Department of Oncology, University of Cambridge, Hutchison/Medical Research Council Research Centre, Cambridge CB2 0XZ, UK.
Development. 2011 Oct;138(19):4267-77. doi: 10.1242/dev.067900. Epub 2011 Aug 18.
During development of the central nervous system, the transition from progenitor maintenance to differentiation is directly triggered by a lengthening of the cell cycle that occurs as development progresses. However, the mechanistic basis of this regulation is unknown. The proneural transcription factor Neurogenin 2 (Ngn2) acts as a master regulator of neuronal differentiation. Here, we demonstrate that Ngn2 is phosphorylated on multiple serine-proline sites in response to rising cyclin-dependent kinase (cdk) levels. This multi-site phosphorylation results in quantitative inhibition of the ability of Ngn2 to induce neurogenesis in vivo and in vitro. Mechanistically, multi-site phosphorylation inhibits binding of Ngn2 to E box DNA, and inhibition of DNA binding depends on the number of phosphorylation sites available, quantitatively controlling promoter occupancy in a rheostat-like manner. Neuronal differentiation driven by a mutant of Ngn2 that cannot be phosphorylated by cdks is no longer inhibited by elevated cdk kinase levels. Additionally, phosphomutant Ngn2-driven neuronal differentiation shows a reduced requirement for the presence of cdk inhibitors. From these results, we propose a model whereby multi-site cdk-dependent phosphorylation of Ngn2 interprets cdk levels to control neuronal differentiation in response to cell cycle lengthening during development.
在中枢神经系统的发育过程中,从祖细胞维持到分化的转变是直接由细胞周期的延长触发的,而细胞周期的延长是随着发育的进展而发生的。然而,这种调节的机制基础尚不清楚。神经生成因子 2(Ngn2)作为神经元分化的主调控因子。在这里,我们证明 Ngn2 在响应不断上升的细胞周期蛋白依赖性激酶(cdk)水平时,在多个丝氨酸-脯氨酸位点上发生磷酸化。这种多部位磷酸化导致 Ngn2 诱导体内和体外神经发生的能力被定量抑制。从机制上讲,多部位磷酸化抑制了 Ngn2 与 E 盒 DNA 的结合,并且 DNA 结合的抑制取决于可用磷酸化位点的数量,以类似变阻器的方式定量控制启动子占据。不能被 cdk 磷酸化的 Ngn2 突变体驱动的神经元分化不再被升高的 cdk 激酶水平所抑制。此外,磷酸化突变体 Ngn2 驱动的神经元分化显示出对 cdk 抑制剂存在的需求降低。根据这些结果,我们提出了一个模型,即 Ngn2 的多部位 cdk 依赖性磷酸化解释了 cdk 水平,以控制发育过程中细胞周期延长时的神经元分化。
