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1. Building a global alliance of biofoundries (vol 10, 2040, 2019)

Author

Hillson, N, Caddick, M, Cai, Y, Carrasco, JA, Chang, MW, Curach, NC, Bell, DJ, Le Feuvre, R, Friedman, DC, Fu, X, Gold, ND, Herrgard, MJ, Holowko, MB, Johnson, JR, Johnson, RA, Keasling, JD, Kitney, RI, Kondo, A, Liu, C, Martin, VJJ, Menolascina, F, Ogino, C, Patron, NJ, Pavan, M, Poh, CL, Pretorius, IS, Rosser, SJ, Scrutton, NS, Storch, M, Tekotte, H, Travnik, E, Vickers, CE, Yew, WS, Yuan, Y, Zhao, H, and Freemont, PS

Subjects
Multidisciplinary Sciences, Science & Technology, MD Multidisciplinary, Science & Technology - Other Topics
Published
2019

2. MafB represses erythroid genes and differentiation through direct interaction with c-Ets-1

Author

Mh, Sieweke, Tekotte H, Frampton J, and Thomas Graf

Subjects
Oncogene Proteins, Transcriptional Activation, Leucine Zippers, Erythrocytes, Erythroblasts, Proto-Oncogene Proteins c-ets, Cell Differentiation, Heme, Saccharomyces cerevisiae, Hematopoietic Stem Cells, Transfection, Recombinant Proteins, Avian Proteins, DNA-Binding Proteins, Proto-Oncogene Protein c-ets-1, Repressor Proteins, Proto-Oncogene Proteins, Receptors, Transferrin, Trans-Activators, Animals, Erythropoiesis, Transcription Factors
Abstract

Using a yeast interaction screen with a DNA-bound Ets-1 protein we have identified MafB as a direct interaction partner. This distant AP-1 relative, which is specifically expressed in myelomonocytic cells, binds to the DNA binding domain of Ets-1 via its basic region/leucine zipper domain. MafB represses Ets-1 transactivation of synthetic promoters containing Ets binding sites in yeast as well as avian cells. Both Ets-1 and Maf family proteins have been implicated in erythroid specific gene expression. Here we show that MafB inhibits Ets-1-mediated transactivation of the transferrin receptor, which is essential for heme synthesis and erythroid differentiation. Consequently, overexpression of MafB in an erythroblast cell line down-regulates the endogenous transferrin receptor gene and inhibits the cells' potential to differentiate into erythrocytes, without affecting cellular proliferation.

Published
1997

12. The S. cerevisiae SET3 complex includes two histone deacetylases, Hos2 and Hst1, and is a meiotic-specific repressor of the sporulation gene program.

Author

Pijnappel, W W, Schaft, D, Roguev, A, Shevchenko, A, Tekotte, H, Wilm, M, Rigaut, G, Séraphin, B, Aasland, R, and Stewart, A F

Abstract

Set3 is one of two proteins in the yeast Saccharomyces cerevisiae that, like Drosophila Trithorax, contains both SET and PHD domains. We found that Set3 forms a single complex, Set3C, with Snt1, YIL112w, Sif2, Cpr1, and two putative histone deacetylases, Hos2 and NAD-dependent Hst1. Set3C includes NAD-dependent and independent deacetylase activities when assayed in vitro. Homology searches suggest that Set3C is the yeast analog of the mammalian HDAC3/SMRT complex. Set3C represses genes in early/middle of the yeast sporulation program, including the key meiotic regulators ime2 and ndt80. Whereas Hos2 is only found in Set3C, Hst1 is also present in a complex with Sum1, supporting previous characterizations of Hst1 and Sum1 as repressors of middle sporulation genes during vegetative growth. However, Hst1 is not required for meiotic repression by Set3C, thus implying that Set3C (-Hst1) and not Hst1-Sum1, is the meiotic-specific repressor of early/middle sporulation genes.

Published
2001
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13. Technological challenges and milestones for writing genomes.

Author

Ostrov N, Beal J, Ellis T, Gordon DB, Karas BJ, Lee HH, Lenaghan SC, Schloss JA, Stracquadanio G, Trefzer A, Bader JS, Church GM, Coelho CM, Efcavitch JW, Güell M, Mitchell LA, Nielsen AAK, Peck B, Smith AC, Stewart CN Jr, and Tekotte H

Subjects
Chromosomes, Computer-Aided Design, DNA chemical synthesis, Gene Editing, Genes, Synthetic, Interdisciplinary Research, Genetic Engineering, Genome, Synthetic Biology instrumentation, Synthetic Biology methods
Published
2019
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14. Author Correction: Building a global alliance of biofoundries.

Author

Hillson N, Caddick M, Cai Y, Carrasco JA, Chang MW, Curach NC, Bell DJ, Feuvre RL, Friedman DC, Fu X, Gold ND, Herrgård MJ, Holowko MB, Johnson JR, Johnson RA, Keasling JD, Kitney RI, Kondo A, Liu C, Martin VJJ, Menolascina F, Ogino C, Patron NJ, Pavan M, Poh CL, Pretorius IS, Rosser SJ, Scrutton NS, Storch M, Tekotte H, Travnik E, Vickers CE, Yew WS, Yuan Y, Zhao H, and Freemont PS

Abstract

The original version of this Comment contained errors in the legend of Figure 2, in which the locations of the fifteenth and sixteenth GBA members were incorrectly given as '(15) Australian Genome Foundry, Macquarie University; (16) Australian Foundry for Advanced Biomanufacturing, University of Queensland.'. The correct version replaces this with '(15) Australian Foundry for Advanced Biomanufacturing (AusFAB), University of Queensland and (16) Australian Genome Foundry, Macquarie University'. This has been corrected in both the PDF and HTML versions of the Comment.

Published
2019
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15. Building a global alliance of biofoundries.

Author

Hillson N, Caddick M, Cai Y, Carrasco JA, Chang MW, Curach NC, Bell DJ, Le Feuvre R, Friedman DC, Fu X, Gold ND, Herrgård MJ, Holowko MB, Johnson JR, Johnson RA, Keasling JD, Kitney RI, Kondo A, Liu C, Martin VJJ, Menolascina F, Ogino C, Patron NJ, Pavan M, Poh CL, Pretorius IS, Rosser SJ, Scrutton NS, Storch M, Tekotte H, Travnik E, Vickers CE, Yew WS, Yuan Y, Zhao H, and Freemont PS

Subjects
Biomedical Research methods, Biotechnology instrumentation, Genetic Engineering, International Cooperation, Organisms, Genetically Modified
Published
2019
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16. Leaf LIMS: A Flexible Laboratory Information Management System with a Synthetic Biology Focus.

Author

Craig T, Holland R, D'Amore R, Johnson JR, McCue HV, West A, Zulkower V, Tekotte H, Cai Y, Swan D, Davey RP, Hertz-Fowler C, Hall A, and Caddick M

Subjects
Database Management Systems, Databases, Factual, Synthetic Biology instrumentation, Synthetic Biology methods
Abstract

This paper presents Leaf LIMS, a flexible laboratory information management system (LIMS) designed to address the complexity of synthetic biology workflows. At the project's inception there was a lack of a LIMS designed specifically to address synthetic biology processes, with most systems focused on either next generation sequencing or biobanks and clinical sample handling. Leaf LIMS implements integrated project, item, and laboratory stock tracking, offering complete sample and construct genealogy, materials and lot tracking, and modular assay data capture. Hence, it enables highly configurable task-based workflows and supports data capture from project inception to completion. As such, in addition to it supporting synthetic biology it is ideal for many laboratory environments with multiple projects and users. The system is deployed as a web application through Docker and is provided under a permissive MIT license. It is freely available for download at https://leaflims.github.io .

Published
2017
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17. Genetic Constructor: An Online DNA Design Platform.

Author

Bates M, Lachoff J, Meech D, Zulkower V, Moisy A, Luo Y, Tekotte H, Franziska Scheitz CJ, Khilari R, Mazzoldi F, Chandran D, and Groban E

Subjects
DNA genetics, Genetic Engineering instrumentation, Software
Abstract

Genetic Constructor is a cloud Computer Aided Design (CAD) application developed to support synthetic biologists from design intent through DNA fabrication and experiment iteration. The platform allows users to design, manage, and navigate complex DNA constructs and libraries, using a new visual language that focuses on functional parts abstracted from sequence. Features like combinatorial libraries and automated primer design allow the user to separate design from construction by focusing on functional intent, and design constraints aid iterative refinement of designs. A plugin architecture enables contributions from scientists and coders to leverage existing powerful software and connect to DNA foundries. The software is easily accessible and platform agnostic, free for academics, and available in an open-source community edition. Genetic Constructor seeks to democratize DNA design, manufacture, and access to tools and services from the synthetic biology community.

Published
2017
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18. A loss of function analysis of host factors influencing Vaccinia virus replication by RNA interference.

Author

Beard PM, Griffiths SJ, Gonzalez O, Haga IR, Pechenick Jowers T, Reynolds DK, Wildenhain J, Tekotte H, Auer M, Tyers M, Ghazal P, Zimmer R, and Haas J

Subjects
Gene Expression Regulation, Gene Knockdown Techniques, High-Throughput Screening Assays, Humans, Reproducibility of Results, Signal Transduction, Transcription, Genetic, Vaccinia metabolism, Host-Pathogen Interactions genetics, RNA Interference, RNA, Small Interfering genetics, Vaccinia genetics, Vaccinia virology, Vaccinia virus physiology, Virus Replication
Abstract

Vaccinia virus (VACV) is a large, cytoplasmic, double-stranded DNA virus that requires complex interactions with host proteins in order to replicate. To explore these interactions a functional high throughput small interfering RNA (siRNA) screen targeting 6719 druggable cellular genes was undertaken to identify host factors (HF) influencing the replication and spread of an eGFP-tagged VACV. The experimental design incorporated a low multiplicity of infection, thereby enhancing detection of cellular proteins involved in cell-to-cell spread of VACV. The screen revealed 153 pro- and 149 anti-viral HFs that strongly influenced VACV replication. These HFs were investigated further by comparisons with transcriptional profiling data sets and HFs identified in RNAi screens of other viruses. In addition, functional and pathway analysis of the entire screen was carried out to highlight cellular mechanisms involved in VACV replication. This revealed, as anticipated, that many pro-viral HFs are involved in translation of mRNA and, unexpectedly, suggested that a range of proteins involved in cellular transcriptional processes and several DNA repair pathways possess anti-viral activity. Multiple components of the AMPK complex were found to act as pro-viral HFs, while several septins, a group of highly conserved GTP binding proteins with a role in sequestering intracellular bacteria, were identified as strong anti-viral VACV HFs. This screen has identified novel and previously unexplored roles for cellular factors in poxvirus replication. This advancement in our understanding of the VACV life cycle provides a reliable knowledge base for the improvement of poxvirus-based vaccine vectors and development of anti-viral theraputics.

Published
2014
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19. Ablation of the regulatory IE1 protein of murine cytomegalovirus alters in vivo pro-inflammatory TNF-alpha production during acute infection.

Author

Rodríguez-Martín S, Kropp KA, Wilhelmi V, Lisnic VJ, Hsieh WY, Blanc M, Livingston A, Busche A, Tekotte H, Messerle M, Auer M, Fraser I, Jonjic S, Angulo A, Reddehase MJ, and Ghazal P

Subjects
Animals, Cell Line, Cytokines metabolism, DNA Replication, DNA, Viral genetics, Female, Herpesviridae Infections virology, Immediate-Early Proteins metabolism, Liver metabolism, Macrophages metabolism, Male, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Muromegalovirus growth & development, Muromegalovirus physiology, Phenotype, Signal Transduction, Tumor Necrosis Factor-alpha analysis, Tumor Necrosis Factor-alpha genetics, Viral Proteins genetics, Viral Proteins metabolism, Virus Replication, Gene Expression Regulation, Viral genetics, Herpesviridae Infections immunology, Immediate-Early Proteins genetics, Muromegalovirus genetics, Tumor Necrosis Factor-alpha metabolism
Abstract

Little is known about the role of viral genes in modulating host cytokine responses. Here we report a new functional role of the viral encoded IE1 protein of the murine cytomegalovirus in sculpting the inflammatory response in an acute infection. In time course experiments of infected primary macrophages (MΦs) measuring cytokine production levels, genetic ablation of the immediate-early 1 (ie1) gene results in a significant increase in TNFα production. Intracellular staining for cytokine production and viral early gene expression shows that TNFα production is highly associated with the productively infected MΦ population of cells. The ie1- dependent phenotype of enhanced MΦ TNFα production occurs at both protein and RNA levels. Noticeably, we show in a series of in vivo infection experiments that in multiple organs the presence of ie1 potently inhibits the pro-inflammatory cytokine response. From these experiments, levels of TNFα, and to a lesser extent IFNβ, but not the anti-inflammatory cytokine IL10, are moderated in the presence of ie1. The ie1- mediated inhibition of TNFα production has a similar quantitative phenotype profile in infection of susceptible (BALB/c) and resistant (C57BL/6) mouse strains as well as in a severe immuno-ablative model of infection. In vitro experiments with infected macrophages reveal that deletion of ie1 results in increased sensitivity of viral replication to TNFα inhibition. However, in vivo infection studies show that genetic ablation of TNFα or TNFRp55 receptor is not sufficient to rescue the restricted replication phenotype of the ie1 mutant virus. These results provide, for the first time, evidence for a role of IE1 as a regulator of the pro-inflammatory response and demonstrate a specific pathogen gene capable of moderating the host production of TNFα in vivo.

Published
2012
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20. Sch9 regulates ribosome biogenesis via Stb3, Dot6 and Tod6 and the histone deacetylase complex RPD3L.

Author

Huber A, French SL, Tekotte H, Yerlikaya S, Stahl M, Perepelkina MP, Tyers M, Rougemont J, Beyer AL, and Loewith R

Subjects
RNA, Transfer biosynthesis, Transcription, Genetic, Gene Expression Regulation, Fungal, RNA, Ribosomal biosynthesis, Ribosomal Proteins biosynthesis, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism, Signal Transduction
Abstract

TORC1 is a conserved multisubunit kinase complex that regulates many aspects of eukaryotic growth including the biosynthesis of ribosomes. The TOR protein kinase resident in TORC1 is responsive to environmental cues and is potently inhibited by the natural product rapamycin. Recent characterization of the rapamycin-sensitive phosphoproteome in yeast has yielded insights into how TORC1 regulates growth. Here, we show that Sch9, an AGC family kinase and direct substrate of TORC1, promotes ribosome biogenesis (Ribi) and ribosomal protein (RP) gene expression via direct inhibitory phosphorylation of the transcriptional repressors Stb3, Dot6 and Tod6. Deletion of STB3, DOT6 and TOD6 partially bypasses the growth and cell size defects of an sch9 strain and reveals interdependent regulation of both Ribi and RP gene expression, and other aspects of Ribi. Dephosphorylation of Stb3, Dot6 and Tod6 enables recruitment of the RPD3L histone deacetylase complex to repress Ribi/RP gene promoters. Taken together with previous studies, these results suggest that Sch9 is a master regulator of ribosome biogenesis through the control of Ribi, RP, ribosomal RNA and tRNA gene transcription.

Published
2011
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21. SCFCdc4 enables mating type switching in yeast by cyclin-dependent kinase-mediated elimination of the Ash1 transcriptional repressor.

Author

Liu Q, Larsen B, Ricicova M, Orlicky S, Tekotte H, Tang X, Craig K, Quiring A, Le Bihan T, Hansen C, Sicheri F, and Tyers M

Subjects
Amino Acid Sequence, CDC28 Protein Kinase, S cerevisiae metabolism, Cell Cycle, Gene Silencing, Molecular Sequence Data, Phosphorylation, Phosphothreonine metabolism, Protein Binding, Protein Processing, Post-Translational, Protein Stability, Protein Transport, Repressor Proteins chemistry, Saccharomyces cerevisiae cytology, Saccharomyces cerevisiae Proteins chemistry, Ubiquitination, Cell Cycle Proteins metabolism, Cyclin-Dependent Kinases metabolism, F-Box Proteins metabolism, Genes, Mating Type, Fungal, Repressor Proteins metabolism, Saccharomyces cerevisiae enzymology, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins metabolism, Transcription, Genetic, Ubiquitin-Protein Ligases metabolism
Abstract

In the budding yeast Saccharomyces cerevisiae, mother cells switch mating types between a and α forms, whereas daughter cells do not. This developmental asymmetry arises because the expression of the HO endonuclease, which initiates the interconversion of a and α mating type cassettes, is extinguished by the daughter-specific Ash1 transcriptional repressor. When daughters become mothers in the subsequent cell cycle, Ash1 must be eliminated to enable a new developmental state. Here, we report that the ubiquitin ligase SCF(Cdc4) mediates the phosphorylation-dependent elimination of Ash1. The inactivation of SCF(Cdc4) stabilizes Ash1 in vivo, and consistently, Ash1 binds to and is ubiquitinated by SCF(Cdc4) in a phosphorylation-dependent manner in vitro. The mutation of a critical in vivo cyclin-dependent kinase (CDK) phosphorylation site (Thr290) on Ash1 reduces its ubiquitination and rate of degradation in vivo and decreases the frequency of mating type switching. Ash1 associates with active Cdc28 kinase in vivo and is targeted to SCF(Cdc4) in a Cdc28-dependent fashion in vivo and in vitro. Ash1 recognition by Cdc4 appears to be mediated by at least three phosphorylation sites that form two redundant diphosphorylated degrons. The phosphorylation-dependent elimination of Ash1 by the ubiquitin-proteasome system thus underpins developmental asymmetry in budding yeast.

Published
2011
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22. Imaging the migrating border cell cluster in living Drosophila egg chambers.

Author

Tekotte H, Tollervey D, and Davis I

Subjects
Animals, Drosophila physiology, Female, Green Fluorescent Proteins, Oogenesis, Ovary cytology, Cell Movement, Drosophila cytology, Microscopy, Interference methods
Abstract

Cell migration is a key process in animal development and central to the spread of cancer. Border cell migration in Drosophila egg chambers is an excellent general model for cell migration, but lacks techniques for studying this process in living cells. Here, we describe a simple and effective method of preparing egg chambers in halocarbon oil. The movement and behavior of the migrating border cells can reproducibly be followed in up to 25 egg chambers simultaneously by time-lapse microscopy using a variety of green fluorescent protein markers on a widefield microscope over a period of 4 hr. Our studies reveal a remarkably linear migration route of the border cell cluster and highly dynamic activity within their cluster. Migrating cells rapidly alter their relative positions and generate transient protrusions. These activities are likely to play key roles in the mechanism of migration and cannot readily be analyzed using fixed samples., (2007 Wiley-Liss, Inc.)

Published
2007
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23. Bruno: a double turn-off for Oskar.

Author

Tekotte H and Davis I

Subjects
Animals, Drosophila Proteins genetics, Gene Silencing, Protein Biosynthesis, RNA, Messenger metabolism, RNA-Binding Proteins genetics, Drosophila Proteins metabolism, Drosophila melanogaster physiology, RNA-Binding Proteins metabolism
Abstract

In Drosophila, the posterior localization of oskar mRNA and its translational regulation are essential for axis specification and germline formation. Recently in Cell, demonstrated that Bruno inhibits cap-dependent translation of oskar mRNA and uncovered a novel Bruno-dependent assembly of oskar mRNA into multimeric RNP particles, which are inaccessible to the translational machinery. This work provides a novel link between mRNA localization, particle formation, and translational regulation.

Published
2006
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24. Intracellular mRNA localization: motors move messages.

Author

Tekotte H and Davis I

Subjects
Animals, Drosophila genetics, Drosophila metabolism, Drosophila Proteins genetics, Dyneins metabolism, Kinesins metabolism, Myosin Type V metabolism, Trans-Activators metabolism, Transcription Factors genetics, Yeasts genetics, Yeasts metabolism, DNA-Binding Proteins, Molecular Motor Proteins metabolism, RNA, Messenger metabolism
Abstract

Intracellular mRNA localization is a common mechanism of post-transcriptional regulation of gene expression. In a wide range of organisms, mRNA localization coupled with translational regulation target the proteins to their site of function. Here, we describe recent exciting evidence that some mRNAs are transported as particles along the cytoskeleton by the molecular motors dynein, kinesin or myosin. We discuss the key questions of how localized mRNAs might be linked to motors and what determines their cytoplasmic destinations.

Published
2002
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25. Dcas is required for importin-alpha3 nuclear export and mechano-sensory organ cell fate specification in Drosophila.

Author

Tekotte H, Berdnik D, Török T, Buszczak M, Jones LM, Cooley L, Knoblich JA, and Davis I

Subjects
Active Transport, Cell Nucleus physiology, Animals, Apoptosis, DNA Helicases metabolism, Drosophila melanogaster genetics, Embryo, Nonmammalian physiology, Gene Expression Regulation, Developmental, In Situ Hybridization, Morphogenesis, Phylogeny, RNA, Messenger genetics, Cellular Apoptosis Susceptibility Protein genetics, Drosophila Proteins, Drosophila melanogaster embryology, Mechanoreceptors embryology, Sense Organs embryology, alpha Karyopherins metabolism
Abstract

We have studied the in vivo function and tissue specificity of Dcas, the Drosophila ortholog of CAS, the importin beta-like export receptor for importin alpha. While dcas mRNA is specifically expressed in the embryonic central nervous system, Dcas protein is maternally supplied to all embryonic cells and its nuclear/cytoplasmic distribution varies in different tissues and times in development. Unexpectedly, hypomorphic alleles of dcas show specific transformations in mechano-sensory organ cell identity, characteristic of mutations that increase Notch signaling. Dcas is essential for efficient importin-alpha3 nuclear export in mechano-sensory cells and the surrounding epidermal cells and is indirectly required for the import of one component of the Notch pathway, but not others tested. We interpret the specificity of the dcas phenotype as indicating that one or more Notch signaling components are particularly sensitive to a disruption in nuclear protein import. We propose that mutations in house keeping genes often cause specific developmental phenotypes, such as those observed in many human genetic disorders., (Copyright 2002 Elsevier Science (USA).)

Published
2002
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26. Perturbing nuclear transport in Drosophila eye imaginal discs causes specific cell adhesion and axon guidance defects.

Author

Kumar JP, Wilkie GS, Tekotte H, Moses K, and Davis I

Subjects
Animals, Animals, Genetically Modified, Axons ultrastructure, Blastoderm metabolism, Cell Adhesion, Drosophila genetics, Drosophila Proteins genetics, Drosophila Proteins metabolism, Eye cytology, Humans, Photoreceptor Cells, Invertebrate embryology, RNA, Messenger genetics, RNA, Messenger metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Deletion, beta Karyopherins genetics, beta Karyopherins metabolism, Active Transport, Cell Nucleus, Drosophila embryology, Drosophila metabolism, Eye embryology
Abstract

To study nucleocytoplasmic transport during multicellular development, we developed a sensitive nuclear protein import assay in living blastoderm embryos. We show that dominant negative truncations of the human nuclear transport receptor karyopherinbeta/Importinbeta (DNImpbeta) disrupt mRNA export and protein import in Drosophila. To test the sensitivity of different developmental processes to nuclear trafficking perturbations, we expressed DNImpbeta behind the morphogenetic furrow of the eye disc, at a time when photoreceptors are patterned and project their axons to the brain. DNImpbeta expression does not disrupt the correct specification of different photoreceptors, but causes a defect in cell adhesion that leads to some photoreceptors descending below the layer of ommatidia. The photoreceptors initially project their axons correctly to the posterior, but later their axons are unable to enter the optic stalk en route to the brain and continue to project an extensive network of misguided axons. The axon guidance and cell adhesion defects are both due to a disruption in the function of Ketel, the Drosophila ortholog of Importinbeta. We conclude that cell adhesion and axon guidance in the eye have specific requirements for nucleocytoplasmic transport, despite involving processes that occur primarily at the cell surface.

Published
2001
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27. Cooperative interaction of ets-1 with USF-1 required for HIV-1 enhancer activity in T cells.

Author

Sieweke MH, Tekotte H, Jarosch U, and Graf T

Subjects
Amino Acid Sequence, Animals, Binding Sites, Cell Line, Cloning, Molecular, DNA, Viral metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Genes, Dominant, HIV-1 physiology, Helix-Loop-Helix Motifs, Humans, Jurkat Cells, Leucine Zippers, Molecular Sequence Data, Mutation, Proto-Oncogene Protein c-ets-1, Proto-Oncogene Proteins c-ets, Quail, Recombinant Fusion Proteins, Transcription Factors genetics, Transcriptional Activation physiology, Transfection, Upstream Stimulatory Factors, HIV Enhancer genetics, HIV-1 genetics, Proto-Oncogene Proteins metabolism, T-Lymphocytes virology, Transcription Factors metabolism
Abstract

The distal enhancer region of the human immunodeficiency virus 1 (HIV-1) long terminal repeat (LTR) is known to be essential for HIV replication and to contain immediately adjacent E-box and Ets binding sites. Based on a yeast one-hybrid screen we have identified the E-box binding protein USF-1 as a direct interaction partner of Ets-1 and found that the complex acts on this enhancer element. The binding surfaces of USF-1 and Ets-1 map to their DNA-binding domains and although these domains are highly conserved, the interaction is very selective within the respective protein family. USF-1 and Ets-1 synergize in specific DNA binding as well as in the transactivation of reporter constructs containing the enhancer element, and mutations of the individual binding sites dramatically reduce reporter activity in T cells. In addition, a dominant negative Ets-1 mutant inhibits both USF-1-mediated transactivation and the activity of the HIV-1 LTR in T cells. The inhibition is independent of Ets DNA-binding sites but requires the Ets binding surface on USF-1, highlighting the importance of the direct protein-protein interaction. Together these results indicate that the interaction between Ets-1 and USF-1 is required for full transcriptional activity of the HIV-1 LTR in T cells.

Published
1998
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28. MafB represses erythroid genes and differentiation through direct interaction with c-Ets-1.

Author

Sieweke MH, Tekotte H, Frampton J, and Graf T

Subjects
Animals, Cell Differentiation, Erythroblasts physiology, Erythrocytes physiology, Hematopoietic Stem Cells physiology, Heme biosynthesis, Leucine Zippers, Proto-Oncogene Protein c-ets-1, Proto-Oncogene Proteins c-ets, Receptors, Transferrin biosynthesis, Recombinant Proteins metabolism, Repressor Proteins metabolism, Saccharomyces cerevisiae, Transcriptional Activation, Transfection, Avian Proteins, DNA-Binding Proteins, Erythroblasts cytology, Erythrocytes cytology, Erythropoiesis physiology, Hematopoietic Stem Cells cytology, Oncogene Proteins metabolism, Proto-Oncogene Proteins metabolism, Trans-Activators metabolism, Transcription Factors metabolism
Abstract

Using a yeast interaction screen with a DNA-bound Ets-1 protein we have identified MafB as a direct interaction partner. This distant AP-1 relative, which is specifically expressed in myelomonocytic cells, binds to the DNA binding domain of Ets-1 via its basic region/leucine zipper domain. MafB represses Ets-1 transactivation of synthetic promoters containing Ets binding sites in yeast as well as avian cells. Both Ets-1 and Maf family proteins have been implicated in erythroid specific gene expression. Here we show that MafB inhibits Ets-1-mediated transactivation of the transferrin receptor, which is essential for heme synthesis and erythroid differentiation. Consequently, overexpression of MafB in an erythroblast cell line down-regulates the endogenous transferrin receptor gene and inhibits the cells' potential to differentiate into erythrocytes, without affecting cellular proliferation.

Published
1997

29. MafB is an interaction partner and repressor of Ets-1 that inhibits erythroid differentiation.

Author

Sieweke MH, Tekotte H, Frampton J, and Graf T

Subjects
Animals, Base Sequence, Binding Sites physiology, Cell Differentiation drug effects, Cell Differentiation physiology, Chick Embryo, Clone Cells physiology, DNA, Complementary physiology, DNA-Binding Proteins metabolism, DNA-Binding Proteins physiology, Erythroblasts physiology, G-Box Binding Factors, Gene Expression Regulation physiology, Genetic Testing, Hematopoiesis genetics, Macrophages physiology, MafB Transcription Factor, Molecular Sequence Data, Oncogene Proteins metabolism, Proto-Oncogene Protein c-ets-1, Proto-Oncogene Proteins antagonists & inhibitors, Proto-Oncogene Proteins c-ets, Receptors, Transferrin genetics, Repressor Proteins genetics, Trans-Activators metabolism, Transcription Factors antagonists & inhibitors, Vertebrates, Yeasts genetics, Avian Proteins, DNA-Binding Proteins genetics, Erythroblasts cytology, Oncogene Proteins genetics, Protein-Tyrosine Kinases metabolism, Proto-Oncogene Proteins metabolism, Trans-Activators genetics, Transcription Factors metabolism
Abstract

Using a yeast one-hybrid screen with a DNA-bound Ets-1 protein, we have identified MafB, an AP-1 like protein, as a direct interaction partner. MafB is specifically expressed in myelomonocytic cells and binds to the DNA-binding domain of Ets-1 via its basic region or leucine-zipper domain. Furthermore, it represses Ets-1 transactivation of synthetic promoters containing Ets binding sites and inhibits Ets-1-mediated transactivation of the transferrin receptor, which is known to be essential for erythroid differentiation. Accordingly, overexpression of MafB in an erythroblast cell line down-regulates the endogenous transferrin receptor gene and inhibits differentiation without affecting cell proliferation. These results highlight the importance of inhibitory interactions between transcription factors in regulating lineage-specific gene expression.

Published
1996
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30. A novel complex of nucleoporins, which includes Sec13p and a Sec13p homolog, is essential for normal nuclear pores.

Author

Siniossoglou S, Wimmer C, Rieger M, Doye V, Tekotte H, Weise C, Emig S, Segref A, and Hurt EC

Subjects
Amino Acid Sequence, Biological Transport, Carboxypeptidases metabolism, Cathepsin A, Epitopes, Fungal Proteins isolation & purification, Membrane Proteins isolation & purification, Molecular Sequence Data, Molecular Weight, Nuclear Envelope ultrastructure, Nuclear Proteins analysis, Nuclear Proteins chemistry, Nuclear Proteins isolation & purification, Poly A metabolism, Proto-Oncogene Proteins c-myc genetics, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins isolation & purification, Sequence Homology, Amino Acid, Staphylococcal Protein A genetics, Yeasts metabolism, Fungal Proteins metabolism, Membrane Proteins metabolism, Nuclear Envelope chemistry, Nuclear Pore Complex Proteins, Nuclear Proteins metabolism, Nuclear Proteins physiology, Saccharomyces cerevisiae Proteins
Abstract

In a genetic screen for nucleoporin-interacting components, a novel nuclear pore protein Nup84p, which exhibits homology to mammalian Nup107p, was isolated. Nup84p forms a complex with five proteins, of which Nup120p, Nup85p, Sec13p, and a Sec13p homolog were identified. Upon isolation of Sec13p-ProtA, nucleoporins were still associated, but the major copurifying band was a 150 kDa protein, showing that Sec13p occurs in two complexes. Disruption of any of the genes encoding Nup84p, Nup85p, or Nup120p caused defects in nuclear membrane and nuclear pore complex organization, as well as in poly(A)+ RNA transport. Thus, the Nup84p complex in conjunction with Sec13-type proteins is required for correct nuclear pore biogenesis.

Published
1996
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