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DNA complexes obtained with the integron integrase IntI1 at the attI1 site.

机译:在attI1位点使用整合子整合酶IntI1获得的DNA复合物。

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摘要

Integrons are genetic elements that are able to capture genes by a site-specific recombination mechanism. Integrons contain a gene coding for a lambda-like integrase that carries out site-specific recombination by interacting with two different target sites; the attI site and the palindromic sequence attC (59 base element). Cassette integrations usually involve the attI site, while cassette excisions use attC . Therefore, the integrase should bind both sites to cleave DNA and perform site-specific recombination reactions. We have used purified maltose-binding protein fused with the integrase (MBP-IntI1) and native IntI1 protein and gel retardation assays with fragments containing the complete and partial attI1 site to show formation of four complexes in this region. Chemical modification of specific nucleotides within the attI1 site was used to investigate their interference with binding of the integrase protein. We attribute IntI1 specific binding to four regions in the attI1 site and a GTTA consensus sequence is found in three of the four regions. Interference by modified guanine and thymine residues in the DNA major groove and adenine residues in the minor groove were observed, indicating that the integrase interacts with both sides of the helix. Binding of IntI1 to attC is also discussed.
机译:整合素是能够通过位点特异性重组机制捕获基因的遗传元件。整合素含有编码λ样整合酶的基因,该基因通过与两个不同的靶位点相互作用而进行位点特异性重组。 attI位点和回文序列attC(59个碱基)。盒式磁带整合通常涉及attI部位,而盒式磁带切除则使用attC。因此,整合酶应当结合两个位点以切割DNA并进行位点特异性重组反应。我们已使用与整合酶(MBP-IntI1)和天然IntI1蛋白融合的纯化的麦芽糖结合蛋白和凝胶阻滞测定法,其中含有完整和部分attI1位点的片段显示出该区域中四个复合物的形成。使用attI1位点内特定核苷酸的化学修饰来研究其对整合酶蛋白结合的干扰。我们将IntI1特异性结合归因于attI1站点的四个区域,并且在四个区域中的三个区域中发现了GTTA共有序列。观察到DNA大槽中修饰的鸟嘌呤和胸腺嘧啶残基和小槽中腺嘌呤残基的干扰,表明整合酶与螺旋的两侧相互作用。还讨论了IntI1与attC的结合。

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