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Redesign of the monomer–monomer interface of Cre recombinase yields an obligate heterotetrameric complex

机译:重新设计Cre重组酶的单体-单体界面可产生专一的异四聚体复合物

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Cre recombinase catalyzes the cleavage and religation of DNA at loxP sites. The enzyme is a homotetramer in its functional state, and the symmetry of the protein complex enforces a pseudo-palindromic symmetry upon the loxP sequence. The Cre-lox system is a powerful tool for many researchers. However, broader application of the system is limited by the fixed sequence preferences of Cre, which are determined by both the direct DNA contacts and the homotetrameric arrangement of the Cre monomers. As a first step toward achieving recombination at arbitrary asymmetric target sites, we have broken the symmetry of the Cre tetramer assembly. Using a combination of computational and rational protein design, we have engineered an alternative interface between Cre monomers that is functional yet incompatible with the wild-type interface. Wild-type and engineered interface halves can be mixed to create two distinct Cre mutants, neither of which are functional in isolation, but which can form an active heterotetramer when combined. When these distinct mutants possess different DNA specificities, control over complex assembly directly discourages recombination at unwanted half-site combinations, enhancing the specificity of asymmetric site recombination. The engineered Cre mutants exhibit this assembly pattern in a variety of contexts, including mammalian cells.
机译:Cre重组酶在loxP位点催化DNA的切割和重新连接。该酶是处于功能状态的同型四聚体,蛋白质复合物的对称性在loxP序列上产生了假回文对称性。 Cre-lox系统是许多研究人员的强大工具。但是,该系统的更广泛应用受到Cre固定序列偏好的限制,后者由Cre单体的直接DNA接触和同四聚体排列决定。作为在任意不对称靶位点实现重组的第一步,我们破坏了Cre四聚体组件的对称性。结合计算和合理的蛋白质设计,我们设计了Cre单体之间的替代界面,该界面具有功能但与野生型界面不兼容。可以将野生型和工程化的半界面混合在一起,以创建两个不同的Cre突变体,它们都不是单独起作用的,但在组合时可以形成活性异四聚体。当这些不同的突变体具有不同的DNA特异性时,对复杂装配的控制将直接阻止在不需要的半位点组合处进行重组,从而增强了不对称位点重组的特异性。工程化的Cre突变体在包括哺乳动物细胞在内的多种环境中均表现出这种装配模式。

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