Structural basis for the assembly of the SMRT/NCoR core transcriptional repression machinery

Oberoi, Jasmeen; Fairall, Louise; Watson, Peter J.; Yang, Jiaqi; Czimmerer, Zsolt; Kampmann, T.; Goult, Benjamin T.; Greenwood, Jacquie A.; Gooch, John; Kallenberger, Bettina C.; Nagy, László; Neuhaus, David; Schwabe, John W. R.

doi:10.1038/nsmb.1983

Cited by 140 publications

(164 citation statements)

References 61 publications

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“…None of these constructs bound to a control NID peptide containing the RTT mutation K305R, confirming specificity. We noted that residues 227-297 of NCoR1, which appear to be involved in binding MeCP2, overlap with the NCoR1 region that interacts with TBL1 and TBLR1 (NCoR1 residues 247-256) (22). This overlap in interaction site suggested that the MeCP2-NCoR1 interaction might be indirect, mediated by interaction of MeCP2 with endogenous TBL1/TBLR1 present in cell lysates.…”

Section: Mecp2mentioning

confidence: 84%

Structure of the MeCP2–TBLR1 complex reveals a molecular basis for Rett syndrome and related disorders

Kruusvee

Lyst

Taylor

et al. 2017

Proc. Natl. Acad. Sci. U.S.A.

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Rett syndrome (RTT) is an X-linked neurological disorder caused by mutations in the methyl-CpG-binding protein 2 (MeCP2) gene. The majority of RTT missense mutations disrupt the interaction of the MeCP2 with DNA or the nuclear receptor corepressor (NCoR)/silencing mediator of retinoic acid and thyroid receptors (SMRT) corepressor complex. Here, we show that the "NCoR/SMRT interaction domain" (NID) of MeCP2 directly contacts transducin beta-like 1 (TBL1) and TBL1 related (TBLR1), two paralogs that are core components of NCoR/SMRT. We determine the cocrystal structure of the MeCP2 NID in complex with the WD40 domain of TBLR1 and confirm by in vitro and ex vivo assays that mutation of interacting residues of TBLR1 and TBL1 disrupts binding to MeCP2. Strikingly, the four MeCP2-NID residues mutated in RTT are those residues that make the most extensive contacts with TBLR1. Moreover, missense mutations in the gene for TBLR1 that are associated with intellectual disability also prevent MeCP2 binding. Our study therefore reveals the molecular basis of an interaction that is crucial for optimal brain function.T he methyl-CpG-binding protein 2 (MeCP2) is a chromatinassociated factor that is highly expressed in the brain (1, 2). Loss-of-function mutations in MeCP2 lead to the severe pediatric neurological disorder, Rett syndrome (RTT) (3), which affects around one in 10,000 girls. In addition, extra copies of the gene cause MeCP2 duplication syndrome (4, 5), a distinct intellectual disability disorder that predominantly affects males (6). The importance of MeCP2 for brain function has prompted investigation of its molecular function. The protein was identified because of its ability to bind DNA via its methyl-CpG-binding domain (MBD) (1, 7) and many residues mutated in RTT disrupt this interaction (8-11). In addition to DNA, numerous protein partners of MeCP2 have been reported (11). Of these protein partners, only the interactions with the nuclear receptor corepressor (NCoR) and its close relative silencing mediator of retinoic acid and thyroid receptors (SMRT) (12-14) are known to be disrupted by RTT missense mutations (13). Accordingly, Rett missense mutations outside the MBD are found clustered within the so-called "NCoR/SMRT interaction domain" (NID) (13) (Fig. 1A and Fig. S1A). One NID mutation, R306C, causes a severe RTT-like phenotype in mice (13,15,16). Moreover, mouse models of MeCP2 duplication syndrome suggest that both the MBD and the NID must be intact for this adverse molecular pathology to develop (16,17).These findings indicate that the NID mediates an essential function of MeCP2. This function may be recruitment of the NCoR/ SMRT corepressor complexes to chromatin. Alternatively, the NID may perform other essential roles, such as DNA binding, whose loss leads to RTT (16). In an attempt to distinguish among these possibilities, we investigated the molecular basis of the interaction between MeCP2 and NCoR/SMRT. The latter are ∼1.2-MDa multisubunit complexes that include NCoR1 (and/or SMRT), HDAC3, GPS2, and...

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Section: Mecp2mentioning

confidence: 84%

Structure of the MeCP2–TBLR1 complex reveals a molecular basis for Rett syndrome and related disorders

Kruusvee

Lyst

Taylor

et al. 2017

Proc. Natl. Acad. Sci. U.S.A.

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“…Recent biochemical studies have highlighted the assembly of the subunit GPS2 into both SMRT and NCOR1 complexes and suggest a structural core function of GPS2 in both (49). However, ChIP assays combined with RNAi also indicated the existence of SMRT and NCOR1 complexes, along with the HDAC3, TBL1, and TBLR1 subunits, that occupied different genes -in macrophages or hepatocytes -despite the lack of GPS2 (29,34).…”

Section: Figurementioning

confidence: 99%

SMRT-GPS2 corepressor pathway dysregulation coincides with obesity-linked adipocyte inflammation

Toubal¹,

Clément²,

Fan³

et al. 2012

J. Clin. Invest.

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Low-grade chronic inflammation is a major characteristic of obesity and results from deregulated white adipose tissue function. Consequently, there is interest in identifying the underlying regulatory mechanisms and components that drive adipocyte inflammation. Here, we report that expression of the transcriptional corepressor complex subunits GPS2 and SMRT was significantly reduced in obese adipose tissue, inversely correlated to inflammatory status, and was restored upon gastric bypass surgery-induced weight loss in morbid obesity. These alterations correlated with reduced occupancy of the corepressor complex at inflammatory promoters, providing a mechanistic explanation for elevated inflammatory transcription. In support of these correlations, RNAi-mediated depletion of GPS2 and SMRT from cultured human adipocytes promoted derepression of inflammatory transcription and elevation of obesity-associated inflammatory markers, such as IL-6 and MCP-1. Furthermore, we identified a regulatory cascade containing PPARγ and TWIST1 that controlled the expression of GPS2 and SMRT in human adipocytes. These findings were clinically relevant, because treatment of diabetic obese patients with pioglitazone, an antidiabetic and antiinflammatory PPARγ agonist, restored expression of TWIST1, GPS2, and SMRT in adipose tissue. Collectively, our findings identify alterations in a regulatory transcriptional network in adipocytes involving the dysregulation of a specific corepressor complex as among the initiating events promoting adipose tissue inflammation in human obesity.

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“…Both proteins contain a LisH domain. LisH-dependent dimerization has been observed for several proteins (Kim et al, 2004;Mikolajka et al, 2006;Oberoi et al, 2011;Delto et al, 2015). This data suggests that the LisH domains encoded by AT5G09630 and AT4G37880 mediate their selfinteraction.…”

Section: Identification Of Mrctlh Components In Arabidopsis Thalianamentioning

confidence: 89%

Integrative meta-analysis of protein interaction data identified multiple GID/MRCTLH protein complexes in plants

Miquel¹,

Vicient²

2017

Plant Omics

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GID/MRCTLH is a protein complex involved in the regulation of several cellular processes through the polyubiquitination and proteosome degradation. It has been described in yeast and mammals. Genes coding for homologous proteins are also present in plant genomes but have been little studied. BLAST analyses revealed that genes coding for members of the GID/MRCTLH complex are found in multiple copies in plants, compared to mammals and yeast. The potential structure of the Arabidopsis GID/MRCTLH complex was estimated based on the Arabidopsis protein interaction database Interactome 2.0. According to these data, Arabidopsis may contain two GID/MRCTLH complexes instead of the one described in yeast and mammals. The structure of the two Arabidopsis complexes seem to be similar to the yeast GID complex, and seem to interact with several other proteins out of the complex. These data suggest that, similarly to yeast and mammals, the plant GID/MRCTLH complexes are involved in the regulation of several cellular processes through proteosome protein degradation.

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Structural basis for the assembly of the SMRT/NCoR core transcriptional repression machinery

Cited by 140 publications

References 61 publications

Structure of the MeCP2–TBLR1 complex reveals a molecular basis for Rett syndrome and related disorders

Structure of the MeCP2–TBLR1 complex reveals a molecular basis for Rett syndrome and related disorders

SMRT-GPS2 corepressor pathway dysregulation coincides with obesity-linked adipocyte inflammation

Integrative meta-analysis of protein interaction data identified multiple GID/MRCTLH protein complexes in plants

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