Lin R, Heylbroeck C, Pitha P M, Hiscott J
Terry Fox Molecular Oncology Group, Lady Davis Institute for Medical Research, McGill University, Montreal, Quebec, Canada.
Mol Cell Biol. 1998 May;18(5):2986-96. doi: 10.1128/MCB.18.5.2986.
The interferon regulatory factors (IRF) consist of a growing family of related transcription proteins first identified as regulators of the alpha beta interferon (IFN-alpha/beta) gene promoters, as well as the interferon-stimulated response element (ISRE) of some IFN-stimulated genes. IRF-3 was originally identified as a member of the IRF family based on homology with other IRF family members and on binding to the ISRE of the ISG15 promoter. IRF-3 is expressed constitutively in a variety of tissues, and the relative levels of IRF-3 mRNA do not change in virus-infected or IFN-treated cells. In the present study, we demonstrate that following Sendai virus infection, IRF-3 is posttranslationally modified by protein phosphorylation at multiple serine and threonine residues, which are located in the carboxy terminus of IRF-3. A combination of IRF-3 deletion and point mutations localized the inducible phosphorylation sites to the region -ISNSHPLSLTSDQ- between amino acids 395 and 407; point mutation of residues Ser-396 and Ser-398 eliminated virus-induced phosphorylation of IRF-3 protein, although residues Ser-402, Thr-404, and Ser-405 were also targets. Phosphorylation results in the cytoplasm-to-nucleus translocation of IRF-3, DNA binding, and increased transcriptional activation. Substitution of the Ser-Thr sites with the phosphomimetic Asp generated a constitutively active form of IRF-3 that functioned as a very strong activator of promoters containing PRDI-PRDIII or ISRE regulatory elements. Phosphorylation also appears to represent a signal for virus-mediated degradation, since the virus-induced turnover of IRF-3 was prevented by mutation of the IRF-3 Ser-Thr cluster or by proteasome inhibitors. Interestingly, virus infection resulted in the association of IRF-3 with the CREB binding protein (CBP) coactivator, as detected by coimmunoprecipitation with anti-CBP antibody, an interaction mediated by the C-terminal domains of both proteins. Mutation of residues Ser-396 and Ser-398 in IRF-3 abrogated its binding to CBP. These results are discussed in terms of a model in which virus-inducible, C-terminal phosphorylation of IRF-3 alters protein conformation to permit nuclear translocation, association with transcriptional partners, and primary activation of IFN- and IFN-responsive genes.
干扰素调节因子(IRF)是一个不断扩大的相关转录蛋白家族,最初被鉴定为αβ干扰素(IFN-α/β)基因启动子以及一些干扰素刺激基因的干扰素刺激反应元件(ISRE)的调节因子。IRF-3最初是基于与其他IRF家族成员的同源性以及与ISG15启动子的ISRE结合而被鉴定为IRF家族的一员。IRF-3在多种组织中组成性表达,并且在病毒感染或干扰素处理的细胞中IRF-3 mRNA的相对水平不变。在本研究中,我们证明在仙台病毒感染后,IRF-3在多个丝氨酸和苏氨酸残基上进行翻译后蛋白磷酸化修饰,这些残基位于IRF-3的羧基末端。IRF-3缺失和点突变的组合将诱导性磷酸化位点定位到氨基酸395和407之间的-ISNSHPLSLTSDQ-区域;丝氨酸-396和丝氨酸-398残基的点突变消除了病毒诱导的IRF-3蛋白磷酸化,尽管丝氨酸-402、苏氨酸-404和丝氨酸-405残基也是靶点。磷酸化导致IRF-3从细胞质向细胞核易位、DNA结合以及转录激活增加。用模拟磷酸化的天冬氨酸取代丝氨酸-苏氨酸位点产生了一种组成性激活形式的IRF-3,它作为含有PRDI-PRDIII或ISRE调节元件的启动子的非常强的激活剂发挥作用。磷酸化似乎也代表了病毒介导降解的信号,因为IRF-3丝氨酸-苏氨酸簇的突变或蛋白酶体抑制剂阻止了病毒诱导的IRF-3周转。有趣的是,如用抗CBP抗体进行共免疫沉淀所检测到的,病毒感染导致IRF-3与CREB结合蛋白(CBP)共激活因子结合,这种相互作用由两种蛋白的C末端结构域介导。IRF-3中丝氨酸-396和丝氨酸-398残基的突变消除了它与CBP的结合。根据一个模型对这些结果进行了讨论,在该模型中,病毒诱导的IRF-3 C末端磷酸化改变蛋白构象以允许核易位、与转录伙伴结合以及IFN和IFN反应基因的初级激活。
