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首页> 外文期刊>Molecular Microbiology >The RecJ DNase strongly suppresses genomic integration of short but not long foreign DNA fragments by homology-facilitated illegitimate recombination during transformation of Acinetobacter baylyi.
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The RecJ DNase strongly suppresses genomic integration of short but not long foreign DNA fragments by homology-facilitated illegitimate recombination during transformation of Acinetobacter baylyi.

机译:RecJ DNase通过不育的Baylyi转化过程中的同源性促进的非法重组,强烈抑制短而长的外来DNA片段的基因组整合。

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摘要

Homology-facilitated illegitimate recombination (HFIR) promotes genomic integration of foreign DNA with a single segment homologous to the recipient genome by homologous recombination in the segment accompanied by illegitimate fusion of the heterologous sequence. During natural transformation of Acinetobacter baylyi HFIR occurs at about 0.01% of the frequency of fully homologous recombination. The role of the 5' single-strand-specific exonuclease RecJ in HFIR was investigated. Deletion of recJ increased HFIR frequency about 20-fold compared with wild type while homologous recombination was not affected. Illegitimate fusion sites were predominantly located within 360 nucleotides away from the homology whereas in wild type most fusion sites were distal (500-2500 nucleotides away). RecJ overproduction reduced the HFIR frequency to half compared with wild type, and transformants with short foreign DNA segments were diminished, leading to on average 866 foreign nucleotides integrated per event (682 in wild type, 115 in recJ). In recJ always the 3' ends of donor DNA were integrated at the homology whereas in wild type these were 3' or 5'. RecJ apparently suppresses HFIR by degrading 5' non-homologous DNA tails at the post-synaptic stage. We propose that the RecJ activity level controls the HFIR frequency during transformation and the amount of foreign DNA integrated per event.
机译:同源性促进的非合法重组(HFIR)通过在片段中进行同源重组并伴有异源序列的非法融合,促进了外源DNA与与受体基因组同源的单个片段的基因组整合。在巴氏不动杆菌的自然转化过程中,HFIR发生在完全同源重组频率的0.01%左右。研究了5'单链特异性核酸外切酶RecJ在HFIR中的作用。与野生型相比,recJ的缺失使HFIR频率增加了约20倍,而同源重组不受影响。不合法的融合位点主要位于距同源性360个核苷酸内,而在野生型中,大多数融合位点位于远端(距离500-2500个核苷酸)。与野生型相比,RecJ的过量生产将HFIR频率降低了一半,外源DNA片段短的转化子减少了,平均每个事件整合了866个外来核苷酸(野生型为682,recJ为115)。在recJ中,供体DNA的3'末端总是以同源性整合,而在野生型中则是3'或5'。 RecJ显然通过在突触后阶段降解5'非同源DNA尾巴来抑制HFIR。我们建议RecJ活性水平控制转化过程中的HFIR频率以及每个事件整合的外源DNA的数量。

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