Brower Christopher S, Rosen Connor E, Jones Richard H, Wadas Brandon C, Piatkov Konstantin I, Varshavsky Alexander
Division of Biology, California Institute of Technology, Pasadena, CA 91125.
Division of Biology, California Institute of Technology, Pasadena, CA 91125
Proc Natl Acad Sci U S A. 2014 Nov 18;111(46):E4936-45. doi: 10.1073/pnas.1419587111. Epub 2014 Nov 4.
The arginyltransferase Ate1 is a component of the N-end rule pathway, which recognizes proteins containing N-terminal degradation signals called N-degrons, polyubiquitylates these proteins, and thereby causes their degradation by the proteasome. At least six isoforms of mouse Ate1 are produced through alternative splicing of Ate1 pre-mRNA. We identified a previously uncharacterized mouse protein, termed Liat1 (ligand of Ate1), that interacts with Ate1 but does not appear to be its arginylation substrate. Liat1 has a higher affinity for the isoforms Ate1(1A7A) and Ate1(1B7A). Liat1 stimulated the in vitro N-terminal arginylation of a model substrate by Ate1. All examined vertebrate and some invertebrate genomes encode proteins sequelogous (similar in sequence) to mouse Liat1. Sequelogs of Liat1 share a highly conserved ∼30-residue region that is shown here to be required for the binding of Liat1 to Ate1. We also identified non-Ate1 proteins that interact with Liat1. In contrast to Liat1 genes of nonprimate mammals, Liat1 genes of primates are subtelomeric, a location that tends to confer evolutionary instability on a gene. Remarkably, Liat1 proteins of some primates, from macaques to humans, contain tandem repeats of a 10-residue sequence, whereas Liat1 proteins of other mammals contain a single copy of this motif. Quantities of these repeats are, in general, different in Liat1 of different primates. For example, there are 1, 4, 13, 13, 17, and 17 repeats in the gibbon, gorilla, orangutan, bonobo, neanderthal, and human Liat1, respectively, suggesting that repeat number changes in this previously uncharacterized protein may contribute to evolution of primates.
精氨酰转移酶Ate1是N端规则途径的一个组成部分,该途径识别含有称为N-降解子的N端降解信号的蛋白质,将这些蛋白质多聚泛素化,从而导致它们被蛋白酶体降解。小鼠Ate1至少有六种同工型是通过Ate1前体mRNA的可变剪接产生的。我们鉴定出一种以前未被表征的小鼠蛋白质,称为Liat1(Ate1的配体),它与Ate1相互作用,但似乎不是其精氨酰化底物。Liat1对同工型Ate1(1A7A)和Ate1(1B7A)具有更高的亲和力。Liat1刺激了Ate1对模型底物的体外N端精氨酰化。所有检测的脊椎动物和一些无脊椎动物基因组都编码与小鼠Liat1序列相似的蛋白质(序列同源)。Liat1的序列同源物共享一个高度保守的约30个残基的区域,此处显示该区域是Liat1与Ate1结合所必需的。我们还鉴定出了与Liat1相互作用的非Ate1蛋白质。与非灵长类哺乳动物的Liat1基因不同,灵长类动物的Liat1基因位于亚端粒区域,该位置往往会使基因在进化上不稳定。值得注意的是,从猕猴到人类的一些灵长类动物的Liat1蛋白包含一个10个残基序列的串联重复,而其他哺乳动物的Liat1蛋白包含该基序的单拷贝。一般来说,不同灵长类动物的Liat1中这些重复的数量不同。例如,长臂猿、大猩猩、猩猩、倭黑猩猩、尼安德特人和人类的Liat1中分别有1、4、13、13、17和17个重复序列,这表明这种以前未被表征的蛋白质中的重复序列数量变化可能对灵长类动物的进化有贡献。