Department of Biochemistry, Max Planck Institute for Developmental Biology, Tübingen, Germany.
EMBO J. 2010 Dec 15;29(24):4146-60. doi: 10.1038/emboj.2010.274. Epub 2010 Nov 9.
miRNA-mediated gene silencing requires the GW182 proteins, which are characterized by an N-terminal domain that interacts with Argonaute proteins (AGOs), and a C-terminal silencing domain (SD). In Drosophila melanogaster (Dm) GW182 and a human (Hs) orthologue, TNRC6C, the SD was previously shown to interact with the cytoplasmic poly(A)-binding protein (PABPC1). Here, we show that two regions of GW182 proteins interact with PABPC1: the first contains a PABP-interacting motif 2 (PAM2; as shown before for TNRC6C) and the second contains the M2 and C-terminal sequences in the SD. The latter mediates indirect binding to the PABPC1 N-terminal domain. In D. melanogaster cells, the second binding site dominates; however, in HsTNRC6A-C the PAM2 motif is essential for binding to both Hs and DmPABPC1. Accordingly, a single amino acid substitution in the TNRC6A-C PAM2 motif abolishes the interaction with PABPC1. This mutation also impairs TNRC6s silencing activity. Our findings reveal that despite species-specific differences in the relative strength of the PABPC1-binding sites, the interaction between GW182 proteins and PABPC1 is critical for miRNA-mediated silencing in animal cells.
miRNA 介导的基因沉默需要 GW182 蛋白,这些蛋白的特点是具有与 Argonaute 蛋白 (AGOs) 相互作用的 N 端结构域和 C 端沉默结构域 (SD)。在黑腹果蝇 (Dm) GW182 和人类 (Hs) 同源物 TNRC6C 中,SD 以前被证明与细胞质多聚 (A) 结合蛋白 (PABPC1) 相互作用。在这里,我们表明 GW182 蛋白的两个区域与 PABPC1 相互作用:第一个包含 PABP 相互作用基序 2 (PAM2;以前在 TNRC6C 中显示过),第二个包含 SD 中的 M2 和 C 端序列。后者介导与 PABPC1 N 端结构域的间接结合。在黑腹果蝇细胞中,第二个结合位点占主导地位;然而,在 HsTNRC6A-C 中,PAM2 基序对于与 Hs 和 DmPABPC1 的结合都是必不可少的。因此,TNRC6A-C PAM2 基序中的单个氨基酸取代会破坏与 PABPC1 的相互作用。这种突变也会损害 TNRC6 的沉默活性。我们的发现表明,尽管在 PABPC1 结合位点的相对强度方面存在种间差异,但 GW182 蛋白与 PABPC1 之间的相互作用对于动物细胞中 miRNA 介导的沉默至关重要。
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