Your search keyword '"Recombinant Fusion Proteins metabolism"' showing total 3,034 results

1. Development and Validation of a Proximity Labeling Fusion Protein Construct to Identify the Protein-Protein Interactions of Transcription Factors.

Author

Leskinen HL and Udvadia AJ

Subjects

Humans, Recombinant Fusion Proteins metabolism, Recombinant Fusion Proteins genetics, Protein Binding, Mass Spectrometry methods, Protein Processing, Post-Translational, Endonucleases, Multifunctional Enzymes, Biotinylation, Protein Interaction Mapping methods, Transcription Factors metabolism, DNA-(Apurinic or Apyrimidinic Site) Lyase metabolism, DNA-(Apurinic or Apyrimidinic Site) Lyase chemistry

Abstract

Dynamic interactions between transcription factors govern changes in gene expression that mediate changes in cell state accompanying injury response and regeneration. Transcription factors frequently function as obligate dimers whose activity is often modulated by post-translational modifications. These critical and often transient interactions are not easily detected by traditional methods to investigate protein-protein interactions. This chapter discusses the design and validation of a fusion protein involving a transcription factor tethered to a proximity labeling ligase, APEX2. In this technique, proteins are biotinylated within a small radius of the transcription factor of interest, regardless of time of interaction. Here we discuss the validations required to ensure proper functioning of the transcription factor proximity labeling tool and the sample preparation of biotinylated proteins for mass spectrometry analysis of putative protein interactors., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

2. Generation of a recombinant version of a biologically active cell-permeant human HAND2 transcription factor from E. coli.

Author

Haridhasapavalan KK, Sundaravadivelu PK, Joshi N, Das NJ, Mohapatra A, Voorkara U, Kaveeshwar V, and Thummer RP

Subjects

Animals, Chick Embryo, Codon metabolism, Humans, Recombinant Fusion Proteins metabolism, Recombinant Proteins genetics, Recombinant Proteins metabolism, Escherichia coli genetics, Escherichia coli metabolism, Transcription Factors metabolism

Abstract

Transcription factor HAND2 has a significant role in vascularization, angiogenesis, and cardiac neural crest development. It is one of the key cardiac factors crucial for the enhanced derivation of functional and mature myocytes from non-myocyte cells. Here, we report the generation of the recombinant human HAND2 fusion protein from the heterologous system. First, we cloned the full-length human HAND2 gene (only protein-coding sequence) after codon optimization along with the fusion tags (for cell penetration, nuclear translocation, and affinity purification) into the expression vector. We then transformed and expressed it in Escherichia coli strain, BL21(DE3). Next, the effect (in terms of expression) of tagging fusion tags with this recombinant protein at two different terminals was also investigated. Using affinity chromatography, we established the one-step homogeneous purification of recombinant human HAND2 fusion protein; and through circular dichroism spectroscopy, we established that this purified protein had retained its secondary structure. We then showed that this purified human protein could transduce the human cells and translocate to its nucleus. The generated recombinant HAND2 fusion protein showed angiogenic potential in the ex vivo chicken embryo model. Following transduction in MEF2C overexpressing cardiomyoblast cells, this purified recombinant protein synergistically activated the α-MHC promoter and induced GFP expression in the α-MHC-eGFP reporter assay. Prospectively, the purified bioactive recombinant HAND2 protein can potentially be a safe and effective molecular tool in the direct cardiac reprogramming process and other biological applications., (© 2022. The Author(s).)

Published

2022

3. Identification of Optimal Expression Parameters and Purification of a Codon-Optimized Human GLIS1 Transcription Factor from Escherichia coli.

Author

Dey C, Venkatesan V, and Thummer RP

Subjects

Cell Line, Tumor, Cell Movement, Cloning, Molecular, Codon, DNA-Binding Proteins chemistry, DNA-Binding Proteins metabolism, Escherichia coli growth & development, Escherichia coli metabolism, Gene Expression, Genetic Vectors, Humans, Protein Structure, Secondary, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins metabolism, Solubility, Transcription Factors chemistry, Transcription Factors metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins isolation & purification, Escherichia coli genetics, Transcription Factors genetics, Transcription Factors isolation & purification

Abstract

GLIS1 has multiple roles in embryonic development and in deriving induced pluripotent stem cells by aiding signaling pathways and chromatin assembly. An inexpensive and simple method to produce human GLIS1 protein from Escherichia coli (E. coli) is demonstrated in this study. Various parameters such as codon usage bias, E. coli strains, media, induction conditions (such as inducer concentration, cell density, time, and temperature), and genetic constructs were investigated to obtain soluble expression of human GLIS1 protein. Using identified expression conditions and an appropriate genetic construct, the human GLIS1 protein was homogeneously purified (purity > 90%) under native conditions. Importantly, the purified protein has upheld a stable secondary structure, as demonstrated by circular dichroism spectroscopy. To the best of our knowledge, this is the first study to report the ideal expression conditions of human GLIS1 protein in E. coli to achieve soluble expression and purification under native conditions, upholding its stable secondary structure post-purification. The biological activity of the purified GLIS1 fusion protein was further assessed in MDA-MB-231 cells. This biologically active human GLIS1 protein potentiates new avenues to understand its molecular mechanisms in different cellular functions in various cancers and in the generation of induced pluripotent stem cells., (© 2021. The Author(s), under exclusive licence to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2022

4. Target protein deglycosylation in living cells by a nanobody-fused split O-GlcNAcase.

Author

Ge Y, Ramirez DH, Yang B, D'Souza AK, Aonbangkhen C, Wong S, and Woo CM

Subjects

Antigens, Neoplasm chemistry, Antigens, Neoplasm genetics, Biological Assay, Catalytic Domain, Drug Delivery Systems methods, Gene Expression, Glycosylation, HEK293 Cells, Histone Acetyltransferases chemistry, Histone Acetyltransferases genetics, Humans, Hyaluronoglucosaminidase chemistry, Hyaluronoglucosaminidase genetics, Hydrolysis, JNK Mitogen-Activated Protein Kinases genetics, Membrane Glycoproteins genetics, Nuclear Pore Complex Proteins genetics, Plasmids chemistry, Plasmids metabolism, Protein Binding, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Single-Domain Antibodies metabolism, Sp1 Transcription Factor genetics, Transcription Factors genetics, Transfection methods, Antigens, Neoplasm metabolism, Histone Acetyltransferases metabolism, Hyaluronoglucosaminidase metabolism, JNK Mitogen-Activated Protein Kinases metabolism, Membrane Glycoproteins metabolism, Nuclear Pore Complex Proteins metabolism, Recombinant Fusion Proteins metabolism, Single-Domain Antibodies chemistry, Sp1 Transcription Factor metabolism, Transcription Factors metabolism

Abstract

O-linked N-acetylglucosamine (O-GlcNAc) is an essential and dynamic post-translational modification that is presented on thousands of nucleocytoplasmic proteins. Interrogating the role of O-GlcNAc on a single target protein is crucial, yet challenging to perform in cells. Herein, we developed a nanobody-fused split O-GlcNAcase (OGA) as an O-GlcNAc eraser for selective deglycosylation of a target protein in cells. After systematic cellular optimization, we identified a split OGA with reduced inherent deglycosidase activity that selectively removed O-GlcNAc from the desired target protein when directed by a nanobody. We demonstrate the generality of the nanobody-fused split OGA using four nanobodies against five target proteins and use the system to study the impact of O-GlcNAc on the transcription factors c-Jun and c-Fos. The nanobody-directed O-GlcNAc eraser provides a new strategy for the functional evaluation and engineering of O-GlcNAc via the selective removal of O-GlcNAc from individual proteins directly in cells.

Published

2021

5. Function of the TRY C-terminal region artificially fused with its homologous transcription factors inducing root hair differentiation in Arabidopsis.

Author

Wakamatsu J, Nagao K, Sumida Y, Tanaka W, Sambongi Y, and Tominaga R

Subjects

Amino Acid Sequence, Arabidopsis cytology, Arabidopsis metabolism, Arabidopsis Proteins metabolism, Cell Differentiation, DNA-Binding Proteins metabolism, Gene Expression Regulation, Plant, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Plant Cells metabolism, Plant Epidermis cytology, Plant Epidermis metabolism, Plant Roots cytology, Plant Roots metabolism, Plants, Genetically Modified, Proto-Oncogene Proteins c-myb metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Alignment, Sequence Homology, Amino Acid, Transcription Factors metabolism, Arabidopsis genetics, Arabidopsis Proteins genetics, DNA-Binding Proteins genetics, Plant Epidermis genetics, Plant Roots genetics, Proto-Oncogene Proteins c-myb genetics, Transcription Factors genetics

Abstract

TRIPTYCHON (TRY) is one of the R3-MYB transcription factors. Its extended C-terminal 19 amino-acid region (CTRY) is considered to affect the ability of root hair differentiation in Arabidopsis. Here, to further understand the function of CTRY, it, together with GFP, was artificially fused with TRY homologs, CPC and ETC1, which do not contain such extended regions and induce root hair differentiation. Arabidopsis transgenic plants carrying the fusion proteins, CPC-CTRY-GFP and ETC1-CTRY-GFP, induced root hair differentiation as observed in those carrying the original proteins without CTRY. The expression levels of the fusion proteins in the transgenic plants were essentially the same as those of the original proteins, although their subcellular localization to nuclei of root epidermal cells was slightly changed by CTRY. Therefore, CTRY does not affect the ability of CPC and ETC1 to induce root hair differentiation when artificially fused, and its function may be restricted in TRY., (© The Author(s) 2021. Published by Oxford University Press on behalf of Japan Society for Bioscience, Biotechnology, and Agrochemistry.)

Published

2021

6. Combining Cell Fate Reprogramming and Protein Engineering to Study Transcription Factor Functions.

Author

Adrian-Segarra JM, Weigel B, and Mall M

Subjects

Cloning, Molecular, Gene Expression, Gene Expression Regulation, Developmental, Humans, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Analysis, DNA, Transcription Factors metabolism, Cell Differentiation genetics, Cellular Reprogramming, Cellular Reprogramming Techniques, Protein Engineering methods, Transcription Factors genetics

Abstract

Gene expression regulation by transcription factors plays a central role in determining and maintaining cell fate during normal development as well as induced cell fate reprogramming. Induction of cell identity-determining gene regulatory networks by reprogramming factors that act as transcriptional activators is key to induce desired cell fates. Conversely, repression of unwanted genetic programs by transcriptional repressors is equally important to ensure cell fate fidelity. Here we describe engineering techniques to create fusion proteins that allow exploration of the major transcriptional contribution (activation or repression) of specific neuronal reprogramming factors during direct cell fate conversion. This method can be extended to every reprogramming regime to enable the functional categorization of any transcription factor., (© 2021. Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2021

7. The B″-family subunits of protein phosphatase 2A are necessary for in-vitro dephosphorylation of the Arabidopsis mechanosensory transcription factor VIP1.

Author

Yoon HS, Fujino K, Liu S, Takano T, and Tsugama D

Subjects

Arabidopsis genetics, Arabidopsis metabolism, Arabidopsis Proteins genetics, Gene Expression Regulation, Plant, Genes, Plant, Osmotic Pressure, Phosphorylation, Plants, Genetically Modified, Protein Interaction Domains and Motifs, Protein Phosphatase 2 genetics, Protein Subunits, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Transcription Factors genetics, Two-Hybrid System Techniques, Arabidopsis Proteins chemistry, Arabidopsis Proteins metabolism, Protein Phosphatase 2 chemistry, Protein Phosphatase 2 metabolism, Transcription Factors metabolism

Abstract

Protein phosphatase 2A (PP2A) B″-family subunits have Ca 2+ -binding EF-hand motifs and can bind PP2A substrates. Arabidopsis thaliana PP2A B″-family subunits are encoded by six genes, and bind a transcription factor, VIP1. VIP1 is dephosphorylated and nuclear-localized by hypo-osmotic stress. However, whether PP2A B″-family subunits mediate the VIP1 dephosphorylation is unclear. Here, we show by yeast two-hybrid and in vitro pull down assays that Arabidopsis PP2A B″-family subunits bind Arabidopsis PP2A A (scaffold) subunits. We also show that VIP1 dephosphorylation in vitro can be induced by a PP2A B″-family subunit., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2020 Elsevier Inc. All rights reserved.)

Published

2021

8. Characterization of the zinc finger proteins ZMYM2 and ZMYM4 as novel B-MYB binding proteins.

Author

Cibis H, Biyanee A, Dörner W, Mootz HD, and Klempnauer KH

Subjects

Carrier Proteins genetics, Cell Cycle Proteins genetics, DNA-Binding Proteins genetics, G1 Phase, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, HEK293 Cells, Hep G2 Cells, Humans, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, S Phase, Sumoylation, Trans-Activators genetics, Transcription Factors genetics, Zinc Fingers, Carrier Proteins metabolism, Cell Cycle Proteins metabolism, DNA-Binding Proteins metabolism, Trans-Activators metabolism, Transcription Factors metabolism

Abstract

B-MYB, a highly conserved member of the MYB transcription factor family, is expressed ubiquitously in proliferating cells and plays key roles in important cell cycle-related processes, such as control of G2/M-phase transcription, cytokinesis, G1/S-phase progression and DNA-damage reponse. Deregulation of B-MYB function is characteristic of several types of tumor cells, underlining its oncogenic potential. To gain a better understanding of the functions of B-MYB we have employed affinity purification coupled to mass spectrometry to discover novel B-MYB interacting proteins. Here we have identified the zinc-finger proteins ZMYM2 and ZMYM4 as novel B-MYB binding proteins. ZMYM4 is a poorly studied protein whose initial characterization reported here shows that it is highly SUMOylated and that its interaction with B-MYB is stimulated upon induction of DNA damage. Unlike knockdown of B-MYB, which causes G2/M arrest and defective cytokinesis in HEK293 cells, knockdown of ZMYM2 or ZMYM4 have no obvious effects on the cell cycle of these cells. By contrast, knockdown of ZMYM2 strongly impaired the G1/S-phase progression of HepG2 cells, suggesting that ZMYM2, like B-MYB, is required for entry into S-phase in these cells. Overall, our work identifies two novel B-MYB binding partners with possible functions in the DNA-damage response and the G1/S-transition.

Published

2020

9. Engineering DNA recognition and allosteric response properties of TetR family proteins by using a module-swapping strategy.

Author

Dimas RP, Jordan BR, Jiang XL, Martini C, Glavy JS, Patterson DP, Morcos F, and Chan CTY

Subjects

Allosteric Regulation, Base Sequence, Binding Sites, Cloning, Molecular, Crystallography, X-Ray, DNA genetics, DNA metabolism, Escherichia coli metabolism, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Gene Expression, Genetic Vectors chemistry, Genetic Vectors metabolism, Kinetics, Models, Molecular, Mutation, Nucleic Acid Conformation, Protein Binding, Protein Conformation, alpha-Helical, Protein Interaction Domains and Motifs, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Repressor Proteins genetics, Repressor Proteins metabolism, Sequence Alignment, Transcription Factors genetics, Transcription Factors metabolism, DNA chemistry, Escherichia coli genetics, Escherichia coli Proteins chemistry, Protein Engineering, Recombinant Fusion Proteins chemistry, Repressor Proteins chemistry, Transcription Factors chemistry

Abstract

The development of synthetic biological systems requires modular biomolecular components to flexibly alter response pathways. In previous studies, we have established a module-swapping design principle to engineer allosteric response and DNA recognition properties among regulators in the LacI family, in which the engineered regulators served as effective components for implementing new cellular behavior. Here we introduced this protein engineering strategy to two regulators in the TetR family: TetR (UniProt Accession ID: P04483) and MphR (Q9EVJ6). The TetR DNA-binding module and the MphR ligand-binding module were used to create the TetR-MphR. This resulting hybrid regulator possesses DNA-binding properties of TetR and ligand response properties of MphR, which is able to control gene expression in response to a molecular signal in cells. Furthermore, we studied molecular interactions between the TetR DNA-binding module and MphR ligand-binding module by using mutant analysis. Together, we demonstrated that TetR family regulators contain discrete and functional modules that can be used to build biological components with novel properties. This work highlights the utility of rational design as a means of creating modular parts for cell engineering and introduces new possibilities in rewiring cellular response pathways., (© The Author(s) 2019. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2019

10. Direct Observation and Analysis of the Dynamics of the Photoresponsive Transcription Factor GAL4.

Author

Raghavan G, Hidaka K, Sugiyama H, and Endo M

Subjects

Binding Sites, DNA chemistry, DNA radiation effects, DNA-Binding Proteins genetics, DNA-Binding Proteins radiation effects, Fungal Proteins genetics, Fungal Proteins radiation effects, Light, Microscopy, Atomic Force, Protein Binding, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins radiation effects, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins radiation effects, Transcription Factors genetics, Transcription Factors radiation effects, DNA metabolism, DNA-Binding Proteins metabolism, Fungal Proteins metabolism, Recombinant Fusion Proteins metabolism, Saccharomyces cerevisiae Proteins metabolism, Transcription Factors metabolism

Abstract

Herein, the direct visualization of the dynamic interaction between a photoresponsive transcription factor fusion, GAL4-VVD, and DNA using high-speed atomic force microscopy (HS-AFM) is reported. A series of different GAL4-VVD movements, such as binding, sliding, stalling, and dissociation, was observed. Inter-strand jumping on two double-stranded (ds) DNAs was also observed. Detailed analysis using a long substrate DNA strand containing five GAL4-binding sites revealed that GAL4-VVD randomly moved on the dsDNA using sliding and hopping to rapidly find specific binding sites, and then stalled to the specific sites to form a stable complex formation. These results suggest the existence of different conformations of the protein to enable sliding and stalling. This single-molecule imaging system with nanoscale resolution provides an insight into the searching mechanism used by DNA-binding proteins., (© 2019 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2019

11. Structural and biochemical analyses of the nuclear pore complex component ELYS identify residues responsible for nucleosome binding.

Author

Kobayashi W, Takizawa Y, Aihara M, Negishi L, Ishii H, and Kurumizaka H

Subjects

Active Transport, Cell Nucleus genetics, Animals, Binding Sites, Cell Cycle genetics, Cloning, Molecular, Cryoelectron Microscopy, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Genetic Vectors chemistry, Genetic Vectors metabolism, Histones genetics, Histones metabolism, Humans, Models, Molecular, Nuclear Pore metabolism, Nuclear Pore ultrastructure, Nuclear Pore Complex Proteins genetics, Nuclear Pore Complex Proteins metabolism, Nucleosomes metabolism, Nucleosomes ultrastructure, Protein Binding, Protein Interaction Domains and Motifs, Protein Structure, Secondary, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Transcription Factors genetics, Transcription Factors metabolism, Xenopus Proteins genetics, Xenopus Proteins metabolism, Xenopus laevis genetics, Xenopus laevis metabolism, DNA-Binding Proteins chemistry, Histones chemistry, Nuclear Pore chemistry, Nuclear Pore Complex Proteins chemistry, Nucleosomes chemistry, Transcription Factors chemistry, Xenopus Proteins chemistry

Abstract

The nuclear pore complex embedded within the nuclear envelope is the essential architecture for trafficking macromolecules, such as proteins and RNAs, between the cytoplasm and nucleus. The nuclear pore complex assembly occurs on chromatin in the post-mitotic phase of the cell cycle. ELYS (MEL-28/AHCTF1) binds to the nucleosome, which is the basic chromatin unit, and promotes assembly of the complex around the chromosomes in cells. Here we show that the Arg-Arg-Lys (RRK) stretch of the C-terminal ELYS region plays an essential role in the nucleosome binding. The cryo-EM structure and the crosslinking mass spectrometry reveal that the ELYS C-terminal region directly binds to the acidic patch of the nucleosome. These results provide mechanistic insight into the ELYS-nucleosome interaction, which promotes the post-mitotic nuclear pore complex formation around chromosomes in cells., Competing Interests: The authors declare no competing interests.

Published

2019

12. Highly Sensitive and Selective Biosensor for a Disaccharide Based on an AraC-Like Transcriptional Regulator Transduced with Bioluminescence Resonance Energy Transfer.

Author

Caron K and Trowell SC

Subjects

Agrobacterium tumefaciens chemistry, Animals, Bacterial Proteins genetics, Bacterial Proteins metabolism, Clostridium perfringens chemistry, Energy Transfer, Green Fluorescent Proteins chemistry, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Lactose metabolism, Ligands, Limit of Detection, Luminescence, Protein Binding, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Renilla chemistry, Transcription Factors genetics, Transcription Factors metabolism, Bacterial Proteins chemistry, Biosensing Techniques methods, Lactose analysis, Milk chemistry, Transcription Factors chemistry

Abstract

Sensitive and selective quantification of individual sugars in complex media is technically challenging and usually requires HPLC separation. Accurate measurement without the need for separation would be highly desirable. The measurement of trace levels of lactose in lactose-reduced milk exemplifies the problem, with the added challenge that trace lactose must be measured in the presence of ≈140 mM glucose and galactose, the products of lactase digestion of lactose. Biosensing is an alternative to HPLC, but current biosensing methods, based on coupled-enzyme assays, tend to have poor sensitivity and complex biochemistry and can be time-consuming. We explored a fundamentally different approach, based on identifying a lactose-specific binding protein compatible with photonic transduction. We identified the BgaR transcriptional regulator of Clostridium perfringens, which is highly selective for lactose, as a suitable ligand binding domain and combined it with a bioluminescence energy resonance transfer transduction system. This BRET-based biosensor showed a 27% decrease in the BRET ratio in the presence of saturating (1 mM) lactose. Using a 5 min assay, the half maximal effective concentration (EC 50 ) for lactose in phosphate-buffered saline (PBS) was 12 μM. The biosensor was 200 times more sensitive to lactose than to glucose or galactose. Sensitivity and selectivity were not significantly affected by the presence of 10% (v/v) dialyzed milk. The biosensor is suitable for direct determination of residual lactose in lactase-treated milk, with a limit of detection of 0.2 μM, 100 times below the most stringent lactose-free standard and without the need to remove fat or protein from the sample.

Published

2018

13. An NAD + -dependent novel transcription factor controls stage conversion in Entamoeba .

Author

Manna D, Lentz CS, Ehrenkaufer GM, Suresh S, Bhat A, and Singh U

Subjects

Amino Acid Sequence, Base Sequence, Biocatalysis, Cell Nucleus metabolism, Consensus Sequence genetics, Entamoeba genetics, Models, Biological, Mutant Proteins metabolism, Promoter Regions, Genetic, Protein Stability, Protozoan Proteins chemistry, Protozoan Proteins metabolism, RNA Interference, Recombinant Fusion Proteins metabolism, Temperature, Trophozoites, Up-Regulation genetics, Entamoeba growth & development, Entamoeba metabolism, Life Cycle Stages genetics, NAD metabolism, Transcription Factors metabolism

Abstract

Developmental switching between life-cycle stages is a common feature among parasitic pathogens to facilitate disease transmission and pathogenesis. The protozoan parasite Entamoeba switches between invasive trophozoites and dormant cysts, but the encystation process remains poorly understood despite being central to amoebic biology. We identify a transcription factor, Encystation Regulatory Motif-Binding Protein (ERM-BP), that regulates encystation. Down-regulation of ERM-BP decreases encystation efficiency resulting in abnormal cysts with defective cyst walls. We demonstrate that direct binding of NAD + to ERM-BP affects ERM-BP conformation and facilitates its binding to promoter DNA. Additionally, cellular NAD + levels increase during encystation and exogenous NAD + enhances encystation consistent with the role of carbon source depletion in triggering Entamoeba encystation. Furthermore, ERM-BP catalyzes conversion of nicotinamide to nicotinic acid, which might have second messenger effects on stage conversion. Our findings link the metabolic cofactors nicotinamide and NAD + to transcriptional regulation via ERM-BP and provide the first mechanistic insights into Entamoeba encystation., Competing Interests: DM, CL, GE, SS, AB, US No competing interests declared, (© 2018, Manna et al.)

Published

2018

14. A zinc-finger fusion protein refines Gal4-defined neural circuits.

Author

Raghu SV, Mohammad F, Chua JY, Lam JSW, Loberas M, Sahani S, Barros CS, and Claridge-Chang A

Subjects

Animals, Gene Expression, Green Fluorescent Proteins metabolism, Protein Multimerization, Serotonergic Neurons metabolism, Drosophila Proteins metabolism, Drosophila melanogaster metabolism, Nerve Net metabolism, Recombinant Fusion Proteins metabolism, Transcription Factors metabolism, Zinc Fingers

Abstract

The analysis of behavior requires that the underlying neuronal circuits are identified and genetically isolated. In several major model species-most notably Drosophila-neurogeneticists identify and isolate neural circuits with a binary heterologous expression-control system: Gal4-UASG. One limitation of Gal4-UASG is that expression patterns are often too broad to map circuits precisely. To help refine the range of Gal4 lines, we developed an intersectional genetic AND operator. Interoperable with Gal4, the new system's key component is a fusion protein in which the DNA-binding domain of Gal4 has been replaced with a zinc finger domain with a different DNA-binding specificity. In combination with its cognate binding site (UASZ) the zinc-finger-replaced Gal4 ('Zal1') was functional as a standalone transcription factor. Zal1 transgenes also refined Gal4 expression ranges when combined with UASGZ, a hybrid upstream activation sequence. In this way, combining Gal4 and Zal1 drivers captured restricted cell sets compared with single drivers and improved genetic fidelity. This intersectional genetic AND operation presumably derives from the action of a heterodimeric transcription factor: Gal4-Zal1. Configurations of Zal1-UASZ and Zal1-Gal4-UASGZ are versatile tools for defining, refining, and manipulating targeted neural expression patterns with precision.

Published

2018

15. Activation of Nrf2 Is Required for Normal and ChREBPα-Augmented Glucose-Stimulated β-Cell Proliferation.

Author

Kumar A, Katz LS, Schulz AM, Kim M, Honig LB, Li L, Davenport B, Homann D, Garcia-Ocaña A, Herman MA, Haynes CM, Chipuk JE, and Scott DK

Subjects

Animals, Basic Helix-Loop-Helix Leucine Zipper Transcription Factors chemistry, Basic Helix-Loop-Helix Leucine Zipper Transcription Factors genetics, Cadaver, Cell Line, Tumor, Cell Proliferation, Humans, Insulin metabolism, Insulin Secretion, Insulin-Secreting Cells cytology, Luminescent Proteins chemistry, Luminescent Proteins genetics, Luminescent Proteins metabolism, Mice, Mice, Inbred C57BL, Mice, Transgenic, Mitochondrial Dynamics, NF-E2-Related Factor 2 antagonists & inhibitors, NF-E2-Related Factor 2 genetics, NF-E2-Related Factor 2 metabolism, Nuclear Proteins chemistry, Nuclear Proteins genetics, Organelle Biogenesis, Oxygen Consumption, Protein Subunits chemistry, Protein Subunits genetics, Protein Subunits metabolism, RNA Interference, Rats, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Tissue Culture Techniques, Transcription Factors chemistry, Transcription Factors genetics, Basic Helix-Loop-Helix Leucine Zipper Transcription Factors metabolism, Gene Expression Regulation, Glucose metabolism, Insulin-Secreting Cells metabolism, NF-E2-Related Factor 2 agonists, Nuclear Proteins metabolism, Transcription Factors metabolism

Abstract

Patients with both major forms of diabetes would benefit from therapies that increase β-cell mass. Glucose, a natural mitogen, drives adaptive expansion of β-cell mass by promoting β-cell proliferation. We previously demonstrated that a carbohydrate response element-binding protein (ChREBPα) is required for glucose-stimulated β-cell proliferation and that overexpression of ChREBPα amplifies the proliferative effect of glucose. Here we found that ChREBPα reprogrammed anabolic metabolism to promote proliferation. ChREBPα increased mitochondrial biogenesis, oxygen consumption rates, and ATP production. Proliferation augmentation by ChREBPα required the presence of ChREBPβ. ChREBPα increased the expression and activity of Nrf2, initiating antioxidant and mitochondrial biogenic programs. The induction of Nrf2 was required for ChREBPα-mediated mitochondrial biogenesis and for glucose-stimulated and ChREBPα-augmented β-cell proliferation. Overexpression of Nrf2 was sufficient to drive human β-cell proliferation in vitro; this confirms the importance of this pathway. Our results reveal a novel pathway necessary for β-cell proliferation that may be exploited for therapeutic β-cell regeneration., (© 2018 by the American Diabetes Association.)

Published

2018

16. Proteasome-mediated protein degradation is enhanced by fusion ubiquitin with unstructured degron.

Author

Inobe T, Tsukamoto M, and Nozaki M

Subjects

HEK293 Cells, Humans, Polyubiquitin metabolism, Saccharomyces cerevisiae metabolism, Ubiquitination, DNA-Binding Proteins metabolism, Proteasome Endopeptidase Complex metabolism, Proteolysis, Recombinant Fusion Proteins metabolism, Saccharomyces cerevisiae Proteins metabolism, Transcription Factors metabolism, Ubiquitin metabolism

Abstract

Methods to induce proteasomal degradation of unwanted proteins are valuable in biomedical studies and thus receive increasing attention. For efficient degradation, the proteasome requires both a ubiquitin tag, which delivers substrates to the proteasome, and an unstructured region, where the proteasome engages the substrate for unfolding and degradation. We fused two degron components into a single molecule to create a fusion protein comprising ubiquitin and Rpn4-derived unstructured region. We demonstrated that the fusion protein retained its function to polyubiquitinate target proteins, thereby inducing more efficient proteasomal target degradation than wild-type ubiquitin in vitro and in cells. These results provide novel strategies for robust degradation enhancement of polyubiquitinated proteins., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2018

17. Engineering the Ultrasensitive Transcription Factors by Fusing a Modular Oligomerization Domain.

Author

Hou J, Zeng W, Zong Y, Chen Z, Miao C, Wang B, and Lou C

Subjects

Allosteric Regulation drug effects, Bacterial Proteins genetics, Escherichia coli drug effects, Escherichia coli genetics, Escherichia coli growth & development, Escherichia coli Proteins genetics, Feedback, Physiological, Gene Regulatory Networks, Isopropyl Thiogalactoside pharmacology, Lac Repressors genetics, Ligands, Multidrug Resistance-Associated Proteins genetics, Promoter Regions, Genetic, Protein Domains, Protein Multimerization, Recombinant Fusion Proteins metabolism, Repressor Proteins genetics, Transcription Factors chemistry, Protein Engineering methods, Recombinant Fusion Proteins genetics, Transcription Factors genetics, Transcription Factors metabolism

Abstract

The dimerization and high-order oligomerization of transcription factors has endowed them with cooperative regulatory capabilities that play important roles in many cellular functions. However, such advanced regulatory capabilities have not been fully exploited in synthetic biology and genetic engineering. Here, we engineered a C-terminally fused oligomerization domain to improve the cooperativity of transcription factors. First, we found that two of three designed oligomerization domains significantly increased the cooperativity and ultrasensitivity of a transcription factor for the regulated promoter. Then, seven additional transcription factors were used to assess the modularity of the oligomerization domains, and their ultrasensitivity was generally improved, as assessed by their Hill coefficients. Moreover, we also demonstrated that the allosteric capability of the ligand-responsive domain remained intact when fusing with the designed oligomerization domain. As an example application, we showed that the engineered ultrasensitive transcription factor could be used to significantly improve the performance of a "stripe-forming" gene circuit. We envision that the oligomerization modules engineered in this study could act as a powerful tool to rapidly tune the underlying response profiles of synthetic gene circuits and metabolic pathway controllers.

Published

2018

18. Supramolecular assembly of the beta-catenin destruction complex and the effect of Wnt signaling on its localization, molecular size, and activity in vivo.

Author

Schaefer KN, Bonello TT, Zhang S, Williams CE, Roberts DM, McKay DJ, and Peifer M

Subjects

Animals, Animals, Genetically Modified, Apc1 Subunit, Anaphase-Promoting Complex-Cyclosome chemistry, Apc1 Subunit, Anaphase-Promoting Complex-Cyclosome genetics, Apc1 Subunit, Anaphase-Promoting Complex-Cyclosome metabolism, Armadillo Domain Proteins chemistry, Armadillo Domain Proteins genetics, Axin Protein chemistry, Axin Protein genetics, Axin Protein metabolism, Axin Signaling Complex chemistry, Axin Signaling Complex genetics, Cell Line, Drosophila Proteins chemistry, Drosophila Proteins genetics, Drosophila melanogaster embryology, Drosophila melanogaster genetics, Drosophila melanogaster metabolism, Glycogen Synthase Kinase 3 genetics, Glycogen Synthase Kinase 3 metabolism, Multiprotein Complexes chemistry, Multiprotein Complexes genetics, Multiprotein Complexes metabolism, Proteolysis, RNA, Messenger genetics, RNA, Messenger metabolism, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Transcription Factors chemistry, Transcription Factors genetics, Transcription, Genetic, Tumor Suppressor Proteins chemistry, Tumor Suppressor Proteins genetics, Tumor Suppressor Proteins metabolism, Wnt1 Protein genetics, Wnt1 Protein metabolism, Armadillo Domain Proteins metabolism, Axin Signaling Complex metabolism, Drosophila Proteins metabolism, Transcription Factors metabolism, Wnt Signaling Pathway

Abstract

Wnt signaling provides a paradigm for cell-cell signals that regulate embryonic development and stem cell homeostasis and are inappropriately activated in cancers. The tumor suppressors APC and Axin form the core of the multiprotein destruction complex, which targets the Wnt-effector beta-catenin for phosphorylation, ubiquitination and destruction. Based on earlier work, we hypothesize that the destruction complex is a supramolecular entity that self-assembles by Axin and APC polymerization, and that regulating assembly and stability of the destruction complex underlie its function. We tested this hypothesis in Drosophila embryos, a premier model of Wnt signaling. Combining biochemistry, genetic tools to manipulate Axin and APC2 levels, advanced imaging and molecule counting, we defined destruction complex assembly, stoichiometry, and localization in vivo, and its downregulation in response to Wnt signaling. Our findings challenge and revise current models of destruction complex function. Endogenous Axin and APC2 proteins and their antagonist Dishevelled accumulate at roughly similar levels, suggesting competition for binding may be critical. By expressing Axin:GFP at near endogenous levels we found that in the absence of Wnt signals, Axin and APC2 co-assemble into large cytoplasmic complexes containing tens to hundreds of Axin proteins. Wnt signals trigger recruitment of these to the membrane, while cytoplasmic Axin levels increase, suggesting altered assembly/disassembly. Glycogen synthase kinase3 regulates destruction complex recruitment to the membrane and release of Armadillo/beta-catenin from the destruction complex. Manipulating Axin or APC2 levels had no effect on destruction complex activity when Wnt signals were absent, but, surprisingly, had opposite effects on the destruction complex when Wnt signals were present. Elevating Axin made the complex more resistant to inactivation, while elevating APC2 levels enhanced inactivation. Our data suggest both absolute levels and the ratio of these two core components affect destruction complex function, supporting models in which competition among Axin partners determines destruction complex activity.

Published

2018

19. Plant Temperature Acclimation and Growth Rely on Cytosolic Ribosome Biogenesis Factor Homologs.

Author

Beine-Golovchuk O, Firmino AAP, Dąbrowska A, Schmidt S, Erban A, Walther D, Zuther E, Hincha DK, and Kopka J

Subjects

Arabidopsis Proteins genetics, Cytosol metabolism, Gene Expression Regulation, Plant, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Mutation, Plant Leaves physiology, Plants, Genetically Modified, RNA, Ribosomal genetics, RNA, Ribosomal metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Ribosomes genetics, Temperature, Transcription Factors genetics, Acclimatization physiology, Arabidopsis physiology, Arabidopsis Proteins metabolism, Ribosomes metabolism, Transcription Factors metabolism

Abstract

Arabidopsis ( Arabidopsis thaliana ) REI1-LIKE (REIL) proteins, REIL1 and REIL2, are homologs of a yeast ribosome biogenesis factor that participates in late cytoplasmic 60S ribosomal subunit maturation. Here, we report that the inhibited growth of the reil1-1 reil2-1 mutant at 10°C can be rescued by the expression of amino-terminal FLUORESCENT PROTEIN (FP)-REIL fusions driven by the UBIQUITIN10 promoter, allowing the analysis of REIL function in planta. Arabidopsis REIL1 appears to be functionally conserved, based on the cytosolic localization of FP-REIL1 and the interaction of native REIL1 with the 60S subunit in wild-type plants. In contrast to its yeast homologs, REIL1 also was present in translating ribosome fractions. Systems analysis revealed that wild-type Arabidopsis remodels the cytosolic translation machinery when grown at 10°C by accumulating cytosolic ribosome subunits and inducing the expression of cytosolic ribosomal RNA, ribosomal genes, ribosome biogenesis factors, and translation initiation or elongation factors. In the reil1-1 reil2-1 mutant, all processes associated with inhibited growth were delayed, although the plants maintained cellular integrity or acquired freezing tolerance. REIL proteins also were implicated in plant-specific processes: nonacclimated reil1-1 reil2-1 exhibited cold-acclimation responses, including activation of the DREB/CBF regulon. In addition, acclimated reil1-1 reil2-1 plants failed to activate FLOWERING LOCUS T expression in mature leaves. Therefore, in the wild type, REIL function may contribute to temperature perception by suppressing premature cold responses during growth at nonstressful temperatures. In conclusion, we suggest that Arabidopsis REIL proteins influence cold-induced plant ribosome remodeling and enhance the accumulation of cytosolic ribosome subunits after cold shift either by de novo synthesis or by recycling them from the translating ribosome fraction., (© 2018 American Society of Plant Biologists. All Rights Reserved.)

Published

2018

20. Development of cyclic AMP receptor protein-based artificial transcription factor for intensifying gene expression.

Author

Zhao P, Wang W, and Tian P

Subjects

Aldehyde Dehydrogenase biosynthesis, Chromatography, High Pressure Liquid, Cyclic AMP Receptor Protein genetics, DNA-Directed RNA Polymerases metabolism, Electrophoresis, Polyacrylamide Gel, Glyceraldehyde analogs & derivatives, Glyceraldehyde metabolism, Klebsiella pneumoniae genetics, Klebsiella pneumoniae metabolism, Lac Repressors genetics, Lactic Acid analogs & derivatives, Lactic Acid metabolism, Operator Regions, Genetic, Propane metabolism, Protein Binding, Recombinant Fusion Proteins genetics, Transcription Factors genetics, Cyclic AMP Receptor Protein metabolism, Gene Expression, Lac Repressors metabolism, Recombinant Fusion Proteins metabolism, Transcription Factors metabolism

Abstract

Vector-dependent gene overexpression typically relies on an efficient operon and sufficient RNA polymerases (RNAPs). The lac (lactose) operon is a paradigm of transcription control, and cyclic AMP receptor protein (CRP) is a global regulator capable of recruiting RNAPs. However, the gap between lac operon and CRP has not been well bridged. In this work, CRP was fused to lac repressor protein (lacI) to form an artificial transcription factor (ATF) with the expectation that when LacI acted on the lacO-positioned upstream of gene of interest, the LacI-tethered CRP would trap RNAPs and thus improve the expression of PuuC, an aldehyde dehydrogenase catalyzing 3-hydroxypropionaldehyde (3-HPA) to 3-hydroxypropionic acid (3-HP) in Klebsiella pneumoniae. As expected, SDS-PAGE and HPLC showed enhanced PuuC expression and 3-HP production, respectively, compared to the control strain without expressing chimeric protein LacI-CRP. Moreover, quantitative real-time PCR demonstrated increased transcription levels of both PuuC and RNAP coding genes. In shake-flask cultivation, the recombinant K. pneumoniae strain coexpressing LacI-CRP and PuuC produced 1.67-fold of 3-HP relative to the stain only overexpressing PuuC. In bioreactor cultivation, the strain coexpressing LacI-CRP and PuuC produced 35.1 g/L 3-HP, whereas the strain without expressing LacI-CRP generated only 9.8 g/L 3-HP. Overall, these results indicated that as an ATF, LacI-CRP significantly boosted PuuC expression and 3-HP production. We envision that LacI-CRP as a plug-and-play part can be used for regulating gene expression.

Published

2018

21. Rapid and Quantitative CELD Assay to Measure the Specificity of Transcription Factor-DNA-Binding Interactions and Identify cis-Elements.

Author

Kalaipandian S and Xue GP

Subjects

Amino Acid Sequence, Binding Sites, Biotinylation, DNA Probes metabolism, DNA-Binding Proteins chemistry, Escherichia coli metabolism, Histidine metabolism, Oligopeptides metabolism, Promoter Regions, Genetic genetics, Protein Binding, Recombinant Fusion Proteins metabolism, Solutions, Transcription Factors chemistry, Cellulase metabolism, DNA-Binding Proteins metabolism, Molecular Biology methods, Regulatory Sequences, Nucleic Acid genetics, Transcription Factors metabolism

Abstract

Specific interaction between transcription factor (TF) and cis-regulatory elements in the context of chromatin is the key to determining gene expression. Thus, it is important to measure DNA-binding specificity and identify cis-elements of TFs of your interest. In this chapter, we described a microwell-based assay to determine DNA-binding specificity by using translational fusion of a TF with a highly active cellulase (CELD), which hydrolyzes 4-methylumbelliferyl β-D-cellobioside to a fluorescent 4-methylumbelliferone product. The hydrolysis activity arrows us to quantify the binding strength between TF-CELD fusion protein and biotinylated DNA sequences in a 96-well microplate. The high-throughput and quantitative nature of CELD assay enable researchers to test a large number of putative DNA-binding sites of TFs, which subsequently leads to the identification of its direct target genes.

Published

2018

22. LMO7 exerts an effect on mitosis progression and the spindle assembly checkpoint.

Author

Tzeng YW, Li DY, Chen Y, Yang CH, Chang CY, and Juang YL

Subjects

Animals, Cell Cycle Proteins chemistry, Cell Cycle Proteins genetics, Cell Line, Tumor, Humans, Interphase, Kinetochores metabolism, LIM Domain Proteins antagonists & inhibitors, LIM Domain Proteins chemistry, LIM Domain Proteins genetics, Luminescent Proteins chemistry, Luminescent Proteins genetics, Luminescent Proteins metabolism, Metaphase, Nuclear Proteins chemistry, Nuclear Proteins genetics, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Prometaphase, Protein Domains, Protein Multimerization, Protein Transport, RNA Interference, Rats, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Spindle Poles metabolism, Transcription Factors antagonists & inhibitors, Transcription Factors chemistry, Transcription Factors genetics, Actin Cytoskeleton metabolism, Cell Cycle Proteins metabolism, Cell Membrane metabolism, LIM Domain Proteins metabolism, M Phase Cell Cycle Checkpoints, Mitosis, Nuclear Proteins metabolism, Transcription Factors metabolism

Abstract

LMO7 (LIM domain only 7) is a transcription regulator for expression of many Emery-Dreifuss muscular dystrophy-relevant genes, and binds to α-actinin and AF6/afadin at adherens junctions for epithelial cell-cell adhesion. In this study, we found that human LMO7 interacted with the spindle assembly checkpoint (SAC) protein MAD1. LMO7 colocalized with actin filaments at the cell membrane but did not colocalize with MAD1 at kinetochores in prometaphase. Our observations reveal that overexpression but not depletion of LMO7 caused a SAC defect, and that the LIM domain of LMO7 was a determinant of its ability to interfere with kinetochore localization of the SAC proteins MAD2 and BUBR1 and cause a SAC defect though the LIM peptide itself did neither bind to MAD1, MAD2 and BUBR1 nor localize to the actin filaments. However, overexpression of LMO7 or the LIM peptide did not interfere with kinetochore localization of MAD1. Additionally, overexpression of the LIM peptide prolonged mitotic timing and interfered with chromosome congression whereas that of LMO7b did not. Taken together, we conclude that LMO7 via its LIM domain acts to control mitosis progression and exerts an effect on the SAC., (Copyright © 2017 Elsevier Ltd. All rights reserved.)

Published

2018

23. HIV-1 Vpr protein directly loads helicase-like transcription factor (HLTF) onto the CRL4-DCAF1 E3 ubiquitin ligase.

Author

Zhou X, DeLucia M, Hao C, Hrecka K, Monnie C, Skowronski J, and Ahn J

Subjects

Binding Sites, Carrier Proteins antagonists & inhibitors, Carrier Proteins chemistry, Carrier Proteins genetics, Cell Line, Tumor, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, Dimerization, Gene Deletion, HEK293 Cells, Humans, Oligopeptides chemistry, Oligopeptides genetics, Oligopeptides metabolism, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Point Mutation, Protein Interaction Domains and Motifs, Protein Multimerization, Protein Serine-Threonine Kinases, RNA Interference, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Transcription Factors chemistry, Transcription Factors genetics, Ubiquitin-Protein Ligases antagonists & inhibitors, Ubiquitin-Protein Ligases chemistry, Ubiquitin-Protein Ligases genetics, Ubiquitination, WD40 Repeats, vpr Gene Products, Human Immunodeficiency Virus chemistry, vpr Gene Products, Human Immunodeficiency Virus genetics, Carrier Proteins metabolism, DNA-Binding Proteins metabolism, Models, Molecular, Proteasome Endopeptidase Complex metabolism, Transcription Factors metabolism, Ubiquitin-Protein Ligases metabolism, vpr Gene Products, Human Immunodeficiency Virus metabolism

Abstract

The viral protein R (Vpr) is an accessory virulence factor of HIV-1 that facilitates infection in immune cells. Cellular functions of Vpr are tied to its interaction with DCAF1, a substrate receptor component of the CRL4 E3 ubiquitin ligase. Recent proteomic approaches suggested that Vpr degrades helicase-like transcription factor (HLTF) DNA helicase in a proteasome-dependent manner by redirecting the CRL4-DCAF1 E3 ligase. However, the precise molecular mechanism of Vpr-dependent HLTF depletion is not known. Here, using in vitro reconstitution assays, we show that Vpr mediates polyubiquitination of HLTF, by directly loading it onto the C-terminal WD40 domain of DCAF1 in complex with the CRL4 E3 ubiquitin ligase. Mutational analyses suggest that Vpr interacts with DNA-binding residues in the N-terminal HIRAN domain of HLTF in a manner similar to the recruitment of another target, uracil DNA glycosylase (UNG2), to the CRL4-DCAF1 E3 by Vpr. Strikingly, Vpr also engages a second, adjacent region, which connects the HIRAN and ATPase/helicase domains. Thus, our findings reveal that Vpr utilizes common as well as distinctive interfaces to recruit multiple postreplication DNA repair proteins to the CRL4-DCAF1 E3 ligase for ubiquitin-dependent proteasomal degradation., (© 2017 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2017

24. Cleavage of osmosensitive transcriptional factor NFAT5 by Coxsackieviral protease 2A promotes viral replication.

Author

Qiu Y, Ye X, Zhang HM, Hanson P, Zhao G, Tong L, Xie R, and Yang D

Subjects

Amino Acid Substitution, Animals, Cell Line, Coxsackievirus Infections immunology, Coxsackievirus Infections metabolism, Coxsackievirus Infections pathology, Enterovirus B, Human immunology, Enterovirus B, Human physiology, Gene Expression Regulation, Humans, Male, Mice, Inbred A, Mutation, Myocarditis immunology, Myocarditis metabolism, Myocarditis pathology, Myocytes, Cardiac immunology, Myocytes, Cardiac metabolism, Myocytes, Cardiac pathology, Nitric Oxide Synthase Type II antagonists & inhibitors, Nitric Oxide Synthase Type II chemistry, Nitric Oxide Synthase Type II genetics, Nitric Oxide Synthase Type II metabolism, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Proteolysis, RNA Interference, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Substrate Specificity, Transcription Factors antagonists & inhibitors, Transcription Factors chemistry, Transcription Factors genetics, Virus Replication, Coxsackievirus Infections virology, Cysteine Endopeptidases metabolism, Enterovirus B, Human enzymology, Myocarditis virology, Myocytes, Cardiac virology, Transcription Factors metabolism, Viral Proteins metabolism

Abstract

Nuclear factor of activated T cells 5 (NFAT5)/Tonicity enhancer binding protein (TonEBP) is a transcription factor induced by hypertonic stress in the kidney. However, the function of NFAT5 in other organs has rarely been studied, even though it is ubiquitously expressed. Indeed, although NFAT5 was reported to be critical for heart development and function, its role in infectious heart diseases has remained obscure. In this study, we aimed to understand the mechanism by which NFAT5 interferes with infection of Coxsackievirus B3 (CVB3), a major cause of viral myocarditis. Our initial results demonstrated that although the mRNA level of NFAT5 remained constant during CVB3 infection, NFAT5 protein level decreased because the protein was cleaved. Bioinformatic prediction and verification of the predicted site by site-directed mutagenesis experiments determined that the NFAT5 protein was cleaved by CVB3 protease 2A at Glycine 503. Such cleavage led to the inactivation of NFAT5, and the 70-kDa N-terminal cleavage product (p70-NFAT5) exerted a dominant negative effect on the full-length NFAT5 protein. We further showed that elevated expression of NFAT5 to counteract viral protease cleavage, especially overexpression of a non-cleavable mutant of NFAT5, significantly inhibited CVB3 replication. Ectopic expression of NFAT5 resulted in elevated expression of inducible nitric oxide synthase (iNOS), a factor reported to inhibit CVB3 replication. The necessity of iNOS for the anti-CVB3 effect of NFAT5 was supported by the observation that inhibition of iNOS blocked the anti-CVB3 effect of NFAT5. In a murine model of viral myocarditis, we observed that treatment with hypertonic saline or mannitol solution upregulated NFAT5 and iNOS expression, inhibited CVB3 replication and reduced tissue damage in the heart. Taken together, our data demonstrate that the anti-CVB3 activity of NFAT5 is impaired during CVB3 infection due to 2A-mediated cleavage of NFAT5. Thus induction of NFAT5 by hypertonic agents may be a promising strategy for the development of anti-CVB3 therapeutics.

Published

2017

25. Inducible somatic embryogenesis in Theobroma cacao achieved using the DEX-activatable transcription factor-glucocorticoid receptor fusion.

Author

Shires ME, Florez SL, Lai TS, and Curtis WR

Subjects

Cacao drug effects, Enzyme Activation, Gene Expression Regulation, Developmental drug effects, Gene Expression Regulation, Plant drug effects, Plant Proteins genetics, Plant Proteins metabolism, Plant Somatic Embryogenesis Techniques, Plants, Genetically Modified, Receptors, Glucocorticoid metabolism, Recombinant Fusion Proteins metabolism, Transcription Factors metabolism, Cacao embryology, Dexamethasone pharmacology, Receptors, Glucocorticoid genetics, Transcription Factors genetics

Abstract

Objectives: To carry out mass propagation of superior plants to improve agricultural and silvicultural production though advancements in plant cell totipotency, or the ability of differentiated somatic plant cells to regenerate an entire plant., Results: The first demonstration of a titratable control over somatic embryo formation in a commercially relevant plant, Theobroma cacao (Chocolate tree), was achieved using a dexamethasone activatable chimeric transcription factor. This four-fold enhancement in embryo production rate utilized a glucocorticoid receptor fused to an embryogenic transcription factor LEAFY COTYLEDON 2. Where previous T. cacao somatic embryogenesis has been restricted to dissected flower parts, this construct confers an unprecedented embryogenic potential to leaves., Conclusions: Activatable chimeric transcription factors provide a means for elucidating the regulatory cascade associated with plant somatic embryogenesis towards improving its use for somatic regeneration of transgenics and plant propagation.

Published

2017

26. Metabolically Derived Lysine Acylations and Neighboring Modifications Tune the Binding of the BET Bromodomains to Histone H4.

Author

Olp MD, Zhu N, and Smith BC

Subjects

Acylation, Animals, Cell Cycle Proteins, Cell Line, Chickens, Histones chemistry, Ligands, Lysine metabolism, Methylation, Molecular Docking Simulation, Nuclear Proteins chemistry, Nuclear Proteins genetics, Nucleosomes, Oligopeptides chemistry, Oligopeptides genetics, Oligopeptides metabolism, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Phosphorylation, Protein Array Analysis, Protein Interaction Domains and Motifs, Protein Serine-Threonine Kinases chemistry, Protein Serine-Threonine Kinases genetics, RNA-Binding Proteins chemistry, RNA-Binding Proteins genetics, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Transcription Factors chemistry, Transcription Factors genetics, Histones metabolism, Models, Molecular, Nuclear Proteins metabolism, Protein Processing, Post-Translational, Protein Serine-Threonine Kinases metabolism, RNA-Binding Proteins metabolism, Transcription Factors metabolism

Abstract

Recent proteomic studies discovered histone lysines are modified by acylations beyond acetylation. These acylations derive from acyl-CoA metabolites, potentially linking metabolism to transcription. Bromodomains bind lysine acylation on histones and other nuclear proteins to influence transcription. However, the extent bromodomains bind non-acetyl acylations is largely unknown. Also unclear are the effects of neighboring post-translational modifications, especially within heavily modified histone tails. Using peptide arrays, binding assays, sucrose gradients, and computational methods, we quantified 10 distinct acylations for binding to the bromodomain and extraterminal domain (BET) family. Four of these acylations (hydroxyisobutyrylation, malonylation, glutarylation, and homocitrullination) had never been tested for bromodomain binding. We found N-terminal BET bromodomains bound acetylated and propionylated peptides, consistent with previous studies. Interestingly, all other acylations inhibited binding of the BET bromodomains to peptides and nucleosomes. To understand how context tunes bromodomain binding, effects of neighboring methylation, phosphorylation, and acylation within histone H4 tails were determined. Serine 1 phosphorylation inhibited binding of the BRD4 N-terminal bromodomain to polyacetylated H4 tails by >5-fold, whereas methylation had no effect. Furthermore, binding of BRDT and BRD4 N-terminal bromodomains to H4K5acetyl was enhanced 1.4-9.5-fold by any neighboring acylation of lysine 8, indicating a secondary H4K8acyl binding site that is more permissive of non-acetyl acylations than previously appreciated. In contrast, C-terminal BET bromodomains exhibited 9.9-13.5-fold weaker binding for polyacylated than for monoacylated H4 tails, indicating the C-terminal bromodomains do not cooperatively bind multiple acylations. These results suggest acyl-CoA levels tune or block recruitment of the BET bromodomains to histones, linking metabolism to bromodomain-mediated transcription.

Published

2017

27. Quantitative Measurement and Thermodynamic Modeling of Fused Enhancers Support a Two-Tiered Mechanism for Interpreting Regulatory DNA.

Author

Samee MAH, Lydiard-Martin T, Biette KM, Vincent BJ, Bragdon MD, Eckenrode KB, Wunderlich Z, Estrada J, Sinha S, and DePace AH

Subjects

Animals, Animals, Genetically Modified, Binding Sites, Blastoderm embryology, Blastoderm metabolism, DNA metabolism, Drosophila Proteins metabolism, Drosophila melanogaster embryology, Drosophila melanogaster metabolism, Homeodomain Proteins metabolism, Lac Operon, Models, Genetic, Protein Binding, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Repressor Proteins metabolism, Thermodynamics, Transcription Factors metabolism, DNA genetics, Drosophila Proteins genetics, Drosophila melanogaster genetics, Enhancer Elements, Genetic, Gene Expression Regulation, Developmental, Homeodomain Proteins genetics, Repressor Proteins genetics, Transcription Factors genetics

Abstract

Computational models of enhancer function generally assume that transcription factors (TFs) exert their regulatory effects independently, modeling an enhancer as a "bag of sites." These models fail on endogenous loci that harbor multiple enhancers, and a "two-tier" model appears better suited: in each enhancer TFs work independently, and the total expression is a weighted sum of their expression readouts. Here, we test these two opposing views on how cis-regulatory information is integrated. We fused two Drosophila blastoderm enhancers, measured their readouts, and applied the above two models to these data. The two-tier mechanism better fits these readouts, suggesting that these fused enhancers comprise multiple independent modules, despite having sequence characteristics typical of single enhancers. We show that short-range TF-TF interactions are not sufficient to designate such modules, suggesting unknown underlying mechanisms. Our results underscore that mechanisms of how modules are defined and how their outputs are combined remain to be elucidated., (Copyright © 2017 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2017

28. Transcriptional regulation of the Nkx3.1 gene in prostate luminal stem cell specification and cancer initiation via its 3' genomic region.

Author

Xie Q and Wang ZA

Subjects

Adult Stem Cells cytology, Adult Stem Cells metabolism, Adult Stem Cells pathology, Androgens toxicity, Animals, Carcinogenesis chemically induced, Carcinogens toxicity, Cell Line, Cell Line, Tumor, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Homeodomain Proteins genetics, Humans, Male, Mice, Inbred C57BL, Mice, Transgenic, Orchiectomy, Prostate cytology, Prostate metabolism, Prostate pathology, Prostatic Neoplasms, Castration-Resistant chemically induced, Prostatic Neoplasms, Castration-Resistant metabolism, Prostatic Neoplasms, Castration-Resistant pathology, Receptors, Androgen chemistry, Receptors, Androgen metabolism, Recombinant Fusion Proteins metabolism, Response Elements drug effects, Transcription Factors genetics, 3' Untranslated Regions drug effects, Adult Stem Cells drug effects, Androgens pharmacology, Homeodomain Proteins metabolism, Prostate drug effects, Transcription Factors metabolism, Transcription, Genetic drug effects

Abstract

NK3 homeobox 1 (Nkx3.1), a transcription factor expressed in the prostate epithelium, is crucial for maintaining prostate cell fate and suppressing tumor initiation. Nkx3.1 is ubiquitously expressed in luminal cells of hormonally intact prostate but, upon androgen deprivation, exclusively labels a type of luminal stem cells named castration-resistant Nkx3.1-expressing cells (CARNs). During prostate cancer initiation, Nkx3.1 expression is frequently lost in both humans and mouse models. Therefore, investigating how Nkx3.1 expression is regulated in vivo is important for understanding the mechanisms of prostate stem cell specification and cancer initiation. Here, using a transgenic mouse line with destabilized GFP, we identified an 11-kb genomic region 3' of the Nkx3.1 transcription start site to be responsible for alterations in Nkx3.1 expression patterns under various physiological conditions. We found that androgen cell-autonomously activates Nkx3.1 expression through androgen receptor (AR) binding to the 11-kb region in both normal luminal cells and CARNs and discovered new androgen response elements in the Nkx3.1 3' UTR. In contrast, we found that, in Pten -/- prostate tumors, loss of Nkx3.1 expression is mediated at the transcriptional level through the 11-kb region despite functional AR in the nucleus. Importantly, the GFP reporter specifically labeled CARNs in the regressed prostate only in the presence of cell-autonomous AR, supporting a facultative model for CARN specification., (© 2017 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2017

29. Cellular requirements for iron-sulfur cluster insertion into the antiviral radical SAM protein viperin.

Author

Upadhyay AS, Stehling O, Panayiotou C, Rösser R, Lill R, and Överby AK

Subjects

Amino Acid Substitution, Apoproteins chemistry, Apoproteins genetics, Apoproteins metabolism, Carrier Proteins antagonists & inhibitors, Carrier Proteins chemistry, Carrier Proteins genetics, HEK293 Cells, Humans, Immunoprecipitation, Iron chemistry, Iron metabolism, Iron Radioisotopes, Iron-Sulfur Proteins chemistry, Iron-Sulfur Proteins genetics, Metallochaperones antagonists & inhibitors, Metallochaperones chemistry, Metallochaperones genetics, Metalloproteins, Mutation, Nuclear Proteins antagonists & inhibitors, Nuclear Proteins chemistry, Nuclear Proteins genetics, Oxidoreductases Acting on CH-CH Group Donors, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Protein Interaction Domains and Motifs, Proteins chemistry, Proteins genetics, RNA Interference, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Transcription Factors antagonists & inhibitors, Transcription Factors chemistry, Transcription Factors genetics, Carrier Proteins metabolism, Iron-Sulfur Proteins metabolism, Metallochaperones metabolism, Models, Biological, Nuclear Proteins metabolism, Proteins metabolism, Transcription Factors metabolism

Abstract

Viperin (RSAD2) is an interferon-stimulated antiviral protein that belongs to the radical S -adenosylmethionine (SAM) enzyme family. Viperin's iron-sulfur (Fe/S) cluster is critical for its antiviral activity against many different viruses. CIA1 (CIAO1), an essential component of the cytosolic iron-sulfur protein assembly (CIA) machinery, is crucial for Fe/S cluster insertion into viperin and hence for viperin's antiviral activity. In the CIA pathway, CIA1 cooperates with CIA2A, CIA2B, and MMS19 targeting factors to form various complexes that mediate the dedicated maturation of specific Fe/S recipient proteins. To date, however, the mechanisms of how viperin acquires its radical SAM Fe/S cluster to gain antiviral activity are poorly understood. Using co-immunoprecipitation and 55 Fe-radiolabeling experiments, we therefore studied the roles of CIA2A, CIA2B, and MMS19 for Fe/S cluster insertion. CIA2B and MMS19 physically interacted with the C terminus of viperin and used CIA1 as the primary viperin-interacting protein. In contrast, CIA2A bound to viperin's N terminus in a CIA1-, CIA2B-, and MMS19-independent fashion. Of note, the observed interaction of both CIA2 isoforms with a single Fe/S target protein is unprecedented in the CIA pathway. 55 Fe-radiolabeling experiments with human cells depleted of CIA1, CIA2A, CIA2B, or MMS19 revealed that CIA1, but none of the other CIA factors, is predominantly required for 55 Fe/S cluster incorporation into viperin. Collectively, viperin maturation represents a novel CIA pathway with a minimal requirement of the CIA-targeting factors and represents a new paradigm for the insertion of the Fe/S cofactor into a radical SAM protein., (© 2017 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2017

30. Yeast PAH1 -encoded phosphatidate phosphatase controls the expression of CHO1 -encoded phosphatidylserine synthase for membrane phospholipid synthesis.

Author

Han GS and Carman GM

Subjects

Basic Helix-Loop-Helix Transcription Factors genetics, CDPdiacylglycerol-Serine O-Phosphatidyltransferase chemistry, CDPdiacylglycerol-Serine O-Phosphatidyltransferase genetics, Gene Deletion, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Mutagenesis, Site-Directed, Mutation, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Phosphatidate Phosphatase chemistry, Phosphatidate Phosphatase genetics, Phospholipids metabolism, Promoter Regions, Genetic, Protein Transport, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Repressor Proteins genetics, Response Elements, Saccharomyces cerevisiae cytology, Saccharomyces cerevisiae enzymology, Saccharomyces cerevisiae growth & development, Saccharomyces cerevisiae physiology, Saccharomyces cerevisiae Proteins chemistry, Saccharomyces cerevisiae Proteins genetics, Transcription Factors genetics, Basic Helix-Loop-Helix Transcription Factors metabolism, CDPdiacylglycerol-Serine O-Phosphatidyltransferase metabolism, Gene Expression Regulation, Fungal, Models, Biological, Phosphatidate Phosphatase metabolism, Repressor Proteins metabolism, Saccharomyces cerevisiae Proteins metabolism, Transcription Factors metabolism

Abstract

The PAH1 -encoded phosphatidate phosphatase (PAP), which catalyzes the committed step for the synthesis of triacylglycerol in Saccharomyces cerevisiae , exerts a negative regulatory effect on the level of phosphatidate used for the de novo synthesis of membrane phospholipids. This raises the question whether PAP thereby affects the expression and activity of enzymes involved in phospholipid synthesis. Here, we examined the PAP-mediated regulation of CHO1 -encoded phosphatidylserine synthase (PSS), which catalyzes the committed step for the synthesis of major phospholipids via the CDP-diacylglycerol pathway. The lack of PAP in the pah1 Δ mutant highly elevated PSS activity, exhibiting a growth-dependent up-regulation from the exponential to the stationary phase of growth. Immunoblot analysis showed that the elevation of PSS activity results from an increase in the level of the enzyme encoded by CHO1 Truncation analysis and site-directed mutagenesis of the CHO1 promoter indicated that Cho1 expression in the pah1 Δ mutant is induced through the inositol-sensitive upstream activation sequence (UAS INO ), a cis -acting element for the phosphatidate-controlled Henry (Ino2-Ino4/Opi1) regulatory circuit. The abrogation of Cho1 induction and PSS activity by a CHO1 UAS INO mutation suppressed pah1 Δ effects on lipid synthesis, nuclear/endoplasmic reticulum membrane morphology, and lipid droplet formation, but not on growth at elevated temperature. Loss of the DGK1 -encoded diacylglycerol kinase, which converts diacylglycerol to phosphatidate, partially suppressed the pah1 Δ-mediated induction of Cho1 and PSS activity. Collectively, these data showed that PAP activity controls the expression of PSS for membrane phospholipid synthesis., (© 2017 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2017

31. A centrosomal protein FOR20 regulates microtubule assembly dynamics and plays a role in cell migration.

Author

Srivastava S and Panda D

Subjects

Animals, Brain Chemistry, Cell Line, Tumor, Cell Movement, Cilia ultrastructure, Epithelial Cells drug effects, Epithelial Cells metabolism, Epithelial Cells ultrastructure, Focal Adhesions drug effects, Focal Adhesions metabolism, Focal Adhesions ultrastructure, Gene Expression, Glutathione Transferase genetics, Glutathione Transferase metabolism, Goats, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, HeLa Cells, Humans, Mice, Microtubule-Associated Proteins genetics, Microtubule-Associated Proteins metabolism, Microtubules ultrastructure, NIH 3T3 Cells, Nocodazole pharmacology, Nuclear Proteins metabolism, Proteins metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Time-Lapse Imaging, Transcription Factors metabolism, Tubulin metabolism, Cilia metabolism, Microtubules metabolism, Nuclear Proteins genetics, Proteins genetics, Transcription Factors genetics, Tubulin genetics

Abstract

Here, we report that a centrosomal protein FOR20 [FOP (FGFR1 (fibroblast growth factor receptor 1) oncogene protein)-like protein of molecular mass of 20 kDa; also named as C16orf63, FLJ31153 or PHSECRG2] can regulate the assembly and stability of microtubules. Both FOR20 IgG antibody and GST (glutathione S -transferase)-tagged FOR20 could precipitate tubulin from the HeLa cell extract, indicating a possible interaction between FOR20 and tubulin. FOR20 was also detected in goat brain tissue extract and it cycled with microtubule-associated proteins. Furthermore, FOR20 bound to purified tubulin and inhibited the assembly of tubulin in vitro. The overexpression of FOR20 depolymerized interphase microtubules and the depletion of FOR20 prevented nocodazole-induced depolymerization of microtubules in HeLa cells. In addition, the depletion of FOR20 suppressed the dynamics of individual microtubules in live HeLa cells. FOR20-depleted MDA-MB-231 cells displayed zigzag motion and migrated at a slower rate than the control cells, indicating that FOR20 plays a role in directed cell migration. The results suggested that the centrosomal protein FOR20 is a new member of the microtubule-associated protein family and that it regulates the assembly and dynamics of microtubules., (© 2017 The Author(s). Published by Portland Press Limited on behalf of the Biochemical Society.)

Published

2017

32. Heterogeneous nuclear ribonucleoprotein K inhibits heat shock-induced transcriptional activity of heat shock factor 1.

Author

Kim HJ, Lee JJ, Cho JH, Jeong J, Park AY, Kang W, and Lee KJ

Subjects

Amino Acid Substitution, Animals, Cell Line, Tumor, Cystine metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Gene Expression Profiling, HEK293 Cells, HSP27 Heat-Shock Proteins genetics, HSP27 Heat-Shock Proteins metabolism, HSP70 Heat-Shock Proteins genetics, HSP70 Heat-Shock Proteins metabolism, Heat Shock Transcription Factors, Heat-Shock Proteins, Heterogeneous-Nuclear Ribonucleoprotein K antagonists & inhibitors, Heterogeneous-Nuclear Ribonucleoprotein K genetics, Hot Temperature adverse effects, Humans, Mice, Molecular Chaperones, Mutation, Oxidation-Reduction, RNA Interference, RNA, Messenger metabolism, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Ribonucleoproteins antagonists & inhibitors, Ribonucleoproteins genetics, Ribonucleoproteins metabolism, Transcription Factors genetics, Transcription Factors metabolism, DNA-Binding Proteins antagonists & inhibitors, Gene Expression Regulation, HSP27 Heat-Shock Proteins antagonists & inhibitors, HSP70 Heat-Shock Proteins antagonists & inhibitors, Heterogeneous-Nuclear Ribonucleoprotein K metabolism, Protein Processing, Post-Translational, Response Elements, Transcription Factors antagonists & inhibitors

Abstract

When cells are exposed to heat shock and various other stresses, heat shock factor 1 (HSF1) is activated, and the heat shock response (HSR) is elicited. To better understand the molecular regulation of the HSR, we used 2D-PAGE-based proteome analysis to screen for heat shock-induced post-translationally modified cellular proteins. Our analysis revealed that two protein spots typically present on 2D-PAGE gels and containing heterogeneous nuclear ribonucleoprotein K (hnRNP K) with trioxidized Cys 132 disappeared after the heat shock treatment and reappeared during recovery, but the total amount of hnRNP K protein remained unchanged. We next tested whether hnRNP K plays a role in HSR by regulating HSF1 and found that hnRNP K inhibits HSF1 activity, resulting in reduced expression of hsp70 and hsp27 mRNAs. hnRNP K also reduced binding affinity of HSF1 to the heat shock element by directly interacting with HSF1 but did not affect HSF1 phosphorylation-dependent activation or nuclear localization. hnRNP K lost its ability to induce these effects when its Cys 132 was substituted with Ser, Asp, or Glu. These findings suggest that hnRNP K inhibits transcriptional activity of HSF1 by inhibiting its binding to heat shock element and that the oxidation status of Cys 132 in hnRNP K is critical for this inhibition., (© 2017 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2017

33. Identification of Two Secondary Ligand Binding Sites in 14-3-3 Proteins Using Fragment Screening.

Author

Sijbesma E, Skora L, Leysen S, Brunsveld L, Koch U, Nussbaumer P, Jahnke W, and Ottmann C

Subjects

14-3-3 Proteins chemistry, 14-3-3 Proteins genetics, Acyltransferases, Amino Acid Sequence, Binding Sites, Biomarkers, Tumor chemistry, Biomarkers, Tumor genetics, Conserved Sequence, Crystallography, X-Ray, Exoribonucleases chemistry, Exoribonucleases genetics, Gene Deletion, Humans, Kinetics, Ligands, Nuclear Magnetic Resonance, Biomolecular, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Peptide Library, Phosphorylation, Protein Conformation, Protein Interaction Domains and Motifs, Protein Interaction Mapping, Protein Isoforms chemistry, Protein Isoforms genetics, Protein Isoforms metabolism, Protein Processing, Post-Translational, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Transcription Factors chemistry, Transcription Factors genetics, 14-3-3 Proteins metabolism, Biomarkers, Tumor metabolism, Exoribonucleases metabolism, Models, Molecular, Transcription Factors metabolism

Abstract

Proteins typically interact with multiple binding partners, and often different parts of their surfaces are employed to establish these protein-protein interactions (PPIs). Members of the class of 14-3-3 adapter proteins bind to several hundred other proteins in the cell. Multiple small molecules for the modulation of 14-3-3 PPIs have been disclosed; however, they all target the conserved phosphopeptide binding channel, so that selectivity is difficult to achieve. Here we report on the discovery of two individual secondary binding sites that have been identified by combining nuclear magnetic resonance-based fragment screening and X-ray crystallography. The two pockets that these fragments occupy are part of at least three physiologically relevant and structurally characterized 14-3-3 PPI interfaces, including those with serotonin N-acetyltransferase and plant transcription factor FT. In addition, the high degree of conservation of the two sites implies their relevance for 14-3-3 PPIs. This first identification of secondary sites on 14-3-3 proteins bound by small molecule ligands might facilitate the development of new chemical tool compounds for more selective PPI modulation.

Published

2017

34. Enhancer of rudimentary homologue interacts with scaffold attachment factor B at the nuclear matrix to regulate SR protein phosphorylation.

Author

Drakouli S, Lyberopoulou A, Papathanassiou M, Mylonis I, and Georgatsou E

Subjects

Active Transport, Cell Nucleus, Animals, Cell Cycle Proteins antagonists & inhibitors, Cell Cycle Proteins chemistry, Cell Cycle Proteins genetics, Cell Line, Tumor, Genes, Reporter, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, HEK293 Cells, Humans, Matrix Attachment Region Binding Proteins chemistry, Matrix Attachment Region Binding Proteins genetics, Microscopy, Fluorescence, Nuclear Matrix-Associated Proteins chemistry, Nuclear Matrix-Associated Proteins genetics, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Phosphorylation, Protein Interaction Domains and Motifs, Protein Multimerization, Protein Serine-Threonine Kinases antagonists & inhibitors, Protein Serine-Threonine Kinases chemistry, Protein Serine-Threonine Kinases genetics, RNA Interference, Rats, Receptors, Estrogen chemistry, Receptors, Estrogen genetics, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Serine-Arginine Splicing Factors chemistry, Transcription Factors antagonists & inhibitors, Transcription Factors chemistry, Transcription Factors genetics, Two-Hybrid System Techniques, Cell Cycle Proteins metabolism, Matrix Attachment Region Binding Proteins metabolism, Nuclear Matrix-Associated Proteins metabolism, Protein Processing, Post-Translational, Protein Serine-Threonine Kinases metabolism, Receptors, Estrogen metabolism, Serine-Arginine Splicing Factors metabolism, Transcription Factors metabolism

Abstract

Scaffold attachment factor B1 (SAFB1) is an integral component of the nuclear matrix of vertebrate cells. It binds to DNA on scaffold/matrix attachment region elements, as well as to RNA and a multitude of different proteins, affecting basic cellular activities such as transcription, splicing and DNA damage repair. In the present study, we show that enhancer of rudimentary homologue (ERH) is a new molecular partner of SAFB1 and its 70% homologous paralogue, scaffold attachment factor B2 (SAFB2). ERH interacts directly in the nucleus with the C-terminal Arg-Gly-rich region of SAFB1/2 and co-localizes with it in the insoluble nuclear fraction. ERH, a small ubiquitous protein with striking homology among species and a unique structure, has also been implicated in fundamental cellular mechanisms. Our functional analyses suggest that the SAFB/ERH interaction does not affect SAFB1/2 function in transcription (e.g. as oestrogen receptor α co-repressors), although it reverses the inhibition exerted by SAFB1/2 on the splicing kinase SR protein kinase 1 (SRPK1), which also binds on the C-terminus of SAFB1/2. Accordingly, ERH silencing decreases lamin B receptor and SR protein phosphorylation, which are major SRPK1 substrates, further substantiating the role of SAFB1 and SAFB2 in the co-ordination of nuclear function., (© 2017 Federation of European Biochemical Societies.)

Published

2017

35. Cell-surface copper transporters and superoxide dismutase 1 are essential for outgrowth during fungal spore germination.

Author

Plante S, Normant V, Ramos-Torres KM, and Labbé S

Subjects

Cation Transport Proteins genetics, Copper metabolism, Enzyme Activation, Gene Deletion, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Luminescent Proteins genetics, Luminescent Proteins metabolism, Microscopy, Fluorescence, Microscopy, Interference, Microscopy, Phase-Contrast, Protein Isoforms genetics, Protein Isoforms metabolism, Protein Transport, RNA, Fungal metabolism, RNA, Messenger metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, SLC31 Proteins, Schizosaccharomyces cytology, Schizosaccharomyces growth & development, Schizosaccharomyces metabolism, Schizosaccharomyces pombe Proteins genetics, Spores, Fungal cytology, Spores, Fungal growth & development, Spores, Fungal metabolism, Transcription Factors genetics, Red Fluorescent Protein, Cation Transport Proteins metabolism, Gene Expression Regulation, Fungal, Schizosaccharomyces physiology, Schizosaccharomyces pombe Proteins metabolism, Spores, Fungal physiology, Superoxide Dismutase-1 metabolism, Transcription Factors metabolism

Abstract

During fungal spore germination, a resting spore returns to a conventional mode of cell division and resumes vegetative growth, but the requirements for spore germination are incompletely understood. Here, we show that copper is essential for spore germination in Schizosaccharomyces pombe Germinating spores develop a single germ tube that emerges from the outer spore wall in a process called outgrowth. Under low-copper conditions, the copper transporters Ctr4 and Ctr5 are maximally expressed at the onset of outgrowth. In the case of Ctr6, its expression is broader, taking place before and during outgrowth. Spores lacking Ctr4, Ctr5, and the copper sensor Cuf1 exhibit complete germination arrest at outgrowth. In contrast, ctr6 deletion only partially interferes with formation of outgrowing spores. At outgrowth, Ctr4-GFP and Ctr5-Cherry first co-localize at the spore contour, followed by re-location to a middle peripheral spore region. Subsequently, they move away from the spore body to occupy the periphery of the nascent cell. After breaking of spore dormancy, Ctr6 localizes to the vacuole membranes that are enriched in the spore body relative to the germ tube. Using a copper-binding tracker, results showed that labile copper is preferentially localized to the spore body. Further analysis showed that Ctr4 and Ctr6 are required for copper-dependent activation of the superoxide dismutase 1 (SOD1) during spore germination. This activation is critical because the loss of SOD1 activity blocked spore germination at outgrowth. Taken together, these results indicate that cell-surface copper transporters and SOD1 are required for completion of the spore germination program., (© 2017 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2017

36. TRIM24 protein promotes and TRIM32 protein inhibits cardiomyocyte hypertrophy via regulation of dysbindin protein levels.

Author

Borlepawar A, Rangrez AY, Bernt A, Christen L, Sossalla S, Frank D, and Frey N

Subjects

Animals, Animals, Newborn, Apoptosis, Cardiomyopathy, Dilated pathology, Cardiomyopathy, Hypertrophic pathology, Carrier Proteins antagonists & inhibitors, Carrier Proteins genetics, Cells, Cultured, Dysbindin, Dystrophin-Associated Proteins chemistry, Dystrophin-Associated Proteins genetics, HEK293 Cells, Humans, Myocytes, Cardiac cytology, Myocytes, Cardiac pathology, Peptide Fragments chemistry, Peptide Fragments genetics, Peptide Fragments metabolism, Protein Stability, Proteolysis, RNA Interference, Rats, Rats, Wistar, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Serum Response Factor agonists, Serum Response Factor antagonists & inhibitors, Serum Response Factor genetics, Signal Transduction, Transcription Factors antagonists & inhibitors, Transcription Factors genetics, Tripartite Motif Proteins antagonists & inhibitors, Tripartite Motif Proteins genetics, Ubiquitin-Protein Ligases antagonists & inhibitors, Ubiquitin-Protein Ligases genetics, Cardiomyopathy, Dilated metabolism, Cardiomyopathy, Hypertrophic metabolism, Carrier Proteins metabolism, Dystrophin-Associated Proteins metabolism, Myocytes, Cardiac metabolism, Serum Response Factor metabolism, Transcription Factors metabolism, Tripartite Motif Proteins metabolism, Ubiquitin-Protein Ligases metabolism

Abstract

We have previously shown that dysbindin is a potent inducer of cardiomyocyte hypertrophy via activation of Rho-dependent serum-response factor (SRF) signaling. We have now performed a yeast two-hybrid screen using dysbindin as bait against a cardiac cDNA library to identify the cardiac dysbindin interactome. Among several putative binding proteins, we identified tripartite motif-containing protein 24 (TRIM24) and confirmed this interaction by co-immunoprecipitation and co-immunostaining. Another tripartite motif (TRIM) family protein, TRIM32, has been reported earlier as an E3 ubiquitin ligase for dysbindin in skeletal muscle. Consistently, we found that TRIM32 also degraded dysbindin in neonatal rat ventricular cardiomyocytes as well. Surprisingly, however, TRIM24 did not promote dysbindin decay but rather protected dysbindin against degradation by TRIM32. Correspondingly, TRIM32 attenuated the activation of SRF signaling and hypertrophy due to dysbindin, whereas TRIM24 promoted these effects in neonatal rat ventricular cardiomyocytes. This study also implies that TRIM32 is a key regulator of cell viability and apoptosis in cardiomyocytes via simultaneous activation of p53 and caspase-3/-7 and inhibition of X-linked inhibitor of apoptosis. In conclusion, we provide here a novel mechanism of post-translational regulation of dysbindin and hypertrophy via TRIM24 and TRIM32 and show the importance of TRIM32 in cardiomyocyte apoptosis in vitro ., (© 2017 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2017

37. Tracking Low-Copy Transcription Factors in Living Bacteria: The Case of the lac Repressor.

Author

Garza de Leon F, Sellars L, Stracy M, Busby SJW, and Kapanidis AN

Subjects

Cell Tracking, Chromosomes, Bacterial metabolism, Diffusion, Fluorescence, Genetic Loci, Microscopy, Recombinant Fusion Proteins metabolism, Subcellular Fractions metabolism, Escherichia coli metabolism, Gene Dosage, Lac Repressors metabolism, Microbial Viability, Transcription Factors metabolism

Abstract

Transcription factors control the expression of genes by binding to specific sites in DNA and repressing or activating transcription in response to stimuli. The lac repressor (LacI) is a well characterized transcription factor that regulates the ability of bacterial cells to uptake and metabolize lactose. Here, we study the intracellular mobility and spatial distribution of LacI in live bacteria using photoactivated localization microscopy combined with single-particle tracking. Since we track single LacI molecules in live cells by stochastically photoactivating and observing fluorescent proteins individually, there are no limitations on the copy number of the protein under study; as a result, we were able to study the behavior of LacI in bacterial strains containing the natural copy numbers (∼40 monomers), as well as in strains with much higher copy numbers due to LacI overexpression. Our results allowed us to determine the relative abundance of specific, near-specific, and non-specific DNA binding modes of LacI in vivo, showing that all these modes are operational inside living cells. Further, we examined the spatial distribution of LacI in live cells, confirming its specific binding to lac operator regions on the chromosome; we also showed that mobile LacI molecules explore the bacterial nucleoid in a way similar to exploration by other DNA-binding proteins. Our work also provides an example of applying tracking photoactivated localization microscopy to studies of low-copy-number proteins in living bacteria., (Copyright © 2017 Biophysical Society. Published by Elsevier Inc. All rights reserved.)

Published

2017

38. Myc inhibits JNK-mediated cell death in vivo.

Author

Huang J, Feng Y, Chen X, Li W, and Xue L

Subjects

Animals, Compound Eye, Arthropod cytology, Compound Eye, Arthropod embryology, Compound Eye, Arthropod growth & development, DNA-Binding Proteins deficiency, DNA-Binding Proteins genetics, Drosophila Proteins deficiency, Drosophila Proteins genetics, Drosophila melanogaster cytology, Female, Gene Expression Regulation, Developmental, Genes, Synthetic, Humans, Larva, Membrane Proteins genetics, Membrane Proteins physiology, Morphogenesis, Protein Isoforms genetics, Protein Isoforms physiology, Proto-Oncogene Mas, Proto-Oncogene Proteins c-myc genetics, Proto-Oncogene Proteins c-myc physiology, Recombinant Fusion Proteins metabolism, Species Specificity, Thorax cytology, Thorax embryology, Thorax growth & development, Transcription Factors deficiency, Transcription Factors genetics, Wings, Animal cytology, Wings, Animal embryology, Wings, Animal growth & development, Apoptosis genetics, DNA-Binding Proteins physiology, Drosophila Proteins physiology, Drosophila melanogaster genetics, Genes, myc, MAP Kinase Signaling System genetics, Transcription Factors physiology

Abstract

The proto-oncogene Myc is well known for its roles in promoting cell growth, proliferation and apoptosis. However, in this study, we found from a genetic screen that Myc inhibits, rather than promotes, cell death triggered by c-Jun N-terminal kinase (JNK) signaling in Drosophila. Firstly, expression of Drosophila Myc (dMyc) suppresses, whereas loss of dMyc enhances, ectopically activated JNK signaling-induced cell death. Secondly, dMyc impedes physiologically activated JNK pathway-mediated cell death. Thirdly, loss of dMyc triggers JNK pathway activation and JNK-dependent cell death. Finally, the mammalian cMyc gene, when expressed in Drosophila, impedes activated JNK signaling-induced cell death. Thus, besides its well-studied apoptosis promoting function, Myc also antagonizes JNK-mediated cell death in Drosophila, and this function is likely conserved from fly to human.

Published

2017

39. Real-Time Monitoring of nfxB Mutant Occurrence and Dynamics in Pseudomonas aeruginosa Biofilm Exposed to Subinhibitory Concentrations of Ciprofloxacin.

Author

Zaborskyte G, Andersen JB, Kragh KN, and Ciofu O

Subjects

Bacterial Proteins metabolism, Biofilms drug effects, Biofilms growth & development, DNA-Binding Proteins metabolism, Genes, Reporter, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Luminescent Proteins genetics, Luminescent Proteins metabolism, Membrane Proteins genetics, Membrane Proteins metabolism, Membrane Transport Proteins genetics, Membrane Transport Proteins metabolism, Microbial Sensitivity Tests, Microscopy, Confocal, Microscopy, Fluorescence, Pseudomonas aeruginosa drug effects, Pseudomonas aeruginosa growth & development, Pseudomonas aeruginosa metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Rheology, Selection, Genetic, Time-Lapse Imaging, Transcription Factors metabolism, Red Fluorescent Protein, Anti-Bacterial Agents pharmacology, Bacterial Proteins genetics, Ciprofloxacin pharmacology, DNA-Binding Proteins genetics, Drug Resistance, Bacterial genetics, Gene Expression Regulation, Bacterial, Mutation, Pseudomonas aeruginosa genetics, Transcription Factors genetics

Abstract

Biofilm infections caused by Pseudomonas aeruginosa are frequently treated with ciprofloxacin (CIP); however, resistance rapidly develops. One of the primary resistance mechanisms is the overexpression of the MexCD-OprJ pump due to a mutation in nfxB , encoding the transcriptional repressor of this pump. The aim of this study was to investigate the effect of subinhibitory concentrations of CIP on the occurrence of nfxB mutants in the wild-type PAO1 flow cell biofilm model. For this purpose, we constructed fluorescent reporter strains (PAO1 background) with an mCherry tag for constitutive red fluorescence and chromosomal transcriptional fusion between the P mexCD promoter and gfp leading to green fluorescence upon mutation of nfxB We observed a rapid development of nfxB mutants by live confocal laser scanning microscopy (CLSM) imaging of the flow cell biofilm (reaching 80 to 90% of the whole population) when treated with 1/10 minimal biofilm inhibitory concentration of CIP for 24 h and 96 h. Based on the observed developmental stages, we propose that nfxB mutants emerged de novo in the biofilm during CIP treatment from filamentous cells, which might have arisen due to the stress responses induced by CIP. Identical nfxB mutations were found in fluorescent colonies from the same flow cell biofilm, especially in 24-h biofilms, suggesting selection and clonal expansion of the mutants during biofilm growth. Our findings point at the significant role of high-enough antibiotic dosages or appropriate combination therapy to avoid the emergence of resistant mutants in biofilms., (Copyright © 2017 American Society for Microbiology.)

Published

2017

40. Identification of CASZ1 NES reveals potential mechanisms for loss of CASZ1 tumor suppressor activity in neuroblastoma.

Author

Liu Z, Lam N, Wang E, Virden RA, Pawel B, Attiyeh EF, Maris JM, and Thiele CJ

Subjects

Amino Acid Sequence, Binding Sites, Cell Line, Tumor, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, Gene Expression, Gene Expression Profiling, Gene Expression Regulation, Neoplastic, Humans, Intracellular Space metabolism, Mutation, Neuroblastoma genetics, Protein Binding, Protein Transport, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Transcription Factors chemistry, Transcription Factors genetics, Transcription, Genetic, Transcriptome, Tumor Suppressor Proteins chemistry, DNA-Binding Proteins metabolism, Neuroblastoma metabolism, Nuclear Export Signals, Transcription Factors metabolism, Tumor Suppressor Proteins metabolism

Abstract

As a transcription factor, localization to the nucleus and the recruitment of cofactors to regulate gene transcription is essential. Nuclear localization and nucleosome remodeling and histone deacetylase (NuRD) complex binding are required for the zinc-finger transcription factor CASZ1 to function as a neuroblastoma (NB) tumor suppressor. However, the critical amino acids (AAs) that are required for CASZ1 interaction with NuRD complex and the regulation of CASZ1 subcellular localization have not been characterized. Through alanine scanning, immunofluorescence cell staining and co-immunoprecipitation, we define a critical region at the CASZ1 N terminus (AAs 23-40) that mediates the CASZ1b nuclear localization and NuRD interaction. Furthermore, we identified a nuclear export signal (NES) at the N terminus (AAs 176-192) that contributes to CASZ1 nuclear-cytoplasmic shuttling in a chromosomal maintenance 1-dependent manner. An analysis of CASZ1 protein expression in a primary NB tissue microarray shows that high nuclear CASZ1 staining is detected in tumor samples from NB patients with good prognosis. In contrast, cytoplasmic-restricted CASZ1 staining or low nuclear CASZ1 staining is found in tumor samples from patients with poor prognosis. These findings provide insight into mechanisms by which CASZ1 regulates transcription, and suggests that regulation of CASZ1 subcellular localization may impact its function in normal development and pathologic conditions such as NB tumorigenesis., Competing Interests: The authors declare no conflict of interest.

Published

2017

41. Identification of Heat Shock Transcription Factor Genes Involved in Thermotolerance of Octoploid Cultivated Strawberry.

Author

Liao WY, Lin LF, Jheng JL, Wang CC, Yang JH, and Chou ML

Subjects

Amino Acid Sequence, Fragaria growth & development, Fragaria metabolism, Gene Expression Regulation, Plant, Heat Shock Transcription Factors, Heat-Shock Proteins metabolism, Hot Temperature, Plants, Genetically Modified genetics, Sequence Alignment, Stress, Physiological genetics, Arabidopsis genetics, DNA-Binding Proteins genetics, Fragaria genetics, Heat-Shock Response genetics, Recombinant Fusion Proteins metabolism, Thermotolerance genetics, Transcription Factors genetics

Abstract

Heat shock transcription factors (HSFs) are mainly involved in the activation of genes in response to heat stress as well as other abiotic and biotic stresses. The growth, development, reproduction, and yield of strawberry are strongly limited by extreme temperatures and droughts. In this study, we used Illumina sequencing and obtained transcriptome data set from Fragaria × ananassa Duchessne cv. Toyonoka. Six contigs and three unigenes were confirmed to encode HSF proteins (FaTHSFs). Subsequently, we characterized the biological functions of two particularly selected unigenes, FaTHSFA2a and FaTHSFB1a , which were classified into class A2 and B HSFs, respectively. Expression assays revealed that FaTHSFA2a and FaTHSFB1a expression was induced by heat shock and correlated well with elevated ambient temperatures. Overexpression of FaTHSFA2a and FaTHSFB1a resulted in the activation of their downstream stress-associated genes, and notably enhanced the thermotolerance of transgenic Arabidopsis plants. Besides, both FaTHSFA2a and FaTHSFB1a fusion proteins localized in the nucleus, indicating their similar subcellular distributions as transcription factors. Our yeast one-hybrid assay suggested that FaTHSFA2a has trans-activation activity, whereas FaTHSFB1a expresses trans-repression function. Altogether, our annotated transcriptome sequences provide a beneficial resource for identifying most genes expressed in octoploid strawberry. Furthermore, HSF studies revealed the possible insights into the molecular mechanisms of thermotolerance, thus rendering valuable molecular breeding to improve the tolerance of strawberry in response to high-temperature stress., Competing Interests: The authors declare no conflict of interest.

Published

2016

42. Molecular mechanism for sphingosine-induced Pseudomonas ceramidase expression through the transcriptional regulator SphR.

Author

Okino N and Ito M

Subjects

Bacterial Proteins genetics, Base Sequence, Ceramidases genetics, Ceramides pharmacology, Gene Deletion, Genes, Bacterial, Genes, araC, Hemolysis, Multigene Family, Promoter Regions, Genetic, Protein Array Analysis, Pseudomonas aeruginosa enzymology, Pseudomonas aeruginosa growth & development, RNA, Bacterial biosynthesis, RNA, Bacterial genetics, RNA, Messenger biosynthesis, RNA, Messenger genetics, Recombinant Fusion Proteins metabolism, Sequence Alignment, Sequence Homology, Nucleic Acid, Sphingomyelins metabolism, Sphingosine metabolism, Sphingosine pharmacology, Substrate Specificity, Transcription Factors deficiency, Transcription Factors genetics, Bacterial Proteins biosynthesis, Ceramidases biosynthesis, Gene Expression Regulation, Bacterial drug effects, Pseudomonas aeruginosa genetics, Transcription Factors physiology, Transcription, Genetic drug effects

Abstract

Pseudomonas aeruginosa, an opportunistic, but serious multidrug-resistant pathogen, secretes a ceramidase capable of cleaving the N-acyl linkage of ceramide to generate fatty acids and sphingosine. We previously reported that the secretion of P. aeruginosa ceramidase was induced by host-derived sphingolipids, through which phospholipase C-induced hemolysis was significantly enhanced. We herein investigated the gene(s) regulating sphingolipid-induced ceramidase expression and identified SphR, which encodes a putative AraC family transcriptional regulator. Disruption of the sphR gene in P. aeruginosa markedly decreased the sphingomyelin-induced secretion of ceramidase, reduced hemolytic activity, and resulted in the loss of sphingomyelin-induced ceramidase expression. A microarray analysis confirmed that sphingomyelin significantly induced ceramidase expression in P. aeruginosa. Furthermore, an electrophoretic mobility shift assay revealed that SphR specifically bound free sphingoid bases such as sphingosine, dihydrosphingosine, and phytosphingosine, but not sphingomyelin or ceramide. A β-galactosidase-assisted promoter assay showed that sphingosine activated ceramidase expression through SphR at a concentration of 100 nM. Collectively, these results demonstrated that sphingosine induces the secretion of ceramidase by promoting the mRNA expression of ceramidase through SphR, thereby enhancing hemolytic phospholipase C-induced cytotoxicity. These results facilitate understanding of the physiological role of bacterial ceramidase in host cells.

Published

2016

43. Single molecule tracking of Ace1p in Saccharomyces cerevisiae defines a characteristic residence time for non-specific interactions of transcription factors with chromatin.

Author

Ball DA, Mehta GD, Salomon-Kent R, Mazza D, Morisaki T, Mueller F, McNally JG, and Karpova TS

Subjects

DNA-Binding Proteins genetics, Heat-Shock Proteins genetics, Heat-Shock Proteins metabolism, Histones genetics, Histones metabolism, Metallothionein genetics, Metallothionein metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins genetics, Time Factors, Transcription Factors genetics, Chromatin metabolism, DNA-Binding Proteins analysis, DNA-Binding Proteins metabolism, Molecular Imaging methods, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins analysis, Saccharomyces cerevisiae Proteins metabolism, Transcription Factors analysis, Transcription Factors metabolism

Abstract

In vivo single molecule tracking has recently developed into a powerful technique for measuring and understanding the transient interactions of transcription factors (TF) with their chromatin response elements. However, this method still lacks a solid foundation for distinguishing between specific and non-specific interactions. To address this issue, we took advantage of the power of molecular genetics of yeast. Yeast TF Ace1p has only five specific sites in the genome and thus serves as a benchmark to distinguish specific from non-specific binding. Here, we show that the estimated residence time of the short-residence molecules is essentially the same for Hht1p, Ace1p and Hsf1p, equaling 0.12-0.32 s. These three DNA-binding proteins are very different in their structure, function and intracellular concentration. This suggests that (i) short-residence molecules are bound to DNA non-specifically, and (ii) that non-specific binding shares common characteristics between vastly different DNA-bound proteins and thus may have a common underlying mechanism. We develop new and robust procedure for evaluation of adverse effects of labeling, and new quantitative analysis procedures that significantly improve residence time measurements by accounting for fluorophore blinking. Our results provide a framework for the reliable performance and analysis of single molecule TF experiments in yeast., (Published by Oxford University Press on behalf of Nucleic Acids Research 2016. This work is written by (a) US Government employee(s) and is in the public domain in the US.)

Published

2016

44. Grass carp reovirus NS26 interacts with cellular lipopolysaccharide-induced tumor necrosis factor-alpha factor, LITAF.

Author

Lu J, Wang H, Zhang Y, Li Y, and Lu L

Subjects

Animals, Cell Line, Cells, Cultured, Protein Binding, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins metabolism, Carps, Fish Diseases metabolism, Fish Diseases virology, Host-Pathogen Interactions, Nuclear Proteins metabolism, Reoviridae physiology, Transcription Factors metabolism, Viral Nonstructural Proteins metabolism

Abstract

The nonstructural protein NS26 of grass carp reovirus (GCRV) is encoded by the 11th genomic dsRNA segment, homolog of which is not found in orthoreoviruses. The role of NS26 in GCRV pathogenesis is still unclear. Previously, grass carp LITAF/SIMPLE protein was identified as a putative binding partner for NS26 in a yeast two-hybrid screen. Here, we further characterized the association between NS26 and LITAF using in vivo and in vitro protein interaction assays. Soluble GST-NS26 and His 6 -LITAF were expressed and purified from E. coli; recombinant NS26 tagged with myc and LITAF tagged with GFP were expressed in Ctenopharyngon idellus kidney cells (CIK) by transient transfection experiments. A GST pulldown assay demonstrated that GST-tagged NS26 efficiently bound to His 6 -LITAF. Co-immunoprecipitation assays demonstrated that GCRV NS26 reciprocally precipitated endogenous LITAF in CIK cells. Double-immunofluorescent analyses revealed myc-NS26 colocalized with GFP-LITAF in CIK cells. Taken together, the current in vitro and in vivo data demonstrated the interaction between cellular LITAF and GCRV NS26.

Published

2016

45. The AAA ATPase MDN1 Acts as a SUMO-Targeted Regulator in Mammalian Pre-ribosome Remodeling.

Author

Raman N, Weir E, and Müller S

Subjects

ATPases Associated with Diverse Cellular Activities, Adenosine Triphosphatases metabolism, Binding Sites, Cloning, Molecular, Co-Repressor Proteins metabolism, Cysteine Endopeptidases metabolism, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Gene Expression Regulation, HEK293 Cells, HeLa Cells, Humans, Protein Binding, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Ribosome Subunits, Large, Eukaryotic metabolism, Ribosome Subunits, Large, Eukaryotic ultrastructure, Signal Transduction, Small Ubiquitin-Related Modifier Proteins metabolism, Transcription Factors metabolism, Adenosine Triphosphatases genetics, Co-Repressor Proteins genetics, Cysteine Endopeptidases genetics, Ribosome Subunits, Large, Eukaryotic genetics, Small Ubiquitin-Related Modifier Proteins genetics, Transcription Factors genetics

Abstract

Biogenesis of translation-competent 80S ribosomes is a multi-step process requiring the sequential action of non-ribosomal trans-acting factors. We previously identified the human PELP1-TEX10-WDR18 complex and the associated SUMO isopeptidase SENP3 as regulators of 60S maturation. We provided evidence that deconjugating SUMO from PELP1 by SENP3 is instrumental for proper ribosome biogenesis. Here we show that SUMO conjugation/deconjugation of PELP1 controls its dynamic association with the AAA ATPase MDN1, a key factor of pre-60S remodeling. We demonstrate that modification of PELP1 promotes the recruitment of MDN1 to pre-60S particles, while deSUMOylation is needed to release both MDN1 and PELP1 from pre-ribosomes. Inactivation of SENP3 traps MDN1 at pre-60S particles and prevents critical remodeling events, ultimately generating aberrant pre-60S complexes. We define MDN1 as a SUMO-targeted AAA ATPase, and we propose that a controlled SUMO cycle on PELP1 serves as regulatory point for mammalian 60S maturation through ordered recruitment and release of MDN1., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published

2016

46. Expression and Protein Interaction Analyses Reveal Combinatorial Interactions of LBD Transcription Factors During Arabidopsis Pollen Development.

Author

Kim M, Kim MJ, Pandey S, and Kim J

Subjects

Fluorescence, Glucuronidase metabolism, Green Fluorescent Proteins metabolism, Models, Biological, Plants, Genetically Modified, Protein Binding, Protein Interaction Mapping, Protoplasts metabolism, Recombinant Fusion Proteins metabolism, Subcellular Fractions metabolism, Arabidopsis growth & development, Arabidopsis metabolism, Arabidopsis Proteins metabolism, Pollen growth & development, Pollen metabolism, Transcription Factors metabolism

Abstract

LATERAL ORGAN BOUNDARIES DOMAIN (LBD) transcription factor gene family members play key roles in diverse aspects of plant development. LBD10 and LBD27 have been shown to be essential for pollen development in Arabidopsis thaliana. From the previous RNA sequencing (RNA-Seq) data set of Arabidopsis pollen, we identified the mRNAs of LBD22, LBD25 and LBD36 in addition to LBD10 and LBD27 in Arabidopsis pollen. Here we conducted expression and cellular analysis using GFP:GUS (green fluorescent protein:β-glucuronidase) reporter gene and subcellular localization assays using LBD:GFP fusion proteins expressed under the control of their own promoters in Arabidopsis. We found that these LBD proteins display spatially and temporally distinct and overlapping expression patterns during pollen development. Bimolecular fluorescence complementation and GST (glutathione S-transferase) pull-down assays demonstrated that protein-protein interactions occur among the LBDs exhibiting overlapping expression during pollen development. We further showed that LBD10, LBD22, LBD25, LBD27 and LBD36 interact with each other to form heterodimers, which are localized to the nucleus in Arabidopsis protoplasts. Taken together, these results suggest that combinatorial interactions among LBD proteins may be important for their function in pollen development in Arabidopsis., (© The Author 2016. Published by Oxford University Press on behalf of Japanese Society of Plant Physiologists. All rights reserved. For permissions, please email: journals.permissions@oup.com.)

Published

2016

47. IRF2BP2 transcriptional repressor restrains naive CD4 T cell activation and clonal expansion induced by TCR triggering.

Author

Sécca C, Faget DV, Hanschke SC, Carneiro MS, Bonamino MH, de-Araujo-Souza PS, and Viola JP

Subjects

Animals, Antigens, CD biosynthesis, Antigens, CD genetics, Antigens, Differentiation, T-Lymphocyte biosynthesis, Antigens, Differentiation, T-Lymphocyte genetics, Apoptosis immunology, Cells, Cultured, Cytokines biosynthesis, Cytokines genetics, Female, Gene Expression Regulation immunology, Humans, Interleukin-2 Receptor alpha Subunit biosynthesis, Interleukin-2 Receptor alpha Subunit genetics, Lectins, C-Type biosynthesis, Lectins, C-Type genetics, Lymphocyte Activation genetics, Male, Mice, Mice, Inbred C57BL, RNA, Messenger biosynthesis, RNA, Messenger genetics, Radiation Chimera, Recombinant Fusion Proteins metabolism, STAT5 Transcription Factor metabolism, Transduction, Genetic, CD4-Positive T-Lymphocytes immunology, Lymphocyte Activation immunology, Receptors, Antigen, T-Cell immunology, Transcription Factors immunology

Abstract

CD4 T cell activation and differentiation mechanisms constitute a complex and intricate signaling network involving several regulatory proteins. IRF2BP2 is a transcriptional repressor that is involved in gene-expression regulation in very diverse biologic contexts. Information regarding the IRF2BP2 regulatory function in CD4 T lymphocytes is very limited and suggests a role for this protein in repressing the expression of different cytokine genes. Here, we showed that Irf2bp2 gene expression was decreased in CD4 T cells upon activation. To investigate the possible regulatory roles for IRF2BP2 in CD4 T cell functions, this protein was ectopically expressed in murine primary-activated CD4 T lymphocytes through retroviral transduction. Interestingly, ectopic expression of IRF2BP2 led to a reduction in CD25 expression and STAT5 phosphorylation, along with an impaired proliferative capacity. The CD69 expression was also diminished in IRF2BP2-overexpressing cells, whereas CD44 and CD62L levels were not altered. In vivo, transferred, IRF2BP2-overexpressing, transduced cells displayed an impaired expansion capacity compared with controls. Furthermore, overexpression of IRF2BP2 in differentiated Th cells resulted in slightly reduced IL-4 and pro-TGF-β production in Th2 and iT regs but had no effect on IFN-γ or IL-17 expression in Th1 and Th17 cells, respectively. Taken together, our data suggest a role for IRF2BP2 in regulating CD4 T cell activation by repressing proliferation and the expression of CD25 and CD69 induced by TCR stimuli., (© Society for Leukocyte Biology.)

Published

2016

48. Positive Feedback Keeps Duration of Mitosis Temporally Insulated from Upstream Cell-Cycle Events.

Author

Araujo AR, Gelens L, Sheriff RS, and Santos SD

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Cell Cycle Proteins metabolism, Cell Line, Tumor, Chromatin metabolism, Epithelial Cells cytology, Epithelial Cells metabolism, Feedback, Physiological, G2 Phase genetics, HeLa Cells, Histones metabolism, Humans, Kinetics, Luminescent Proteins genetics, Luminescent Proteins metabolism, Molecular Imaging, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Time Factors, Transcription Factors metabolism, Transcription, Genetic, Red Fluorescent Protein, Cell Cycle Proteins genetics, Chromatin chemistry, Histones genetics, Mitosis, Models, Statistical, Transcription Factors genetics

Abstract

Cell division is characterized by a sequence of events by which a cell gives rise to two daughter cells. Quantitative measurements of cell-cycle dynamics in single cells showed that despite variability in G1-, S-, and G2 phases, duration of mitosis is short and remarkably constant. Surprisingly, there is no correlation between cell-cycle length and mitotic duration, suggesting that mitosis is temporally insulated from variability in earlier cell-cycle phases. By combining live cell imaging and computational modeling, we showed that positive feedback is the molecular mechanism underlying the temporal insulation of mitosis. Perturbing positive feedback gave rise to a sluggish, variable entry and progression through mitosis and uncoupled duration of mitosis from variability in cell cycle length. We show that positive feedback is important to keep mitosis short, constant, and temporally insulated and anticipate it might be a commonly used regulatory strategy to create modularity in other biological systems., (Copyright © 2016 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2016

49. Chromatin Kinases Act on Transcription Factors and Histone Tails in Regulation of Inducible Transcription.

Author

Josefowicz SZ, Shimada M, Armache A, Li CH, Miller RM, Lin S, Yang A, Dill BD, Molina H, Park HS, Garcia BA, Taunton J, Roeder RG, and Allis CD

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Cell Cycle Proteins metabolism, Cell Line, Tumor, Chromatin metabolism, Epithelial Cells cytology, Epithelial Cells metabolism, Feedback, Physiological, HeLa Cells, Histones metabolism, Humans, Kinetics, Luminescent Proteins genetics, Luminescent Proteins metabolism, Molecular Imaging, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Time Factors, Transcription Factors metabolism, Transcription, Genetic, Red Fluorescent Protein, Cell Cycle Proteins genetics, Chromatin chemistry, Histones genetics, Mitosis, Models, Statistical, Transcription Factors genetics

Abstract

The inflammatory response requires coordinated activation of both transcription factors and chromatin to induce transcription for defense against pathogens and environmental insults. We sought to elucidate the connections between inflammatory signaling pathways and chromatin through genomic footprinting of kinase activity and unbiased identification of prominent histone phosphorylation events. We identified H3 serine 28 phosphorylation (H3S28ph) as the principal stimulation-dependent histone modification and observed its enrichment at induced genes in mouse macrophages stimulated with bacterial lipopolysaccharide. Using pharmacological and genetic approaches, we identified mitogen- and stress-activated protein kinases (MSKs) as primary mediators of H3S28ph in macrophages. Cell-free transcription assays demonstrated that H3S28ph directly promotes p300/CBP-dependent transcription. Further, MSKs can activate both signal-responsive transcription factors and the chromatin template with additive effects on transcription. Specific inhibition of MSKs in macrophages selectively reduced transcription of stimulation-induced genes. Our results suggest that MSKs incorporate upstream signaling inputs and control multiple downstream regulators of inducible transcription., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published

2016

50. p63 is required beside p53 for PERP-mediated apoptosis in uveal melanoma.

Author

Awais R, Spiller DG, White MR, and Paraoan L

Subjects

Apoptosis drug effects, Apoptosis radiation effects, Cell Line, Tumor, DNA Damage, Gene Expression Regulation, Neoplastic, Humans, Immunoblotting, Melanoma genetics, Melanoma metabolism, Microscopy, Confocal, Real-Time Polymerase Chain Reaction, Recombinant Fusion Proteins metabolism, TNF-Related Apoptosis-Inducing Ligand pharmacology, Transcription Factors biosynthesis, Transcription Factors genetics, Transcriptional Activation, Tumor Suppressor Proteins biosynthesis, Tumor Suppressor Proteins genetics, Ultraviolet Rays, Uveal Neoplasms genetics, Uveal Neoplasms metabolism, Apoptosis physiology, Melanoma pathology, Transcription Factors physiology, Tumor Suppressor Proteins physiology, Uveal Neoplasms pathology

Abstract

Background: PERP (p53 apoptosis effector related to PMP-22), a transcriptional target of p53, is downregulated and contributes to the impairment of apoptosis in uveal melanoma (UM). Intriguingly, PERP is not induced in UM despite functional p53. p63, located on chromosome 3, which is characteristically altered in high-risk UM, can transactivate PERP. Here, we determine the functional role of p63 expression in the initiation of p53/PERP-mediated apoptosis in UM., Methods: PERP expression was monitored by quantitative PCR (qPCR) and immunoblotting in UM cell lines treated with DNA-damaging agents. The functional role of p63 was assessed by transient expression of p63-turbo GFP (p63-tGFP) in the apoptosis- resistant, 3q-deficient OCM-1 cells. Expression and localisation of p63, PERP and p53, and induction of apoptosis were characterised by qPCR, immunoblotting and live cell confocal microscopy., Results: PERP expression was significantly downregulated in all UM cell lines. DNA-damaging treatments failed to induce apoptosis and activate PERP in OCM-1 cells, which displayed non-functional levels of p63. Expression of p63-tGFP induced apoptosis with marked increase in PERP expression and associated p53 accumulation., Conclusions: Lack of p63 contributes to reduced PERP levels and impaired p53-mediated apoptosis in UM. p63 expression is required for PERP-mediated apoptosis in UM.

Published

2016