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Regulated cellular partitioning of SR protein-specific kinases in mammalian cells

机译:哺乳动物细胞中SR蛋白特异性激酶的调控细胞分裂

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Reversible phosphorylation of the SR family of splicing factors plays an important role in pre-mRNA processing in the nucleus. Interestingly, the SRPK family of kinases specific for SR proteins is localized in the cytoplasm, which is critical for nuclear import of SR proteins in a phosphorylation-dependent manner. Here, we report molecular dissection of the mechanism involved in partitioning SRPKs in the cytoplasm. Common among all SRPKs, the bipartite kinase catalytic core is separated by a unique spacer sequence. The spacers in mammalian SRPK1 and SRPK2 share little sequence homology, but they function interchangeably in restricting the kinases in the cytoplasm. Removal of the spacer in SRPK1 had little effect on the kinase activity, but it caused a quantitative translocation of the kinase to the nucleus and consequently induced aggregation of splicing factors in the nucleus. Rather than carrying a nuclear export signal as suggested previously, we found multiple redundant signals in the spacer that act together to anchor the kinase in the cytoplasm. Interestingly, a cell cycle signal induced nuclear translocation of the kinase at the G(2)/M boundary. These findings suggest that SRPKs may play an important role in linking signaling to RNA metabolism in higher eukaryotic cells.
机译:剪接因子SR家族的可逆磷酸化在细胞核中的前mRNA加工中起重要作用。有趣的是,对SR蛋白特异的激酶SRPK家族位于细胞质中,这对于以磷酸化依赖性方式对SR蛋白的核导入至关重要。在这里,我们报告分子解剖涉及在细胞质中分配SRPKs的机制。在所有SRPK中共有的二分体激酶催化核心被独特的间隔序列隔开。哺乳动物SRPK1和SRPK2中的间隔子几乎没有序列同源性,但是它们在限制细胞质中的激酶方面可互换地起作用。 SRPK1中间隔子的去除对激酶活性几乎没有影响,但是它导致了激酶向核的定量转移,并因此诱导了剪接因子在核中的聚集。我们没有像先前建议的那样携带核输出信号,而是在间隔区中发现了多个冗余信号,这些信号共同作用将激酶锚定在细胞质中。有趣的是,细胞周期信号诱导激酶在G(2)/ M边界的核易位。这些发现表明,SRPKs在将信号转导至高级真核细胞的RNA代谢中可能发挥重要作用。

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