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Non-homologous DNA end joining in plant cells is associated with deletions and filler DNA insertions.

机译:植物细胞中非同源DNA末端连接与缺失和填充DNA插入有关。

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摘要

Double strand DNA breaks in plants are primarily repaired via non-homologous end joining. However, little is known about the molecular events underlying this process. We have studied non-homologous end joining of linearized plasmid DNA with different termini configurations following transformation into tobacco cells. A variety of sequences were found at novel end junctions. Joining with no sequence alterations was rare. In most cases, deletions were found at both ends, and rejoining usually occurred at short repeats. A distinct feature of plant junctions was the presence of relatively large, up to 1.2 kb long, insertions (filler DNA), in approximately 30% of the analyzed clones. The filler DNA originated either from internal regions of the plasmid or from tobacco genomic DNA. Some insertions had a complex structure consisting of several reshuffled plasmid-related regions. These data suggest that double strand break repair in plants involves extensive end degradation, DNA synthesis following invasion of ectopic templates and multiple template switches. Such a mechanism is reminiscent of the synthesis-dependent recombination in bacteriophage T4. It can also explain the frequent 'DNA scrambling' associated with illegitimate recombination in plants.
机译:植物中的双链DNA断裂主要通过非同源末端连接修复。但是,对该过程的分子事件知之甚少。我们已经研究了转化到烟草细胞后具有不同末端构型的线性化质粒DNA的非同源末端连接。在新颖的末端连接处发现了多种序列。没有序列改变的连接是罕见的。在大多数情况下,在两端发现缺失,并且重新结合通常发生在短的重复中。植物连接的一个显着特征是在大约30%的分析克隆中存在相对较大的长达1.2 kb的插入(填充DNA)。填充物DNA要么来源于质粒的内部区域,要么来源于烟草基因组DNA。一些插入物具有由几个改组的质粒相关区域组成的复杂结构。这些数据表明植物中的双链断裂修复涉及广泛的末端降解,异位模板入侵和多个模板开关后的DNA合成。这种机制使人联想到噬菌体T4中依赖于合成的重组。它还可以解释与植物中非法重组相关的频繁“ DNA加扰”。

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  • 作者

    Gorbunova, V; Levy, A A;

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  • 年度 1997
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  • 原文格式 PDF
  • 正文语种 en
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