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Combinatorial control of Spo11 alternative splicing by modulation of RNA polymerase II dynamics and splicing factor recruitment during meiosis

机译:通过调节RNA聚合酶II动力学和分裂过程中RNA聚合酶II动力学和剪接因子募集的组合控制

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Homologous recombination and chromosome segregation in meiosis rely on the timely expression of two splice variants of the endonuclease SPO11, named α and β, which respectively skip or include exon 2. However, in spite of its physiological importance, the mechanism underlying Spo11 alternative splicing in meiosis is still unknown. By screening the activity of factors that are predicted to bind the alternatively spliced region of Spo11, we identified hnRNPH as a key regulator of SPO11α splicing in mouse spermatocytes. Although hnRNPH was not upregulated in meiosis concomitantly with the switch in splicing, its recruitment to Spo11 pre-mRNA was favored by selective modulation of RNA polymerase II (RNAPII) phosphorylation and processivity in proximity of exon 2. The hnRNPH binding sites were localized near those of splicing factors that promote SPO11β splicing, suggesting that hnRNPH favors exon 2 skipping by competing out positive regulators. Indeed, hnRNPH binds proximal to a consensus motif for Sam68, a positive regulator of SPO11β splicing in vitro and in vivo, and it interferes with Sam68 binding to the Spo11 pre-mRNA. Thus, our work reveals that modulation of RNAPII dynamics in concert with hnRNPH recruitment exerts a combinatorial control of the timely regulated Spo11 splicing during meiosis.
机译:MeIosis的同源重组和染色体偏析依赖于同内核酸酶Spo11的及时表达的二核酸酶Spo11,命名α和β,其分别跳过或包括外显子2。然而,尽管其生理重要性,所以Spo11替代剪接的机制减数分裂仍然未知。通过筛选预测粘合SpO11的替代剪接区域的因素的活动,我们鉴定了HNRNPH作为剪接小鼠精子细胞的SPO11α关键调节器。虽然HNRNPH在分段中伴随着剪接切换的分数均匀,但是通过选择性调节RNA聚合酶II(RNAPII)磷酸化和外显子的处理率的选择性调节其募集.HNRNPH结合位点在那里附近定位促进Spo11β剪接的拼接因子,旨在通过竞争阳性调节器跳过外显子2跳跃。实际上,HNRNPH与SAM68的共有型基序结合在体外和体内剪接SPO11β的正调节剂,并且它干扰SAM68与SPO11前mRNA结合。因此,我们的作品揭示了与HNRNPH招生的音乐会调制rNAPII动力学施加在减数分裂期间及时调节的SPO11拼接的组合控制。

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