Structural Basis for the Antiproliferative Activity of the Tob-hCaf1
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Authors: | Masataka Horiuchi Kosei Takeuchi Nobuo Noda Nobuyuki Muroya Toru Suzuki Takahisa Nakamura Junko Kawamura-Tsuzuku Kiyohiro Takahasi Tadashi Yamamoto Fuyuhiko Inagaki |
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Affiliation: | ‡Department of Structural Biology, Graduate School of Pharmaceutical Sciences, Hokkaido University, N12, W6, Kita-ku, Sapporo 060-0812, Japan, the §Division of Molecular and Cellular Biology, Graduate School of Medical and Dental Sciences, Niigata University, Asahi-machi, Chuo-ku, Niigata 951-8510, Japan, and the ¶Department of Oncology, Institute of Medical Science, University of Tokyo, 4-6-1 Shiroganedai, Minato-ku, Tokyo 108-8639, Japan |
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Abstract: | The Tob/BTG family is a group of antiproliferative proteins containing two highly homologous regions, Box A and Box B. These proteins all associate with CCR4-associated factor 1 (Caf1), which belongs to the ribonuclease D (RNase D) family of deadenylases and is a component of the CCR4-Not deadenylase complex. Here we determined the crystal structure of the complex of the N-terminal region of Tob and human Caf1 (hCaf1). Tob exhibited a novel fold, whereas hCaf1 most closely resembled the catalytic domain of yeast Pop2 and human poly(A)-specific ribonuclease. Interestingly, the association of hCaf1 was mediated by both Box A and Box B of Tob. Cell growth assays using both wild-type and mutant proteins revealed that deadenylase activity of Caf1 is not critical but complex formation is crucial to cell growth inhibition. Caf1 tethers Tob to the CCR4-Not deadenylase complex, and thereby Tob gathers several factors at its C-terminal region, such as poly(A)-binding proteins, to exert antiproliferative activity.The Tob/BTG family (also called the APRO family) is a group of antiproliferative proteins (1, 2) consisting of Tob (3), Tob2 (4), BTG1 (5), BTG2/Tis21/PC3 (6-8), PC3B (9), and ANA/BTG3 (10, 11) in mammalian cells, {"type":"entrez-nucleotide","attrs":{"text":"AF177464","term_id":"5916227","term_text":"AF177464"}}AF177464 in Drosophila, and FOG-3 in Caenorhabditis elegans (12). A recent genome project reported that the BTG/Tob family protein had already existed in Choanoflagellida Monosiga brevicollis MX1. The N-terminal region of the Tob/BTG family proteins is conserved and includes two highly homologous regions, Box A and Box B. The Tob/BTG family proteins are involved in cell cycle regulation in a variety of cells such as T lymphocytes, fibroblasts, epithelial cells, and germ cells. In Tob-deficient mice, the incidence of liver tumors is higher than in wild-type mice. Furthermore, because the levels of tob expression are often repressed in human lung cancers, suppression of its expression is thought to contribute to tumor progression (13).The antiproliferative activities of the Tob/BTG family proteins are due to their association with target proteins in cells. For example, Tob associates with SMAD family proteins and acts as a negative regulator of SMAD signaling. In osteoblasts, this negative regulation occurs via association with SMAD 1, 5, 6, and 8 (14, 15), and via association with SMAD 2 and 4 in anergic quiescent T cells (16). Tob/BTG family proteins also bind to protein arginine methyltransferase, which regulates chromatin assembly by histone methylation (17). Much evidence has been accumulated to suggest that CCR4-associated factor 1 (Caf1),2 also known as Cnot7 and involved in the CCR4-Not deadenylase complex, is a common binding partner of the Tob/BTG family proteins (4, 18-21). To reveal the functions of Caf1 in vivo, caf1-/- mice have been generated in two groups. Male caf1-deficient mice are infertile because of a malfunction of the testicular somatic cells that leads to a defect in spermatogenesis (22, 23). Genetic analysis of the nematode C. elegans also suggests that FOG3 (Tob orthologue) interacts with CCF1, the C. elegans homologue of Caf1, and that this interaction is essential for germ cells to initiate spermatogenesis (24).Mouse and human Caf1 (mCaf1 and hCaf1) were found as homologues of yeast Pop2, a component of the CCR4-Not complex (18, 25). Yeast Pop2 displays weak RNase activity but enhances the deadenylation of the poly(A) tail of mRNA by the CCR4-Not deadenylase complex (26-29). The primary structure of mammalian Caf1 is related to that of the ribonuclease D (RNase D) family, and all of the active site residues are well conserved (30). Indeed, both mCaf1 and hCaf1 have deadenylase activity (31-33).Although the relationship between cell cycle repression and poly(A) deadenylation is not well understood, mRNA degradation and synthesis are major events in maintaining the cell cycle (34). The mRNAs in a eukaryotic cell have a wide range of half-lives. Degradation of mRNA is initiated by shortening of the poly(A) tail. Thereafter, the 5′-cap structure is removed and the remaining portion of the mRNA is rapidly degraded. The degradation of eukaryotic mRNAs is regulated precisely at each stage of the cell cycle. Tob was reported to associate with inducible poly(A)-binding protein (iPABP) and to abrogate the translation of interleukin-2 mRNA in vitro (35). Recent reports also showed that Tob and BTG2 interact with the CCR4-Not deadenylase complex using the Tob/BTG2 domain and the cytoplasmic poly(A)-binding protein (PABPC1) using the C-terminal tail and enhanced mRNA degradation (36-38).To help elucidate the relationship between the antiproliferative activity of Tob and the degradation of the poly(A) tail, we determined the crystal structure of the Tob-hCaf1 complex. We found that hCaf1 has a structure similar to yeast Pop2 and human PARN of deadenylases, exonuclease I, and the Klenow fragment of DNA polymerase I from Escherichia coli. In contrast, Tob has a novel structure. Specifically, Box A and Box B mediate the interaction between Tob and hCaf1. Cell growth assays using the wild and mutant proteins, together with the structural studies, revealed that the complex formation is crucial to cell growth inhibition. |
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