Functional Analysis of the SIN3-Histone Deacetylase RPD3-RbAp48-Histone H4 Connection in the XenopusOocyte

ABSTRACT We investigated the protein associations and enzymatic requirements for the Xenopus histone deacetylase catalytic subunit RPD3 to direct transcriptional repression in Xenopus oocytes. Endogenous Xenopus RPD3 is present in nuclear and cytoplasmic pools, whereas RbAp48 and SIN3 are predominantly nuclear. We cloned Xenopus RbAp48 and SIN3 and show that expression of RPD3, but not RbAp48 or SIN3, leads to an increase in nuclear and cytoplasmic histone deacetylase activity and transcriptional repression of the TRβA promoter. This repression requires deacetylase activity and nuclear import of RPD3 mediated by a carboxy-terminal nuclear localization signal. Exogenous RPD3 is not incorporated into previously described oocyte deacetylase and ATPase complexes but cofractionates with a component of the endogenous RbAp48 in the oocyte nucleus. We show that RPD3 associates with RbAp48 through N- and C-terminal contacts and that RbAp48 also interacts with SIN3. XenopusRbAp48 selectively binds to the segment of the N-terminal tail immediately proximal to the histone fold domain of histone H4 in vivo. Exogenous RPD3 may be targeted to histones through interaction with endogenous RbAp48 to direct transcriptional repression of theXenopus TRβA promoter in the oocyte nucleus. However, the exogenous RPD3 deacetylase functions to repress transcription in the absence of a requirement for association with SIN3 or other targeted corepressors.

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Saccharomyces cerevisiae BUR6 encodes a DRAP1/NC2alpha homolog that has both positive and negative roles in transcription in vivo.

Molecular and Cellular Biology ◽

10.1128/mcb.17.4.2057 ◽

1997 ◽

Vol 17 (4) ◽

pp. 2057-2065 ◽

Cited By ~ 60

Author(s):

G Prelich

Keyword(s):

Saccharomyces Cerevisiae ◽

Essential Gene ◽

Nucleotide Sequence Analysis ◽

Detectable Effect ◽

Histone Fold ◽

Histone Fold Domain ◽

Tata Box Binding Protein ◽

Mutant Phenotypes ◽

Carboxy Terminal

BUR3 and BUR6 were identified previously by selecting for mutations that increase transcription from an upstream activating sequence (UAS)-less promoter in Saccharomyces cerevisiae. The bur3-1 and bur6-1 mutations are recessive, increase transcription from a suc2 delta uas allele, and cause other mutant phenotypes, suggesting that Bur3p and Bur6p function as general repressors of the basal transcriptional machinery. The molecular cloning and characterization of BUR3 and BUR6 are presented here. BUR3 is identical to MOT1, a previously characterized essential gene that encodes an ATP-dependent inhibitor of the TATA box-binding protein. Cloning and nucleotide sequence analysis reveals that BUR6 encodes a homolog of DRAP1 (also called NC2alpha), a mammalian repressor of basal transcription. Strains that contain a bur6 null allele are viable but grow extremely poorly, demonstrating that BUR6 is critical for normal cell growth in yeast. The Bur6p histone fold domain is required for function; an extensive nonoverlapping set of deletion alleles throughout the histone fold domain impairs BUR6 function in vivo, whereas mutations in the amino- and carboxy-terminal tails have no detectable effect. BUR6 and BUR3/MOT1 have different functions depending on promoter context: although the bur3-1 and bur6-1 mutations increase transcription from delta uas promoters, they result in reduced transcription from the wild-type GAL1 and GAL10 promoters. This transcriptional defect is due to the inability of the GAL10 UAS to function in bur6-1 strains. The similar phenotypes of bur6 and bur3 (mot1) mutations suggest that Bur6p and Mot1p have related, but not identical, functions in modulating the activity of the general transcription machinery in vivo.

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A Functional Interaction between the Carboxy-Terminal Domain of RNA Polymerase II and Pre-mRNA Splicing

The Journal of Cell Biology ◽

10.1083/jcb.136.1.5 ◽

1997 ◽

Vol 136 (1) ◽

pp. 5-18 ◽

Cited By ~ 91

Author(s):

Lei Du ◽

Stephen L. Warren

Keyword(s):

Rna Polymerase Ii ◽

Mammalian Cells ◽

Mrna Splicing ◽

Splicing Factors ◽

Functional Interaction ◽

Carboxy Terminal Domain ◽

Localization Signal ◽

Nuclear Domains ◽

Carboxy Terminal

In the preceding study we found that Sm snRNPs and SerArg (SR) family proteins co-immunoprecipitate with Pol II molecules containing a hyperphosphorylated CTD (Kim et al., 1997). The association between Pol IIo and splicing factors is maintained in the absence of pre-mRNA, and the polymerase need not be transcriptionally engaged (Kim et al., 1997). The latter findings led us to hypothesize that a phosphorylated form of the CTD interacts with pre-mRNA splicing components in vivo. To test this idea, a nested set of CTD-derived proteins was assayed for the ability to alter the nuclear distribution of splicing factors, and to interfere with splicing in vivo. Proteins containing heptapeptides 1-52 (CTD52), 1-32 (CTD32), 1-26 (CTD26), 1-13 (CTD13), 1-6 (CTD6), 1-3 (CTD3), or 1 (CTD1) were expressed in mammalian cells. The CTD-derived proteins become phosphorylated in vivo, and accumulate in the nucleus even though they lack a conventional nuclear localization signal. CTD52 induces a selective reorganization of splicing factors from discrete nuclear domains to the diffuse nucleoplasm, and significantly, it blocks the accumulation of spliced, but not unspliced, human β-globin transcripts. The extent of splicing factor disruption, and the degree of inhibition of splicing, are proportional to the number of heptapeptides added to the protein. The above results indicate a functional interaction between Pol II's CTD and pre-mRNA splicing.

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Mapping and Functional Characterization of the TAF11 Interaction with TFIIA

Molecular and Cellular Biology ◽

10.1128/mcb.25.3.945-957.2005 ◽

2005 ◽

Vol 25 (3) ◽

pp. 945-957 ◽

Cited By ~ 19

Author(s):

M. M. Robinson ◽

G. Yatherajam ◽

R. T. Ranallo ◽

A. Bric ◽

M. R. Paule ◽

...

Keyword(s):

Functional Characterization ◽

Regulation Of Gene Expression ◽

Small Subunit ◽

Molecular Organization ◽

Functional Link ◽

Essential Information ◽

Histone Fold ◽

Histone Fold Domain ◽

Promoter Dna

ABSTRACT TFIIA interacts with TFIID via association with TATA binding protein (TBP) and TBP-associated factor 11 (TAF11). We previously identified a mutation in the small subunit of TFIIA (toa2-I27K) that is defective for interaction with TAF11. To further explore the functional link between TFIIA and TAF11, the toa2-I27K allele was utilized in a genetic screen to isolate compensatory mutants in TAF11. Analysis of these compensatory mutants revealed that the interaction between TAF11 and TFIIA involves two distinct regions of TAF11: the highly conserved histone fold domain and the N-terminal region. Cells expressing a TAF11 allele defective for interaction with TFIIA exhibit conditional growth phenotypes and defects in transcription. Moreover, TAF11 imparts changes to both TFIIA-DNA and TBP-DNA contacts in the context of promoter DNA. These alterations appear to enhance the formation and stabilization of the TFIIA-TBP-DNA complex. Taken together, these studies provide essential information regarding the molecular organization of the TAF11-TFIIA interaction and define a mechanistic role for this association in the regulation of gene expression in vivo.

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The TFIID Components Human TAFII140 andDrosophila BIP2 (TAFII155) Are Novel Metazoan Homologues of Yeast TAFII47 Containing a Histone Fold and a PHD Finger

Molecular and Cellular Biology ◽

10.1128/mcb.21.15.5109-5121.2001 ◽

2001 ◽

Vol 21 (15) ◽

pp. 5109-5121 ◽

Cited By ~ 42

Author(s):

Yann-Gaël Gangloff ◽

Jean-Christophe Pointud ◽

Sylvie Thuault ◽

Lucie Carré ◽

Christophe Romier ◽

...

Keyword(s):

Rna Polymerase Ii ◽

Sequence Similarity ◽

Protein A ◽

Amino Acid Sequences ◽

Molecular Organization ◽

Phd Finger ◽

Histone Fold ◽

Histone Fold Domain ◽

High Degree

ABSTRACT The RNA polymerase II transcription factor TFIID comprises the TATA binding protein (TBP) and a set of TBP-associated factors (TAFIIs). TFIID has been extensively characterized for yeast, Drosophila, and humans, demonstrating a high degree of conservation of both the amino acid sequences of the constituent TAFIIs and overall molecular organization. In recent years, it has been assumed that all the metazoan TAFIIs have been identified, yet no metazoan homologues of yeast TAFII47 (yTAFII47) and yTAFII65 are known. Both of these yTAFIIs contain a histone fold domain (HFD) which selectively heterodimerizes with that of yTAFII25. We have cloned a novel mouse protein, TAFII140, containing an HFD and a plant homeodomain (PHD) finger, which we demonstrated by immunoprecipitation to be a mammalian TFIID component. TAFII140 shows extensive sequence similarity toDrosophila BIP2 (dBIP2) (dTAFII155), which we also show to be a component of DrosophilaTFIID. These proteins are metazoan homologues of yTAFII47 as their HFDs selectively heterodimerize with dTAFII24 and human TAFII30, metazoan homologues of yTAFII25. We further show that yTAFII65 shares two domains with theDrosophila Prodos protein, a recently described potential dTAFII. These conserved domains are critical for yTAFII65 function in vivo. Our results therefore identify metazoan homologues of yTAFII47 and yTAFII65.

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Subunits of the Heterotrimeric Transcription Factor NF-Y Are Imported into the Nucleus by Distinct Pathways Involving Importin β and Importin 13

Molecular and Cellular Biology ◽

10.1128/mcb.25.13.5339-5354.2005 ◽

2005 ◽

Vol 25 (13) ◽

pp. 5339-5354 ◽

Cited By ~ 79

Author(s):

Joerg Kahle ◽

Matthias Baake ◽

Detlef Doenecke ◽

Werner Albig

Keyword(s):

Nuclear Import ◽

Mutational Analysis ◽

Dependent Manner ◽

Amino Acid Residues ◽

Nuclear Targeting ◽

Binding Studies ◽

Histone Fold ◽

Localization Signal ◽

Conserved Core

ABSTRACT The transcriptional activator NF-Y is a heterotrimeric complex composed of NF-YA, NF-YB, and NF-YC, which specifically binds the CCAAT consensus present in about 30% of eukaryotic promoters. All three subunits contain evolutionarily conserved core regions, which comprise a histone fold motif (HFM) in the case of NF-YB and NF-YC. Our results of in vitro binding studies and nuclear import assays reveal two different transport mechanisms for NF-Y subunits. While NF-YA is imported by an importin β-mediated pathway, the NF-YB/NF-YC heterodimer is translocated into the nucleus in an importin 13-dependent manner. We define a nonclassical nuclear localization signal (ncNLS) in NF-YA, and mutational analysis indicates that positively charged amino acid residues in the ncNLS are required for nuclear targeting of NF-YA. Importin β binding is restricted to the monomeric, uncomplexed NF-YA subunit. In contrast, the nuclear import of NF-YB and NF-YC requires dimer formation. Only the NF-YB/NF-YC dimer, but not the monomeric components, are recognized by importin 13 and are imported into the nucleus. Importin 13 competes with NF-YA for binding to the NF-YB/NF-YC dimer. Our data suggest that a distinct binding platform derived from the HFM of both subunits, NF-YB/NF-YC, mediates those interactions.

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MafG Sumoylation Is Required for Active Transcriptional Repression

Molecular and Cellular Biology ◽

10.1128/mcb.02193-05 ◽

2006 ◽

Vol 26 (12) ◽

pp. 4652-4663 ◽

Cited By ~ 36

Author(s):

Hozumi Motohashi ◽

Fumiki Katsuoka ◽

Chika Miyoshi ◽

Yasuhiro Uchimura ◽

Hisato Saitoh ◽

...

Keyword(s):

Binding Site ◽

Histone Deacetylase ◽

Transcriptional Repression ◽

Cultured Cells ◽

Physiological Role ◽

Histone Deacetylase Inhibition ◽

Dna Binding Site ◽

Repressor Complex ◽

Repressor Activity

ABSTRACT A straightforward mechanism for eliciting transcriptional repression would be to simply block the DNA binding site for activators. Such passive repression is often mediated by transcription factors that lack an intrinsic repressor activity. MafG is a bidirectional regulator of transcription, a repressor in its homodimeric state but an activator when heterodimerized with p45. Here, we report that MafG is conjugated to SUMO-2/3 in vivo. To clarify the possible physiological role(s) for sumoylation in regulating MafG activity, we evaluated mutant and wild-type MafG in transgenic mice and cultured cells. Whereas sumoylation-deficient MafG activated p45-dependent transcription normally and did not affect heterodimer activity, repression by the sumoylation-deficient MafG mutant was severely compromised in vivo. Furthermore, the SUMO-dependent repression activity of MafG was sensitive to histone deacetylase inhibition. Thus, repression by MafG is not achieved through simple passive repression by competing for the activator binding site but requires sumoylation, which then mediates transcriptional repression through recruitment of a repressor complex containing histone deacetylase activity.

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Mechanisms Directing the Nuclear Localization of the CtBP Family Proteins

Molecular and Cellular Biology ◽

10.1128/mcb.02402-05 ◽

2006 ◽

Vol 26 (13) ◽

pp. 4882-4894 ◽

Cited By ~ 47

Author(s):

Alexis Verger ◽

Kate G. R. Quinlan ◽

Linda A. Crofts ◽

Stefania Spanò ◽

Daniela Corda ◽

...

Keyword(s):

Nuclear Localization ◽

Nuclear Import ◽

Nuclear Localization Signal ◽

Transcriptional Repression ◽

Intracellular Trafficking ◽

Nuclear Accumulation ◽

Splice Isoforms ◽

Localization Signal ◽

Splice Isoform ◽

Partner Proteins

ABSTRACT The C-terminal binding protein (CtBP) family includes four proteins (CtBP1 [CtBP1-L], CtBP3/BARS [CtBP1-S], CtBP2, and RIBEYE) which are implicated both in transcriptional repression and in intracellular trafficking. However, the precise mechanisms by which different CtBP proteins are targeted to different subcellular regions remains unknown. Here, we report that the nuclear import of the various CtBP proteins and splice isoforms is differentially regulated. We show that CtBP2 contains a unique nuclear localization signal (NLS) located within its N-terminal region, which contributes to its nuclear accumulation. Using heterokaryon assays, we show that CtBP2 is capable of shuttling between the nucleus and cytoplasm of the cell. Moreover, CtBP2 can heterodimerize with CtBP1-L and CtBP1-S and direct them to the nucleus. This effect strongly depends on the CtBP2 NLS. PXDLS motif-containing transcription factors, such as BKLF, that bind CtBP proteins can also direct them to the nucleus. We also report the identification of a splice isoform of CtBP2, CtBP2-S, that lacks the N-terminal NLS and localizes to the cytoplasm. Finally, we show that mutation of the CtBP NADH binding site impairs the ability of the proteins to dimerize and to associate with BKLF. This reduces the nuclear accumulation of CtBP1. Our results suggest a model in which the nuclear localization of CtBP proteins is influenced by the CtBP2 NLS, by binding to PXDLS motif partner proteins, and through the effect of NADH on CtBP dimerization.

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Histone Folds Mediate Selective Heterodimerization of Yeast TAFII25 with TFIID Components yTAFII47 and yTAFII65 and with SAGA Component ySPT7

Molecular and Cellular Biology ◽

10.1128/mcb.21.5.1841-1853.2001 ◽

2001 ◽

Vol 21 (5) ◽

pp. 1841-1853 ◽

Cited By ~ 54

Author(s):

Yann-Gaël Gangloff ◽

Steven L. Sanders ◽

Christophe Romier ◽

Doris Kirschner ◽

P. Anthony Weil ◽

...

Keyword(s):

Temperature Sensitive ◽

Saga Complex ◽

Yeast Two Hybrid ◽

Conserved Residues ◽

Histone Fold ◽

Histone Fold Domain ◽

Necessary And Sufficient ◽

Two Hybrid ◽

Temperature Sensitive Phenotype

ABSTRACT We show that the yeast TFIID (yTFIID) component yTAFII47 contains a histone fold domain (HFD) with homology to that previously described for hTAFII135. Complementation in vivo indicates that the yTAFII47 HFD is necessary and sufficient for vegetative growth. Mutation of highly conserved residues in the α1 helix of the yTAFII47 HFD results in a temperature-sensitive phenotype which can be suppressed by overexpression of yTAFII25, as well as by yTAFII40, yTAFII19, and yTAFII60. In yeast two-hybrid and bacterial coexpression assays, the yTAFII47 HFD selectively heterodimerizes with yTAFII25, which we show contains an HFD with homology to the hTAFII28 family We additionally demonstrate that yTAFII65 contains a functional HFD which also selectively heterodimerizes with yTAFII25. These results reveal the existence of two novel histone-like pairs in yTFIID. The physical and genetic interactions described here show that the histone-like yTAFIIs are organized in at least two substructures within TFIID rather than in a single octamer-like structure as previously suggested. Furthermore, our results indicate that ySPT7 has an HFD homologous to that of yTAFII47 which selectively heterodimerizes with yTAFII25, defining a novel histone-like pair in the SAGA complex.

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The Plant NF-Y DNA Matrix In Vitro and In Vivo

Plants ◽

10.3390/plants8100406 ◽

2019 ◽

Vol 8 (10) ◽

pp. 406 ◽

Cited By ~ 2

Author(s):

Nerina Gnesutta ◽

Matteo Chiara ◽

Andrea Bernardini ◽

Matteo Balestra ◽

David S. Horner ◽

...

Keyword(s):

Saturation Mutagenesis ◽

Sequence Specificity ◽

Histone Fold ◽

Nuclear Factor Y ◽

Histone Fold Domain ◽

Genes Encoding ◽

Core Histones ◽

Ccaat Box

Nuclear Factor Y (NF-Y) is an evolutionarily conserved trimer formed by a Histone-Fold Domain (HFD) heterodimeric module shared by core histones, and the sequence-specific NF-YA subunit. In plants, the genes encoding each of the three subunits have expanded in number, giving rise to hundreds of potential trimers. While in mammals NF-Y binds a well-characterized motif, with a defined matrix centered on the CCAAT box, the specificity of the plant trimers has yet to be determined. Here we report that Arabidopsis thaliana NF-Y trimeric complexes, containing two different NF-YA subunits, bind DNA in vitro with similar affinities. We assayed precisely sequence-specificity by saturation mutagenesis, and analyzed genomic DNA sites bound in vivo by selected HFDs. The plant NF-Y CCAAT matrix is different in nucleotides flanking CCAAT with respect to the mammalian matrix, in vitro and in vivo. Our data point to flexible DNA-binding rules by plant NF-Ys, serving the scope of adapting to a diverse audience of genomic motifs.

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Nuclear import of hnRNP A1 is mediated by a novel cellular cofactor related to karyopherin-beta

Journal of Cell Science ◽

10.1242/jcs.110.11.1325 ◽

1997 ◽

Vol 110 (11) ◽

pp. 1325-1331 ◽

Cited By ~ 12

Author(s):

R.A. Fridell ◽

R. Truant ◽

L. Thorne ◽

R.E. Benson ◽

B.R. Cullen

Keyword(s):

Nuclear Import ◽

Hnrnp A1 ◽

Cellular Cofactor ◽

Basic Class ◽

Localization Signal ◽

In Trans ◽

Cellular Import ◽

Nuclear Ribonucleoprotein

Heterogeneous nuclear ribonucleoprotein A1 contains a sequence, termed M9, that functions as a potent nuclear localization signal (NLS) yet bears no similarity to the well-defined basic class of NLSs. Here, we report the identification of a novel human protein, termed MIP, that binds M9 specifically both in vivo and in vitro yet fails to interact with non-functional M9 point mutants. Of note, the 101 kDa MIP protein bears significant homology to human karyopherin/importin-beta, a protein known to mediate the function of basic NLSs. The in vitro nuclear import of a protein substrate containing the M9 NLS was found to be dependent on provision of the MIP protein in trans. Cytoplasmic microinjection of a truncated form of MIP that retains the M9 binding site blocked the in vivo nuclear import of a substrate containing the M9 NLS yet failed to affect the import of a similar substrate bearing a basic NLS. These data indicate that nuclear import of hnRNP A1 is mediated by a novel cellular import pathway that is distinct from, yet evolutionarily related to, the pathway utilized by basic NLS sequences.

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