Your search keyword '"Thomas Oelgeschläger"' showing total 22 results

1. Taspase1 processing alters TFIIA cofactor properties in the regulation of TFIID

Author

Diane Frances Lee, Thomas Oelgeschläger, James J. Hsieh, Valentina S Caputo, and Barbora Malecova

Subjects

Transcription, Genetic, TATA box, Repressor, RNA polymerase II, Biochemistry, Initiator element, Transcription (biology), Endopeptidases, Genetics, Humans, Promoter Regions, Genetic, TATA-Binding Protein Associated Factors, biology, fungi, Phosphoproteins, TATA Box, Molecular biology, Cell biology, DNA-Binding Proteins, Protein Subunits, TAF1, Transcription Factor TFIIA, biology.protein, Transcription Factor TFIID, RNA Polymerase II, Transcription factor II D, Transcription factor II A, Research Paper, HeLa Cells, Transcription Factors, Biotechnology

Abstract

TFIIA is an important positive regulator of TFIID, the primary promoter recognition factor of the basal RNA polymerase II transcription machinery. TFIIA antagonises negative TFIID regulators such as negative cofactor 2 (NC2), promotes specific binding of the TBP subunit of TFIID to TATA core promoter sequence elements and stimulates the interaction of TBP-associated factors (TAFs) in the TFIID complex with core promoter elements located downstream of TATA, such as the initiator element (INR). Metazoan TFIIA consists of 3 subunits, TFIIAα (35 kDa), β (19 kDa) and γ (12 kDa). TFIIAα and β subunits are encoded by a single gene and result from site-specific cleavage of a 55 kDa TFIIA(α/β) precursor protein by the protease Taspase1. Metazoan cells have been shown to contain variable amounts of TFIIA (55/12 kDa) and Taspase1-processed TFIIA (35/19/12 kDa) depending on cell type, suggesting distinct gene-specific roles of unprocessed and Taspase1-processed TFIIA. How precisely Taspase1 processing affects TFIIA functions is not understood. Here we report that Taspase1 processing alters TFIIA interactions with TFIID and the conformation of TFIID/TFIIA promoter complexes. We further show that Taspase1 processing induces increased sensitivity of TFIID/TFIIA complexes to the repressor NC2, which is counteracted by the presence of an INR core promoter element. Our results provide first evidence that Taspase1 processing affects TFIIA regulation of TFIID and suggest that Taspase1 processing of TFIIA is required to establish INR-selective core promoter activity in the presence of NC2.

Published

2015

2. SUMO-1 Modification of Human Transcription Factor (TF) IID Complex Subunits

Author

Corinne Potel, Ronald T. Hay, Thomas Oelgeschläger, Michaël Boyer-Guittaut, Gill Elliott, Ellis Jaffray, Kivanç Birsoy, and Joanna M. P. Desterro

Subjects

biology, TATA box, fungi, genetic processes, information science, RNA polymerase II, macromolecular substances, Cell Biology, Biochemistry, Molecular biology, Cell biology, TAF1, TAF4, Transcription preinitiation complex, TAF2, health occupations, biology.protein, Transcription factor II D, Molecular Biology, Transcription factor II A

Abstract

The TFIID complex is composed of the TATA-binding protein (TBP) and TBP-associated factors (TAFs) and is the only component of the general RNA polymerase II (RNAP II) transcription machinery with intrinsic sequence-specific DNA-binding activity. Binding of transcription factor (TF) IID to the core promoter region of protein-coding genes is a key event in RNAP II transcription activation and is the first and rate-limiting step of transcription initiation complex assembly. Intense research efforts in the past have established that TFIID promoter-binding activity as well as the function of TFIID-promoter complexes is tightly regulated through dynamic TFIID interactions with positive- and negative-acting transcription regulatory proteins. However, very little is known about the role of post-translational modifications in the regulation of TFIID. Here we show that the human TFIID subunits hsTAF5 and hsTAF12 are modified by the small ubiquitin-related modifier SUMO-1 in vitro and in human cells. We identify Lys-14 in hsTAF5 and Lys-19 in hsTAF12 as the primary SUMO-1 acceptor sites and show that SUMO conjugation has no detectable effect on nuclear import or intranuclear distribution of hsTAF5 and hsTAF12. Finally, we demonstrate that purified human TFIID complex can be SUMO-1-modified in vitro at both hsTAF5 and hsTAF12. We find that SUMO-1 conjugation at hsTAF5 interferes with binding of TFIID to promoter DNA, whereas modification of hsTAF12 has no detectable effect on TFIID promoter-binding activity. Our observations suggest that reversible SUMO modification at hsTAF5 contributes to the dynamic regulation of TFIID promoter-binding activity in human cells.

Published

2005

3. The Histone-Fold Protein Complex CHRAC-15/17 Enhances Nucleosome Sliding and Assembly Mediated by ACF

Author

Sarah Elderkin, Thomas Oelgeschläger, Margaret Grimaldi, Iwao Kukimoto, and Patrick Varga-Weisz

Subjects

Protein Folding, Time Factors, Recombinant Fusion Proteins, Molecular Sequence Data, Solenoid (DNA), Chromatin remodeling, Histones, Nucleosome, Animals, Humans, Chromatin structure remodeling (RSC) complex, Amino Acid Sequence, Molecular Biology, DNA Polymerase III, Glutathione Transferase, biology, Dose-Response Relationship, Drug, Sequence Homology, Amino Acid, DNA, DNA Polymerase II, Cell Biology, Molecular biology, Linker DNA, Chromatin, Cell biology, ChIP-sequencing, Nucleosomes, Protein Structure, Tertiary, DNA-Binding Proteins, Nucleoproteins, Histone fold, Chromatosome, biology.protein, Drosophila, Protein Binding

Abstract

The histone fold is a structural motif with which two related proteins interact and is found in complexes involved in wrapping DNA, the nucleosome, and transcriptional regulation, as in NC2. We reveal a novel function for histone-fold proteins: facilitation of nucleosome remodeling. ACF1-ISWI complex (ATP-dependent chromatin assembly and remodeling factor [ACF]) associates with histone-fold proteins (CHRAC-15 and CHRAC-17 in the human chromatin accessibility complex [CHRAC]) whose functional relevance has been unclear. We show that these histone-fold proteins facilitate ATP-dependent nucleosome sliding by ACF. Direct interaction of the CHRAC-15/17 complex with the ACF1 subunit is essential for this process. CHRAC-17 interacts with another histone-fold protein, p12, in DNA polymerase ϵ, but CHRAC-15 is essential for interaction with ACF and enhancement of nucleosome sliding. Surprisingly, CHRAC-15/17, p12/CHRAC-17, and NC2 complexes facilitate ACF-mediated chromatin assembly by a mechanism different from nucleosome sliding enhancement, suggesting a general activity of H2A/H2B type histone-fold complexes in chromatin assembly.

Published

2004

4. Regulation of RNA polymerase II activity by CTD phosphorylation and cell cycle control

Author

Thomas Oelgeschläger

Subjects

Physiology, Kinase, genetic processes, Clinical Biochemistry, RNA polymerase II, Cell Biology, Biology, Cell cycle, environment and public health, Cell biology, enzymes and coenzymes (carbohydrates), Transcription (biology), Cyclin-dependent kinase, health occupations, biology.protein, bacteria, Phosphorylation, CTD, Tyrosine kinase

Abstract

The carboxyl-terminal domain (CTD) of the largest subunit of mammalian RNA polymerase II (RNAP II) consists of 52 repeats of a consensus heptapeptide and is subject to phosphorylation and dephosphorylation events during each round of transcription. RNAP II activity is regulated during the cell cycle and cell cycle-dependend changes in RNAP II activity correlate well with CTD phosphorylation. In addition, global changes in the CTD phosphorylation status are observed in response to mitogenic or cytostatic signals such as growth factors, mitogens and DNA-damaging agents. Several CTD kinases are members of the cyclin-dependent kinase (CDK) superfamily and associate with transcription initiation complexes. Other CTD kinases implicated in cell cycle regulation include the mitogen-activated protein kinases ERK-1/2 and the c-Abl tyrosine kinase. These observations suggest that reversible RNAP II CTD phosphorylation may play a key role in linking cell cycle regulatory events to coordinated changes in transcription.

Published

2001

5. Transcription Activation via Enhanced Preinitiation Complex Assembly in a Human Cell-Free System Lacking TAFIIs

Author

Robert G. Roeder, Yong Tao, Yun Kyoung Kang, and Thomas Oelgeschläger

Subjects

Cell Extracts, Transcriptional Activation, Saccharomyces cerevisiae Proteins, Proline, Fungal Proteins, Humans, Promoter Regions, Genetic, Molecular Biology, TATA-Binding Protein Associated Factors, Mediator Complex, Cell-Free System, biology, General transcription factor, Cell Biology, Molecular biology, Protein Structure, Tertiary, Cell biology, DNA-Binding Proteins, Mutagenesis, Transcription preinitiation complex, Trans-Activators, Transcription factor II H, biology.protein, Transcription Factor TFIID, Transcription factor II F, Transcription factor II E, Transcription factor II D, Transcription factor II B, Transcription factor II A, HeLa Cells, Transcription Factors

Abstract

In contrast to previous findings in cell-free systems reconstituted with partially purified metazoan factors, we demonstrate dramatic activation of transcription in a TBP-dependent but TAF II -independent manner in HeLa nuclear extracts immunodepleted of TBP and major TAF II s. Single-round transcription assays reveal that TAF II -independent activation is manifested at the level of productive preinitiation complex formation and that TAF II s actually impair functional preinitiation complex assembly in a core promoter–specific manner. Furthermore, TAF II s appear to elevate absolute levels of transcription under multiple-round transcription conditions, presumably by facilitating secondary initiation events. Finally, human coactivator activities related to those in yeast RNA polymerase II/mediator complexes appear to function in unfractionated HeLa nuclear extracts.

Published

1998

6. Considerations of transcriptional control mechanisms: Do TFIID–core promoter complexes recapitulate nucleosome-like functions?

Author

Alexander Hoffmann, Thomas Oelgeschläger, and Robert G. Roeder

Subjects

Genetics, Multidisciplinary, Transcription, Genetic, TATA box, fungi, genetic processes, information science, Review, macromolecular substances, Computational biology, Biology, Nucleosomes, Transcription Factors, TFII, TAF1, TAF4, Transcription preinitiation complex, Transcription Factor TFIID, TAF2, health occupations, Animals, Humans, Transcription factor II D, Promoter Regions, Genetic, Transcription factor II A

Abstract

The general transcription initiation factor TFIID was originally identified, purified, and characterized with a biochemical assay in which accurate transcription initiation is reconstituted with multiple, chromatographically separable activities. Biochemical analyses have demonstrated that TFIID is a multiprotein complex that directs preinitiation complex assembly on both TATA box-containing and TATA-less promoters, and some TFIID subunits have been shown to be molecular targets for activation domains in DNA-binding regulatory proteins. These findings have most commonly been interpreted to support the view that transcriptional activation by upstream factors is the result of enhanced TFIID recruitment to the core promoter. Recent insights into the architecture and cell-cycle regulation of the multiprotein TFIID complex prompt both a reassessment of the functional role of TFIID in gene activation and a review of some of the less well-appreciated literature on TFIID. We present a speculative model for diverse functional roles of TFIID in the cell, explore the merits of the model in the context of published data, and suggest experimental approaches to resolve unanswered questions. Finally, we point out how the proposed functional roles of TFIID in eukaryotic class II transcription fit into a model for promoter recognition and activation that applies to both eubacteria and eukaryotes.

Published

1997

7. Specific Interactions and Potential Functions of Human TAFII100

Author

Masami Horikoshi, Yong Tao, Tohru Yamamoto, Satoshi Hasegawa, Ritsuko Takada, Thomas Oelgeschläger, Mohamed Guermah, Ernest Martinez, and Robert G. Roeder

Subjects

DNA, Complementary, Transcription, Genetic, Macromolecular Substances, TATA box, Protein subunit, Molecular Sequence Data, genetic processes, information science, macromolecular substances, Biology, Biochemistry, Transcription Factors, TFII, Humans, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Genetics, TATA-Binding Protein Associated Factors, General transcription factor, Cell Biology, Cell biology, DNA-Binding Proteins, TAF1, TAF4, TAF2, health occupations, Transcription Factor TFIID, Transcription factor II D, Peptides, Sequence Alignment, Transcription factor II A, HeLa Cells, Protein Binding, Transcription Factors

Abstract

Human transcription initiation factor TFIID contains the TATA-binding protein (TBP) and several TBP-associated factors (TAFs). To investigate the structural organization and function of TFIID, we have cloned and expressed a cDNA encoding the third largest human TFIID subunit, hTAFII100. Immunoprecipitation studies demonstrate that hTAFII100 is an integral subunit that is associated with all transcriptionally-competent forms of TFIID. They further suggest that at least part of the N-terminal region lies on the surface of TFIID, while a C-terminal region containing conserved WD-40 repeats appears inaccessible. Both in vivo and in vitro assays indicate that hTAFII100 interacts strongly with the histone H4-related hTAFII80 and the histone H3-related hTAFII31, as well as a stable complex comprised of both hTAFII80 and hTAFII31. Apparently weaker interactions of hTAFII100 with TBP, hTAFII250, hTAFII28, and hTAFII20, but not hTAFII55, also have been observed. These results suggest a role for hTAFII100 in stabilizing interactions of TAFs, especially the histone-like TAFs, in TFIID. In addition, functional studies show that anti-hTAFII100 antibodies selectively inhibit basal transcription from a TATA-less initiator-containing promoter, relative to a TATA-containing promoter, suggesting a possible core promoter-specific function for hTAFII100.

Published

1997

8. Topology and reorganization of a human TFIID–promoter complex

Author

Thomas Oelgeschläger, Robert G. Roeder, and Cheng Ming Chiang

Subjects

Photochemistry, Protein Conformation, TATA box, Molecular Sequence Data, genetic processes, information science, macromolecular substances, Biology, Crystallography, X-Ray, Topology, Humans, Promoter Regions, Genetic, Transcription factor, TATA-Binding Protein Associated Factors, Multidisciplinary, General transcription factor, fungi, DNA, TATA Box, TAF1, Transcription Factor TFIID, TAF2, health occupations, Nucleic Acid Conformation, RNA, Transcription factor II A, Protein Binding, Transcription Factors

Abstract

TRANSCRIPTION factor TFIID is a multiprotein complex composed of a TATA-box-binding subunit, TBP, and several tightly associated factors (TAFs) 1,2 . Human TFIID-promoter interactions are restricted to the TATA-box region on most core promoters 3,4 but extend over a large promoter region downstream of the TATA box and the transcription start site on the Ad2ML promoter 3-6 TFIID downstream interactions are thought to be functionally relevant because they can be induced by transcriptional activators 7-10 , which in some cases requires TFIIA 9,10 , result in stabilization of the TFIID-promoter complex 9,10 , and correlate with increased recruitment of the remaining general transcription factors 8,10 . Here we examine the topological organization of human TFIID complexes bound to the Ad2ML promoter. Our data provide insight into the relative disposition of DNA and several TFIID subunits, as well as evidence for DNA wrapping by TFIID, and suggest a direct role of TFIIA in the stable positioning of promoter DNA relative to TAFs.

Published

1996

9. Mutational Analysis of the Function of Gln115 in the EcoRI Restriction Endonuclease, a Critical Amino Acid for Recognition of the Inner Thymidine Residue in the Sequence -GAATTC- and for Coupling Specific DNA Binding to Catalysis

Author

Albert Jeltsch, Günter Maass, Thomas Oelgeschläger, Heiner Wolfes, Jürgen Alves, and Alfred Pingoud

Subjects

Models, Molecular, Stereochemistry, Glutamine, Molecular Sequence Data, EcoRI, Deoxyribonuclease EcoRI, chemistry.chemical_compound, Recognition sequence, Structural Biology, Denaturation (biochemistry), Site-directed mutagenesis, Molecular Biology, Protein secondary structure, chemistry.chemical_classification, Binding Sites, Base Sequence, biology, Amino acid, DNA-Binding Proteins, Models, Chemical, Biochemistry, chemistry, Mutagenesis, biology.protein, DNA, Thymidine, Methyl group

Abstract

The Gln115 residue of the Eco RI restriction endonuclease has been proposed to form a hydrophobic contact to the methyl group of the inner thymidine of the Eco RI recognition sequence -GAATTC- and to be involved in intramolecular hydrogen bonds to the main-chain at positions 140 and 143 as well as to the side-chain of Asn173. We have exchanged Gln115 for Ala and Glu by site-directed mutagenesis and analysed the purified mutant proteins (Q115A) biochemically and physico-chemically. Q115A and Q115E have the same secondary structure composition as wild-type Eco RI but are less stable towards thermal denaturation than the wild-type enzyme. In contrast to wild-type Eco RI the mutant proteins show a biphasic denaturation profile under alkaline pH, presumably because the amino acid exchange labilizes one part of the molecule, which unfolds before the rest of the protein is denatured. Q115A is catalytically inactive under normal buffer conditions, in part due to a diminished affinity towards DNA. At low ionic strength and alkaline pH, as well as in the presence of Mn 2+ , i.e. under conditions where wild-type Eco RI shows a relaxed specificity, Q115A is active, however not as much as wild-type Eco RI. Under these conditions it cleaves the canonical sequence -GAATTC- with the same k cat / K m values as the sequence -GAAUTC-, which differs from the former sequence by a single methyl group, while wild-type Eco Ri shows a tenfold lower k cat / K m for cleavage of -GAAUTC- than for -GAATTC-. Binding experiments, carried out in the absence of Mg 2+ , demonstrate that Q115A has a similar affinity towards -GAATTC-, as to -GAAUTC- while wild-type Eco RI binds to -GAATTC- with a tenfold preference over -GAAUTC-. On the basis of these thermodynamic and kinetic results it can be concluded that the hydrophobic contact between the γ-methylene group of Gln115 and the methyl group of the inner thymidine contributes about 3 kJ/mol (0·7 kcal/mol) to the energy of interaction, both in the ground and the transition state. Q115E is catalytically inactive under normal buffer conditions, but becomes active at low ionic strength or in the presence of Mn 2+ . Different from Q115A, Q115E is inactive at alkaline pH and its DNA binding affinity is highest at acidic pH. The dependence of its DNA cleavage activity on pH, which is governed by a p K a of 7·35, can be attributed to the protonation of the newly introduced glutamic acid residue, if it is assumed that the carboxyl group is located in a non-polar environment and/or involved in a hydrogen bond as the donor. Taken together, these results demonstrate that Gln115, as suggested on the basis of the revised Eco RI-DNA co-crystal structure, interacts with the inner thymidine of the Eco RI recognition sequence and has a structure stabilizing role. In addition, our results suggest that Gln115 is crucial for coupling specific DNA binding to catalysis under normal buffer conditions and we suggest that this coupling is achieved because direct and indirect involvement of Gln115 in base recognition induces local conformational alterations of the C-terminal region of β-strand β 3 , which contains Lys113 and Glu111 that are constituents of the catalytic centre of Eco RI. Activation of the catalytic centre, therefore, could be triggered by Gln115.

Published

1993

10. A site-directed mutagenesis study to identify amino acid residues involved in the catalytic function of the restriction endonuclease EcoRV

Author

Michaela Liedtke, V Thielking, Rüter T, E Köhler, Jürgen Alves, Alfred Pingoud, F Peters, Heiner Wolfes, Thomas Oelgeschläger, and U Selent

Subjects

DNA, Bacterial, Proline, Molecular Sequence Data, EcoRI, HindIII, Biochemistry, Catalysis, Structure-Activity Relationship, Amino Acid Sequence, Amino Acids, Deoxyribonucleases, Type II Site-Specific, Site-directed mutagenesis, Aspartic Acid, Binding Sites, Base Sequence, biology, Hydrolysis, Lysine, EcoRV, Restriction enzyme, Directed mutagenesis, Phosphodiester bond, Mutagenesis, Site-Directed, biology.protein, Sequence motif

Abstract

We have used site-directed mutagenesis of the EcoRV restriction endonuclease to change amino acid side chains that have been shown crystallographically to be in close proximity to the scissile phosphodiester bond of the DNA substrate. DNA cleavage assays of the resulting mutant proteins indicate that the largest effects on nucleolytic activity result from substitution of Asp74, Asp90, and Lys92. We suggest on the basis of structural information, mutagenesis data, and analogies with other nucleases that Asp74 and Asp90 might be involved in Mg2+ binding and/or catalysis and that Lys92 probably stabilizes the pentacovalent phosphorus in the transition state. These amino acids are part of a sequence motif, Pro-Asp...Asp/Glu-X-Lys, which is also present in EcoRI. In both enzymes, it is located in a structurally similar context near the scissile phosphodiester bond. A preliminary mutational analysis with EcoRI indicates that this sequence motif is of similar functional importance for EcoRI and EcoRV. On the basis of these results, a proposal is made for the mechanism of DNA cleavage by EcoRV and EcoRI.

Published

1992

11. TFIIB recognition elements control the TFIIA-NC2 axis in transcriptional regulation

Author

Barbora Malecova, Thomas Oelgeschläger, Wensheng Deng, and Stefan G. E. Roberts

Subjects

Genetics, Transcription, Genetic, TATA box, Response element, Promoter, Cell Biology, Articles, Biology, Phosphoproteins, Cell Line, QR, Transcription Factor TFIIA, Transcription preinitiation complex, Transcriptional regulation, Transcription Factor TFIIB, Humans, Promoter Regions, Genetic, Molecular Biology, Transcription factor, Transcription factor II B, Transcription factor II A, Transcription Factors

Abstract

TFIIB recognizes DNA sequence-specific motifs that can flank the TATA elements of the promoters of protein-encoding genes. The TFIIB recognition elements (BRE(u) and BRE(d)) can have positive or negative effects on transcription in a promoter context-dependent manner. Here we show that the BREs direct the selective recruitment of TFIIA and NC2 to the promoter. We find that TFIIA preferentially associates with BRE-containing promoters while NC2 is recruited to promoters that lack consensus BREs. The functional relevance of the BRE-dependent recruitment of TFIIA and NC2 was determined by small interfering RNA-mediated knockdown of TFIIA and NC2, both of which elicited BRE-dependent effects on transcription. Our results confirm the established functional reciprocity of TFIIA and NC2. However, our findings show that TFIIA assembly at BRE-containing promoters results in reduced transcriptional activity, while NC2 acts as a positive factor at promoters that lack functional BREs. Taken together, our results provide a basis for the selective recruitment of TFIIA and NC2 to the promoter and give new insights into the functional relationship between core promoter elements and general transcription factor activity.

Published

2009

12. The initiator core promoter element antagonizes repression of TATA-directed transcription by negative cofactor NC2

Author

Sevil Yavuz, Barbora Malecova, Michaël Boyer-Guittaut, Thomas Oelgeschläger, Petra Gross, Estrogènes, Expression génique et pathologies du Système Nerveux Central - UFC (E2SNC / ESTROGENES), Université de Franche-Comté (UFC), and Université Bourgogne Franche-Comté [COMUE] (UBFC)-Université Bourgogne Franche-Comté [COMUE] (UBFC)

Subjects

MESH: Cell Nucleus, Transcription, Genetic, TATA box, Response element, MESH: TATA Box, Biology, Models, Biological, Biochemistry, MESH: Phosphoproteins, MESH: HIV-1, 03 medical and health sciences, Initiator element, MESH: Promoter Regions, Genetic, Humans, MESH: Protein Binding, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, MESH: Models, Genetic, Promoter Regions, Genetic, Molecular Biology, 030304 developmental biology, Cell Nucleus, Genetics, 0303 health sciences, MESH: Humans, Models, Genetic, MESH: Transcription Factor TFIIA, MESH: Transcription Factor TFIIB, MESH: Transcription, Genetic, 030302 biochemistry & molecular biology, fungi, MESH: Models, Biological, Promoter, Cell Biology, MESH: Transcription Factors, Phosphoproteins, TATA Box, MESH: Hela Cells, Transcription Factor TFIIA, Transcription preinitiation complex, HIV-1, Transcription Factor TFIIB, Transcription factor II D, Transcription factor II B, Transcription factor II A, HeLa Cells, Protein Binding, Transcription Factors

Abstract

International audience; Core promoter regions of protein-coding genes in metazoan genomes are structurally highly diverse and can contain several distinct core promoter elements, which direct accurate transcription initiation and determine basal promoter strength. Diversity in core promoter structure is an important aspect of transcription regulation in metazoans as it provides a basis for gene-selective function of activators and repressors. The basal activity of TATA box-containing promoters is dramatically enhanced by the initiator element (INR), which can function in concert with the TATA box in a synergistic manner. Here we report that a functional INR provides resistance to NC2 (Dr1/DRAP1), a general repressor of TATA promoters. INR-mediated resistance to NC2 is established during transcription initiation complex assembly and requires TBP-associated factors (TAFs) and TAF- and INR-dependent cofactor activity. Remarkably, the INR appears to stimulate TATA-dependent transcription similar to activators by strongly enhancing recruitment of TFIIA and TFIIB and, at the same time, by compromising NC2 binding.

Published

2007

13. Sumoylation delays the ATF7 transcription factor subcellular localization and inhibits its transcriptional activity

Author

Bruno Chatton, Pierre-Jacques Hamard, Thomas Oelgeschläger, Barbara Camuzeaux, Charlotte Hauss, Marc Vigneron, Michaël Boyer-Guittaut, Claude Kedinger, Denis Dujardin, Institut Gilbert-Laustriat : Biomolécules, Biotechnologie, Innovation Thérapeutique, and Université Louis Pasteur - Strasbourg I-Centre National de la Recherche Scientifique (CNRS)

Subjects

MESH: Cell Nucleus, Protein sumoylation, Ubiquitin-Protein Ligases, SUMO-1 Protein, SUMO protein, Biology, Cell Line, Genetics, Transcriptional regulation, Humans, Transcription factor, Molecular Biology, Cell Nucleus, MESH: Humans, General transcription factor, MESH: SUMO-1 Protein, [SDV.BBM.BM]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Molecular biology, Promoter, Sciences du Vivant [q-bio]/Biotechnologies, MESH: Ubiquitin-Protein Ligases, Molecular biology, Activating Transcription Factors, MESH: Cell Line, Cell biology, Nuclear Pore Complex Proteins, MESH: Activating Transcription Factors, MESH: Protein Processing, Post-Translational, RANBP2, MESH: Molecular Chaperones, Transcription factor II D, Protein Processing, Post-Translational, MESH: Nuclear Pore Complex Proteins, Molecular Chaperones

Abstract

Over the past few years, small ubiquitin-like modifier (SUMO) modification has emerged as an important regulator of diverse pathways and activities including protein localization and transcriptional regulation. We identified a consensus sumoylation motif (IKEE), located within the N-terminal activation domain of the ATF7 transcription factor and thus investigated the role of this modification. ATF7 is a ubiquitously expressed transcription factor, homologous to ATF2, that binds to CRE elements within specific promoters. This protein is able to heterodimerize with Jun or Fos proteins and its transcriptional activity is mediated by interaction with TAF12, a subunit of the general transcription factor TFIID. In the present article, we demonstrate that ATF7 is sumoylated in vitro (using RanBP2 as a E3-specific ligase) and in vivo. Moreover, we show that ATF7 sumoylation affects its intranuclear localization by delaying its entry into the nucleus. Furthermore, SUMO conjugation inhibits ATF7 transactivation activity by (i) impairing its association with TAF12 and (ii) blocking its binding-to-specific sequences within target promoters.

Published

2007

14. Core promoter-selective RNA polymerase II transcription

Author

Petra Gross and Thomas Oelgeschläger

Subjects

Genetics, Genome, RNA, Transfer, Met, Transcription, Genetic, Macromolecular Substances, TATA box, Response element, Promoter, RNA polymerase II, Biology, Biochemistry, TATA Box, Cell biology, biology.protein, Animals, Transcription factor II F, Transcription factor II E, RNA Polymerase II, Transcription factor II D, Promoter Regions, Genetic, RNA polymerase II holoenzyme

Abstract

The initiation of mRNA synthesis in eukaryotic cells is a complex and highly regulated process that requires the assembly of general transcription factors and RNAP II (RNA polymerase II; also abbreviated as Pol II) into a pre-initiation complex at the core promoter. The core promoter is defined as the minimal DNA region that is sufficient to direct low levels of activator-independent (basal) transcription by RNAP II in vitro. The core promoter typically extends approx. 40 bp up- and down-stream of the start site of transcription and can contain several distinct core promoter sequence elements. Core promoters in higher eukaryotes are highly diverse in structure, and each core promoter sequence element is only found in a subset of genes. So far, only TATA box and INR (initiator) element have been shown to be capable of directing accurate RNAP II transcription initiation independent of other core promoter elements. Computational analysis of metazoan genomes suggests that the prevalence of the TATA box has been overestimated in the past and that the majority of human genes are TATA-less. While TATA-mediated transcription initiation has been studied in great detail and is very well understood, very little is known about the factors and mechanisms involved in the function of the INR and other core promoter elements. Here we summarize our current understanding of the factors and mechanisms involved in core promoter-selective transcription and discuss possible pathways through which diversity in core promoter architecture might contribute to combinatorial gene regulation in metazoan cells.

Published

2006

15. Nuclear export determines the cytokine sensitivity of STAT transcription factors

Author

Andreas Marg, Uwe Vinkemeier, Burkhard Wiesner, Barbora Malecova, Inga Lödige, and Thomas Oelgeschläger

Subjects

Transcriptional Activation, Cytoplasm, Time Factors, Transcription, Genetic, Blotting, Western, Green Fluorescent Proteins, Active Transport, Cell Nucleus, SH2 domain, Biochemistry, Models, Biological, stat, src Homology Domains, Transactivation, chemistry.chemical_compound, Genes, Reporter, Serine, Humans, Protein inhibitor of activated STAT, STAT1, Phosphorylation, Nuclear export signal, Molecular Biology, STAT4, Transcription factor, STAT6, Glutathione Transferase, Cell Nucleus, Microscopy, Confocal, Dose-Response Relationship, Drug, biology, Chemistry, Tyrosine phosphorylation, Cell Biology, Molecular biology, Recombinant Proteins, Protein Structure, Tertiary, Cell biology, Alternative Splicing, STAT Transcription Factors, STAT1 Transcription Factor, biology.protein, Cytokines, Tyrosine, Peptides, Dimerization, HeLa Cells, Plasmids

Abstract

Cytokine-dependent gene activation critically depends upon the tyrosine phosphorylation (activation) of STAT transcription factors at membrane-bound cytokine receptors. The extent of STAT activation and hence the specificity of signaling is primarily determined by structural complementarity between the SH2 domain of the STATs and the tyrosine-phosphorylated receptor chains. Here, we identified constitutive nucleocytoplasmic shuttling as another mechanism that controls the differential activation of STAT transcription factors. Our analysis of nucleocytoplasmic cycling of STAT1 revealed that the expression of the alternatively spliced transactivation domain and its signal-dependent serine phosphorylation maximized the rate of nuclear export. Export modulation occurred independently of retention factors or the export receptor CRM1, and was observed both before and during stimulation of cells with cytokines. Our data indicated a dual role for the transactivation domain. It enhanced the nuclear retention of activated STAT1, but had the opposite effect on inactivated molecules. Accordingly, and despite their identical receptor recognition, the STAT1 splice variants differed strongly in the amplitude of tyrosine phosphorylation and in the duration of the cytokine signal. Thus, regulated nuclear export determined the cytokine sensitivity of the shuttling STAT1 transcription factors by controlling their availability at the receptor kinase complex.

Published

2005

16. SUMO-1 modification of human transcription factor (TF) IID complex subunits: inhibition of TFIID promoter-binding activity through SUMO-1 modification of hsTAF5

Author

Michaël, Boyer-Guittaut, Kivanç, Birsoy, Corinne, Potel, Gill, Elliott, Ellis, Jaffray, Joanna M, Desterro, Ron T, Hay, and Thomas, Oelgeschläger

Subjects

TATA-Binding Protein Associated Factors, Binding Sites, Models, Genetic, Sequence Homology, Amino Acid, Transcription, Genetic, Protein Conformation, Lysine, Immunoblotting, Molecular Sequence Data, SUMO-1 Protein, DNA, Transfection, Models, Biological, Recombinant Proteins, Protein Structure, Tertiary, Epitopes, Catalytic Domain, Humans, Electrophoresis, Polyacrylamide Gel, Transcription Factor TFIID, Amino Acid Sequence, RNA Polymerase II, Promoter Regions, Genetic, HeLa Cells, Protein Binding

Abstract

The TFIID complex is composed of the TATA-binding protein (TBP) and TBP-associated factors (TAFs) and is the only component of the general RNA polymerase II (RNAP II) transcription machinery with intrinsic sequence-specific DNA-binding activity. Binding of transcription factor (TF) IID to the core promoter region of protein-coding genes is a key event in RNAP II transcription activation and is the first and rate-limiting step of transcription initiation complex assembly. Intense research efforts in the past have established that TFIID promoter-binding activity as well as the function of TFIID-promoter complexes is tightly regulated through dynamic TFIID interactions with positive- and negative-acting transcription regulatory proteins. However, very little is known about the role of post-translational modifications in the regulation of TFIID. Here we show that the human TFIID subunits hsTAF5 and hsTAF12 are modified by the small ubiquitin-related modifier SUMO-1 in vitro and in human cells. We identify Lys-14 in hsTAF5 and Lys-19 in hsTAF12 as the primary SUMO-1 acceptor sites and show that SUMO conjugation has no detectable effect on nuclear import or intranuclear distribution of hsTAF5 and hsTAF12. Finally, we demonstrate that purified human TFIID complex can be SUMO-1-modified in vitro at both hsTAF5 and hsTAF12. We find that SUMO-1 conjugation at hsTAF5 interferes with binding of TFIID to promoter DNA, whereas modification of hsTAF12 has no detectable effect on TFIID promoter-binding activity. Our observations suggest that reversible SUMO modification at hsTAF5 contributes to the dynamic regulation of TFIID promoter-binding activity in human cells.

Published

2005

17. Regulation of RNA polymerase II activity by CTD phosphorylation and cell cycle control

Author

Thomas, Oelgeschläger

Subjects

Transcription, Genetic, Cell Cycle, Animals, Humans, RNA Polymerase II, Phosphorylation, Protein Kinases, Cyclin-Dependent Kinases, Protein Structure, Tertiary

Abstract

The carboxyl-terminal domain (CTD) of the largest subunit of mammalian RNA polymerase II (RNAP II) consists of 52 repeats of a consensus heptapeptide and is subject to phosphorylation and dephosphorylation events during each round of transcription. RNAP II activity is regulated during the cell cycle and cell cycle-dependend changes in RNAP II activity correlate well with CTD phosphorylation. In addition, global changes in the CTD phosphorylation status are observed in response to mitogenic or cytostatic signals such as growth factors, mitogens and DNA-damaging agents. Several CTD kinases are members of the cyclin-dependent kinase (CDK) superfamily and associate with transcription initiation complexes. Other CTD kinases implicated in cell cycle regulation include the mitogen-activated protein kinases ERK-1/2 and the c-Abl tyrosine kinase. These observations suggest that reversible RNAP II CTD phosphorylation may play a key role in linking cell cycle regulatory events to coordinated changes in transcription.

Published

2002

18. Association of human TFIID-promoter complexes with silenced mitotic chromatin in vivo

Author

Thomas Oelgeschläger and Rossitza Christova

Subjects

Mitosis, RNA polymerase II, Promoter, Cell Biology, Biology, Phosphoproteins, Molecular biology, Chromatin, Cell biology, Transcription Factors, TFII, Transcription Factor TFIID, biology.protein, Transcription Factor TFIIB, Humans, Gene Silencing, RNA Polymerase II, Transcription factor II D, Promoter Regions, Genetic, Transcription factor II B, RNA polymerase II holoenzyme, HeLa Cells, Transcription Factors

Abstract

When eukaryotic cells enter mitosis, transcription is abruptly silenced. Earlier studies indicated that most transcription factors and RNA polymerase II (RNAP II) are displaced when chromatin is condensed into mitotic chromosomes. A more recent study suggested that hitherto unidentified factors might 'bookmark' previously active genes for rapid reactivation after cell division. Here we used chromatin immunoprecipitation (ChIP) assays to examine the association of TFIID, TFIIB, NC2 and RNAP II with various gene promoters in asynchronous and mitotic human cell populations. We show that TFIID and TFIIB can remain associated with active gene promoters during mitosis whereas RNA polymerase II is displaced, and also that NC2, originally identified as ubiquitous repressor of transcription, is associated with active gene promoters in asynchronous cell populations and is displaced from some, but not all, genes in mitotic cells. Consistent with the remarkable stability of TFIID-promoter complexes observed in vitro, our data suggest that these complexes can withstand condensation of chromatin into transcriptionally silent chromosomes. Stable TFIID-promoter complexes are therefore implicated in the propagation of cell-type-specific gene expression patterns through cell division.

Published

2001

19. The C-terminal domain-phosphorylated IIO form of RNA polymerase II is associated with the transcription repressor NC2 (Dr1/DRAP1) and is required for transcription activation in human nuclear extracts

Author

Enrique Castaño, Thomas Oelgeschläger, Robert G. Roeder, Petra Gross, and Zhengxin Wang

Subjects

Transcriptional Activation, genetic processes, RNA polymerase II, chemistry.chemical_compound, RNA polymerase, Animals, Humans, Phosphorylation, RNA polymerase II holoenzyme, Cell Nucleus, Multidisciplinary, biology, General transcription factor, Histocompatibility Antigens Class II, Biological Sciences, Phosphoproteins, Molecular biology, TATA Box, Rats, enzymes and coenzymes (carbohydrates), chemistry, biology.protein, health occupations, bacteria, Transcription factor II F, Transcription factor II E, RNA Polymerase II, Transcription factor II D, Transcription factor II B, Transcription Factors

Abstract

Activation of class II gene transcription may involve alleviation of transcription repression as well as stimulation of the assembly and function of the general RNA polymerase (RNAP) II transcription machinery. Here, we investigated whether activator-reversible transcription repression by NC2 (Dr1/DRAP1) contributes to maximum induction levels in unfractionated HeLa nuclear extracts. Surprisingly, we found that depletion of NC2 does not significantly affect basal transcription, but dramatically reduces activated transcription. Immunoblot analyses revealed that the loss of activator function coincides with selective removal of the C-terminal domain (CTD)-hyperphosphorylated RNAP IIO along with NC2. Coimmunoprecipitation experiments with purified factors confirmed that NC2 interacts with RNAP IIO, but not with the unphosphorylated or hypophosphorylated RNAP IIA or CTD-less RNAP IIB forms. Finally, we demonstrate that, in contrast to previously published observations in cell-free systems reconstituted with purified factors, only the CTD-phosphorylated form of RNAP II can mediate activator function in the context of unfractionated HeLa nuclear extracts. These findings reveal an unexpected link between NC2 and transcription activation and suggest that regulation of RNAP II transcription through reversible CTD phosphorylation might be more complex than previously proposed.

Published

2000

20. Downstream promoter sequences facilitate the formation of a specific transcription factor IID-promoter complex topology required for efficient transcription from the megalin/low density lipoprotein receptor-related protein 2 promoter

Author

Robert G. Roeder, Gunnar Westin, Anders Knutson, Thomas Oelgeschläger, and Enrique Castaño

Subjects

Membrane Glycoproteins, Base Sequence, Transcription, Genetic, TATA box, Response element, CAAT box, DNA Footprinting, Heymann Nephritis Antigenic Complex, Molecular Conformation, Promoter, Cell Biology, DNA, Biology, Topology, Biochemistry, Molecular biology, TAF1, Transcription Factors, TFII, TAF2, Humans, Transcription Factor TFIID, Transcription factor II D, Promoter Regions, Genetic, Molecular Biology, Transcription factor II A

Abstract

Megalin/low density lipoprotein receptor-related protein 2 (LRP-2) is an endocytic receptor expressed in highly specialized cell types such as parathyroid cells and epithelia of the kidney. Previous experiments identified a nonconsensus TATA element, with the sequence TAGAAAA, as crucial for accurate and efficient transcription from the LRP-2 promoter. Here we show that, in addition to the TAGA element, promoter sequences downstream of the transcription start site contribute significantly to transcription both in vitro and in transfected cells. Deletion and point mutational analyses reveal that the promoter region located between positions +5 and +11 (sequence TTTTGGC) is of particular importance. Complementation experiments in nuclear extracts lacking transcription factor IID (TFIID) activity show that TATA-binding protein-associated factors of TFIID are essential for the function of LRP-2 downstream promoter sequences. Interestingly, DNase I footprinting studies show that the downstream region between positions +5 and +11 does not significantly affect overall TFIID affinity to the promoter but that it profoundly affects the topology of the TFIID x promoter complex not only downstream of the transcription start site, but in particular in the TATA box region. Our observations suggest a model for a novel downstream sequence function, in which TATA-binding protein-associated factor-promoter interactions downstream of the transcription start site modulate TFIID-DNA interactions in the TATA box region.

Published

2000

21. Core promoter-specific function of a mutant transcription factor TFIID defective in TATA-box binding

Author

Qiang Zhou, Thomas Oelgeschläger, Robert G. Roeder, Noelle D. L'Etoile, Ernest Martinez, and Arnold J. Berk

Subjects

Transcription, Genetic, TATA box, genetic processes, Molecular Sequence Data, information science, Arabidopsis, macromolecular substances, Biology, Initiator element, Transcription Factor TFIIIB, Humans, Amino Acid Sequence, Promoter Regions, Genetic, Multidisciplinary, Binding Sites, Models, Genetic, TATA-Box Binding Protein, fungi, RNA Polymerase III, DNA-Directed RNA Polymerases, Molecular biology, TATA Box, Cell biology, DNA-Binding Proteins, TAF1, Transcription Factor TFIID, TAF2, Mutation, health occupations, RNA Polymerase II, Transcription factor II D, Transcription factor II A, Research Article, HeLa Cells, Protein Binding, Transcription Factors

Abstract

In conjunction with other general initiation factors, the TATA box-binding protein (TBP) can direct basal transcription by RNA polymerase II from TATA-containing promoters, but its stable interaction with TBP-associated factors (TAFs) in the TFIID complex is required both for activator-dependent transcription and for basal transcription directed by an initiator element. We have generated a TATA-binding-defective TFIID complex containing an amino acid substitution in the DNA-binding surface of its TBP subunit. This mutated TFIID is defective in both basal and activated transcription from core promoters containing only a TATA box but supports transcription from initiator-containing promoters independently of the presence or absence of a TATA sequence. Our results show that a functional initiator element is needed to bypass the requirement for an active TATA DNA-binding surface in TFIID and imply that gene-specific transcription can be achieved by modulating distinct core promoter-specific TFIID functions--e.g., TBP-TATA versus TAF-initiator interactions.

Published

1995

22. Probing the function of individual amino acid residues in the DNA binding site of the EcoRI restriction endonuclease by analysing the toxicity of genetically engineered mutants

Author

Jürgen Alves, Alfred Pingoud, Thomas Oelgeschläger, Thomas Rüter, Geiger R, and Anja Fliess

Subjects

Models, Molecular, Site-Specific DNA-Methyltransferase (Adenine-Specific), Protein Conformation, Mutant, Genetic Vectors, Molecular Sequence Data, EcoRI, Biology, medicine.disease_cause, Deoxyribonuclease EcoRI, Substrate Specificity, Genetics, medicine, Escherichia coli, Amino Acid Sequence, Binding site, Site-directed mutagenesis, Binding Sites, Wild type, General Medicine, Molecular biology, Bacteriophage lambda, DNA binding site, Restriction enzyme, Biochemistry, DNA, Viral, Mutation, biology.protein, Plasmids

Abstract

We have developed an assay that allows analysis of the activity of EcoRI restriction endonuclease (ENase) and its mutants in vivo. This assay is based on the fact that wild type (wt) EcoRI ENase is toxic for Escherichia coli cells not expressing the EcoRI methyltransferase (MTase). The viability factor defined by the ratio of the viable counts of E. coli cultures having or not having expressed the ecoRIR gene for a defined time is 10−6 for wt EcoRI ENase and close to one for a totally inactive EcoRI ENase mutant. While the EcoRI MTase (M·EcoRI) provides substantial protection against the toxic effects of the wt EcoRI ENase and several of the mutants, some mutants become more toxic in the presence of M·EcoRI. Twenty-four different DNA-binding-site mutants of EcoRI ENase were characterized in their activity in vivo with this assay. The results obtained allow us to conclude that the structural integrity of the region at and around aa 200 seems to be very critical for the enzymatic function of EcoRI ENase: nonconservative replacements theare lead to viability factors of 1–10−2. While our results indicate that the region around aa 144 and 145 is also involved in the EcoRI ENase-catalyzed reaction, it is also evident that the effects of mutation there are not as large: viability factors of approx. 10−3 are obtained even for drastic replacements. These results are discussed in the light of the x-ray structure analysis of an EcoRI ENase-DNA recognition complex.

Published

1990