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Promoter-driven splicing regulation in fission yeast

机译:裂变酵母中启动子驱动的剪接调控

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摘要

The meiotic cell cycle is modified from the mitotic cell cycle by having a premeiotic S phase which leads to high levels of recombination, two rounds of nuclear division with no intervening DNA synthesis, and a reductional pattern of chromosome segregation. Rem1 is a cyclin that is expressed only during meiosis in the fission yeast Schizosaccharomyces pombe. Cells in which rem1 has been deleted show a decreased intragenic meiotic recombination and a delay at the onset of meiosis I. When ectopically expressed in mitotically growing cells, Rem1 induces a G1 arrest followed by severe mitotic catastrophes. Here we show that rem1 expression is regulated at the level of both transcription and splicing, encoding for two proteins with different function depending on the intron retention. We have determined that the regulation of rem1 splicing is not dependent on any transcribed region of the gene. Furthermore, when the rem1 promoter is fused to other intron-containing genes, the chimeras show a meiotic-specific regulation of splicing, exactly as endogenous rem1. This regulation is dependent on two transcription factors of the forkhead family, Mei4 and Fkh2. While Mei4 induces both transcription and splicing of rem1, Fkh2 is responsible for the intron retention of the transcript during vegetative growth and pre-meiotic S phase.
机译:减数分裂细胞周期是由有丝分裂前期S期从有丝分裂细胞周期改造而来的,前期S期导致高水平的重组,两轮核分裂而无间断的DNA合成以及染色体分离的减少模式。 Rem1是一种细胞周期蛋白,仅在减数分裂裂殖酵母裂殖酵母中减数分裂时表达。 rem1被删除的细胞显示出减少的基因内减数分裂重组和减数分裂I发作的延迟。当在有丝分裂生长的细胞中异位表达时,Rem1诱导G1停滞,继而发生严重的有丝分裂灾难。在这里,我们显示rem1的表达受转录和剪接水平的调节,根据内含子的保留编码两种具有不同功能的蛋白质。我们已经确定,rem1剪接的调控不依赖于该基因的任何转录区域。此外,当rem1启动子与其他含内含子的基因融合时,嵌合体显示出与剪接有关的减数分裂特异性调控,就像内源性rem1一样。该调节取决于叉头家族的两个转录因子Mei4和Fkh2。 Mei4诱导rem1的转录和剪接,而Fkh2在营养生长和减数分裂前S期期间负责转录物的内含子保留。

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    Moldón Vara, Alberto;

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  • 年度 2008
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  • 原文格式 PDF
  • 正文语种 eng
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