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Topology and replication of a nuclear episomal plasmid in the rodent malaria Plasmodium berghei

机译:啮齿动物疟疾伯氏疟原虫中核附加型质粒的拓扑和复制

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The rodent malaria Plasmodium berghei is one of a small number of species of Plasmodium that can currently be genetically transformed through experimentally controlled uptake of exogenous DNA by bloodistage parasites. Circular DNA containing a selectable marker replicates and is maintained under selection pressure in a randomly segregating episomal form during the first weeks after transformation. In this study, using pulsed field gel electrophoresis and ionising radiation, we show that in dividing asexual blood stage parasites the episomes are completely converted, within 2 weeks post-infection, into non-rearranged circular concatamers ranging in size between about 9 and 15 copies of the monomer. These occur as slow-moving aggregates held together by radiation-sensitive linkers consisting partly of single-stranded DNA. The process generating these complexes is not clear but 2D gel analysis showed that Cairns-type replication origins were absent and it seems most likely that the initial concatamerisation takes place using a rolling circle mechanism followed by circularisation through internal recombination. We propose a model in which continued rolling circle replication of the large circular concatamers and the recombinational activity of the tails of the rolling circles could lead to the formation of the large aggregates.
机译:啮齿动物疟疾伯氏疟原虫是目前可通过实验控制的血液寄生虫对外源DNA的实验控制摄取而遗传转化的少数疟原虫之一。含有选择标记的环状DNA在复制后的最初几周内以随机分离的游离形式复制并维持在选择压力下。在这项研究中,使用脉冲场凝胶电泳和电离辐射,我们表明在分割无性血液阶段的寄生虫后,附加体在感染后2周内完全转化为大小在9到15拷贝之间的非重排环状辅酶单体。这些以缓慢移动的聚集体形式存在,这些聚集体由部分由单链DNA组成的辐射敏感接头保持在一起。生成这些复合物的过程尚不清楚,但2D凝胶分析表明不存在凯恩斯型复制起点,似乎最有可能使用滚环机制进行初始共聚合,然后通过内部重组进行环化。我们提出了一个模型,在该模型中,大型圆形催化物的连续滚动环复制和滚动环尾部的重组活性可能导致大聚集体的形成。

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