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Transposition of the rice miniature inverted repeat transposable element mPing in Arabidopsis thaliana

机译:拟南芥中水稻微型反向重复转座子mPing的转座

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摘要

An active miniature inverted repeat transposable element (MITE), mPing, was discovered by computer-assisted analysis of rice genome sequence. The mPing element is mobile in rice cell culture and in a few rice strains where it has been amplified to >1,000 copies during recent domestication. However, determination of the transposase source and characterization of the mechanism of transposition have been hampered by the high copy number of mPing and the presence of several candidate autonomous elements in the rice genome. Here, we report that mPing is active in Arabidopsis thaliana, where its transposition is catalyzed by three sources of transposase from rice: the autonomous Ping and Pong elements and by a cDNA derived from a Ping transcript. In addition to transposase, the product of a second element-encoded ORF of unknown function is also required for mPing transposition. Excision of mPing in A. thaliana is usually precise, and transposed copies usually insert into unlinked sites in the genome that are preferentially in or near genes. As such, this will be a valuable assay system for the dissection of MITE transposition and a potentially powerful tagging system for gene discovery in eukaryotes.
机译:通过计算机辅助分析水稻基因组序列发现了一种活性微型反向重复转座因子(mITE)。 mPing元件可在水稻细胞培养物中和一些水稻菌株中移动,在最近的驯化过程中,mPing元素已被扩增至> 1,000拷贝。然而,转座酶来源的确定和转座机制的表征已被高水平的mPing拷贝数和水稻基因组中几种候选自主元件的存在所困扰。在这里,我们报道mPing在拟南芥中很活跃,其转座由水稻转座酶的三种来源催化:自主的Ping和Pong元件以及源自Ping转录本的cDNA。除转座酶外,mPing转座还需要未知功能的第二个元素编码的ORF的乘积。拟南芥中mPing的切除通常很精确,转座后的拷贝通常插入基因组中优先位于基因内或附近的未连接位点。因此,这将是用于解剖MITE转座的有价值的测定系统,并且是用于真核生物中基因发现的潜在强大的标记系统。

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