确定LEDGF / p75,Transportin-SR2(TNPO3),von Hippel-Lindau结合蛋白1(VBP1)和蔗糖非发酵5(SNF5)是HIV-1整合酶的细胞结合伴侣。

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