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The RecBCD and SbcCD DNases suppress homology-facilitated illegitimate recombination during natural transformation of Acinetobacter baylyi

机译:RecBCD和SBCCD DNases抑制了在贝利氏菌的天然转化期间同源促进的非法复合

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During natural transformation of Acinetobacter baylyi, the genomic integration of foreign (non-homologous) DNA is possible when the DNA contains a single segment homologous to the recipient genome (anchor) through homologous recombination in the anchor facilitating illegitimate recombination in the neighbouring foreign DNA (homology-facilitated illegitimate recombination; HFIR). DNA integration by HFIR occurs about 10?000 times less frequently than fully homologous recombination, but at least 100?000-fold more frequently than integration in the absence of any homology. We investigated the influence of the RecBCD enzyme (DNase/helicase) and SbcCD DNase (DNA-structure-specific single-strand endonuclease and exonuclease) on HFIR. In a recBCD null mutant the acquisition of foreign DNA was elevated 11-fold relative to wild-type cells by a 6.9-fold increased HFIR frequency and by the integration of longer stretches of foreign DNA in each event. In an sbcCD null mutant, the foreign DNA acquisition was 4.5-fold higher than in the wild-type, while homologous transformation with large DNA molecules was unaffected and increased 3.2-fold with small DNA fragments. The sbcCD mutation partially suppressed the high UV sensitivity and low viability of the recBCD mutant and also decreased its foreign DNA acquisition by HFIR to the lower level of the sbcCD mutant. We propose that suppression of HFIR results from the elimination of double-stranded intermediates of the HFIR process during transformation by RecBCD, and by SbcCD interfering with branched molecules. Our results provide evidence that the homologous recombination enzymes RecBCD and SbcCD control the level of foreign DNA acquisition by HFIR.
机译:在百叶腺素的自然转化期间,当DNA通过在邻近的外国DNA中的锚固中的同源重组中含有与受体基因组(锚)同源同源的单个段同源的单个段,促进邻近的外国DNA(同源性促进的非法重组; HFIR)。通过HFIR的DNA整合发生比完全同源重组的频率低约10?000倍,但在没有任何同源性的情况下,通常比整合更频繁地倍增100 000倍。我们研究了RECBCD酶(DNA酶/螺旋酶)和SBCCD DNA酶(DNA-结构特异性单链内切核酸酶和外切核酸酶)对HFIR的影响。在Recbcd Null突变体中,相对于野生型细胞的11倍,通过6.9倍的HFIR频率和每种事件中的延伸延伸的延伸延伸的延伸延伸的整合,将外来DNA的采集升高11倍。在SBCCD NULL突变体中,外国DNA采集比野生型高4.5倍,而具有大DNA分子的同源转化不受影响并随着小DNA片段增加3.2倍。 SBCCD突变部分抑制了RECBCD突变体的高UV敏感性和低可存度,并且还通过HFIR降低了其外来DNA采集到SBCCD突变体的较低水平。我们提出抑制HFIR的抑制来自消除RecBCD转化过程中HFIR过程的双链中间体,并通过SBCCD干扰支链分子。我们的结果提供了证据表明,同源重组酶RecBCD和SBCCD通过HFIR控制了外国DNA征收的水平。

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