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Resolvase-like recombination performed by the TP901-1 integrase

机译:由TP901-1整合酶进行分离酶样重组

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The site-specific recombination system of temperate lactococcal bacteriophage TP901-1 is unusual in several respects. First, the integrase belongs to the family of extended resolvases rather than to the λ integrase family and second, in the presence of this integrase, a 56?bp attP fragment is sufficient for efficient recombination with the chromosomal attB site in the host Lactococcus lactis subsp. cremoris MG1363. In the present work, this attB site was analysed and a 43?bp attB region was found to be the smallest fragment able to participate fully in recombination. In vitro studies showed that the TP901-1 integrase binds this 43?bp attB fragment, the 56?bp attP and a larger attP fragment with equal affinity. Mutational analysis of the 5?bp common core region (TCAAT) showed that the TC dinucleotide is essential for recombination, but not for binding of the integrase, whereas none of the last three bases are important for recombination. When a number of attL sites, obtained by recombination between an attB site containing a mutation in this TC dinucleotide and a wild-type attP site, were sequenced, a mix of sites with the wild-type or the mutated sequence was obtained. These results are consistent with the hypothesis that the TC dinucleotide constitutes the TP901-1 overlap region. A 2?bp overlap region has been observed in recombination reactions catalysed by all other members of the resolvase/invertase family tested so far. By selecting for attB sites with a decreased ability to participate in recombination, two bases located outside the core region of attB were shown to be involved in the in vitro binding of the TP901-1 integrase.
机译:在几个方面,温带乳酸乳杆菌噬菌体TP901-1的特异性重组系统是不寻常的。首先,整体酶属于延长的分辨率系列而不是λ整体酶系列,而第二个,在该整体酶的存在下,56?BP Attp片段足以与染色体患者乳酸乳酸乳糜液中的染色体attb位点进行高效重组。 Cremoris mg1363。在目前的工作中,分析了该attB网站,并发现了43个?BP attb区域是能够充分参与重组的最小片段。体外研究表明,TP901-1整合酶结合该43〜BP attb片段,56〜BP ATTP和具有相同亲和力的较大的ATTP片段。 5?BP常见核心区(TCAAT)的突变分析表明,TC二核苷酸对重组至关重要,但不用于整合酶的结合,而最后三个碱的结合对于重组是重要的。当测序含有该TC二核苷酸和野生型ATTP位点的诱变位点之间的attB位点之间的重组获得的att1位点时,获得了具有野生型或突变序列的位点的混合物。这些结果与TC二核苷酸构成TP901-1重叠区域的假设一致。已经观察到由迄今为止测试的溶解酶/转化酶系列的所有其他成员催化的重组反应中观察到2磅重叠区域。通过选择具有降低的参与重组能力的attB站点,位于attB的核心区域之外的两个碱基显示参与TP901-1整合酶的体外结合。

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