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PKC-mediated phosphorylation of nuclear lamins at a single serine residue regulates interphase nuclear size in Xenopus and mammalian cells

机译:PKC介导的单个丝氨酸残基核纤层蛋白的磷酸化调节爪蟾和哺乳动物细胞的相间核大小

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摘要

How nuclear size is regulated is a fundamental cell-biological question with relevance to cancers, which often exhibit enlarged nuclei. We previously reported that conventional protein kinase C (cPKC) contributes to nuclear size reductions that occur during early Xenopus development. Here we report that PKC-mediated phosphorylation of lamin B3 (LB3) contributes to this mechanism of nuclear size regulation. By mapping PKC phosphorylation sites on LB3 and testing the effects of phosphomutants in Xenopus laevis embryos, we identify the novel site S267 as being an important determinant of nuclear size. Furthermore, FRAP studies demonstrate that phosphorylation at this site increases lamina dynamics, providing a mechanistic explanation for how PKC activity influences nuclear size. We subsequently map this X. laevis LB3 phosphorylation site to a conserved site in mammalian lamin A (LA), S268. Manipulating PKC activity in cultured mammalian cells alters nuclear size, as does expression of LA-S268 phosphomutants. Taken together, these data demonstrate that PKC-mediated lamin phosphorylation is a conserved mechanism of nuclear size regulation.
机译:如何调节核大小是一个与癌症有关的基本细胞生物学问题,而癌症通常表现出核增大。我们先前曾报道常规蛋白激酶C(cPKC)有助于非洲爪蟾早期发育期间发生的核尺寸减小。在这里我们报告说,PKC介导的层粘连蛋白B3(LB3)的磷酸化有助于核大小调节的这一机制。通过绘制LB3上的PKC磷酸化位点并测试非洲爪蟾胚胎中的磷突变体的作用,我们确定了新位点S267是核大小的重要决定因素。此外,FRAP研究表明,该位点的磷酸化增加了椎板动力学,为PKC活性如何影响核大小提供了机械解释。我们随后将此X. laevis LB3磷酸化位点定位到哺乳动物层粘连蛋白A(LA)S268中的保守位点。操纵培养的哺乳动物细胞中的PKC活性会改变核的大小,就像LA-S268磷酸突变体的表达一样。综上所述,这些数据表明PKC介导的核纤层蛋白磷酸化是核大小调节的保守机制。

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