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Requirements for double-strand cleavage by chimeric restriction enzymes with zinc finger DNA-recognition domains

机译:具有锌指DNA识别域的嵌合限制酶对双链裂解的要求

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This study concerns chimeric restriction enzymes that are hybrids between a zinc finger DNA-binding domain and the non-specific DNA-cleavage domain from the natural restriction enzyme FokI. Because of the flexibility of DNA recognition by zinc fingers, these enzymes are potential tools for cleaving DNA at arbitrarily selected sequences. Efficient doublestrand cleavage by the chimeric nucleases requires two binding sites in close proximity. When cuts were mapped on the DNA strands, it was found that they occur in pairs separated by approx 4 bp with a 5' overhang, as for native FokI. Furthermore, amino acid changes in the dimer interface of the cleavage domain abolished activity. These results reflect a requirement for dimerization of the cleavage domain. The dependence of cleavage efficiency on the distance between two inverted binding sites was determined and both upper and lower limits were defined. Two different zinc finger combinations binding to non-identical sites also supported specific cleavage. Molecular modeling was employed to gain insight into the precise location of the cut sites. These results define requirements for effective targets of chimeric nucleases and will guide the design of novel specificities for directed DNA cleavage in vitro and in vivo.
机译:这项研究涉及嵌合限制酶,该酶是锌指DNA结合结构域和天然限制酶FokI的非特异性DNA切割结构域之间的杂种。由于锌指可灵活识别DNA,因此这些酶是在任意选择的序列上切割DNA的潜在工具。嵌合核酸酶有效的双链切割需要两个紧密相邻的结合位点。当将切割图谱定位在DNA链上时,发现它们与天然FokI成对出现,相距约4 bp,突出端为5'。此外,切割结构域的二聚体界面中的氨基酸变化消除了活性。这些结果反映了对切割结构域二聚化的要求。确定切割效率对两个反向结合位点之间距离的依赖性,并定义上限和下限。结合到不同位点的两种不同的锌指组合也支持特异性切割。使用分子建模来深入了解切割部位的精确位置。这些结果确定了嵌合核酸酶有效靶标的要求,并将指导体外和体内定向DNA切割的新特异性设计。

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