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1. Iron-sulfur clusters are involved in post-translational arginylation

Author

Verna Van, Janae B. Brown, Corin R. O’Shea, Hannah Rosenbach, Ijaz Mohamed, Nna-Emeka Ejimogu, Toan S. Bui, Veronika A. Szalai, Kelly N. Chacón, Ingrid Span, Fangliang Zhang, and Aaron T. Smith

Subjects
Science
Abstract

The enzyme ATE1 catalyzes eukaryotic post-translation arginylation, a key protein modification necessary for cellular homeostasis. Here, the authors show that ATE1s are previously unrealized iron-sulfur proteins that use this oxygen-sensitive inorganic cofactor to control cellular arginylation

Published
2023
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2. Molecular Features and Metal Ions That Influence 10-23 DNAzyme Activity

Author

Hannah Rosenbach, Julian Victor, Manuel Etzkorn, Gerhard Steger, Detlev Riesner, and Ingrid Span

Subjects
catalysis, deoxyribozymes (DNAzymes), gene silencing, metal ion cofactors, RNA hydrolysis, Organic chemistry, QD241-441
Abstract

Deoxyribozymes (DNAzymes) with RNA hydrolysis activity have a tremendous potential as gene suppression agents for therapeutic applications. The most extensively studied representative is the 10-23 DNAzyme consisting of a catalytic loop and two substrate binding arms that can be designed to bind and cleave the RNA sequence of interest. The RNA substrate is cleaved between central purine and pyrimidine nucleotides. The activity of this DNAzyme in vitro is considerably higher than in vivo, which was suggested to be related to its divalent cation dependency. Understanding the mechanism of DNAzyme catalysis is hindered by the absence of structural information. Numerous biological studies, however, provide comprehensive insights into the role of particular deoxynucleotides and functional groups in DNAzymes. Here we provide an overview of the thermodynamic properties, the impact of nucleobase modifications within the catalytic loop, and the role of different metal ions in catalysis. We point out features that will be helpful in developing novel strategies for structure determination and to understand the mechanism of the 10-23 DNAzyme. Consideration of these features will enable to develop improved strategies for structure determination and to understand the mechanism of the 10-23 DNAzyme. These insights provide the basis for improving activity in cells and pave the way for developing DNAzyme applications.

Published
2020
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3. Maturation strategy influences expression levels and cofactor occupancy in Fe–S proteins

Author

Melissa Jansing, Steffen Mielenbrink, Hannah Rosenbach, Sabine Metzger, and Ingrid Span

Subjects
Inorganic Chemistry, Biochemistry
Abstract

Iron–sulfur clusters are ubiquitous cofactors required for fundamental biological processes. Structural and spectroscopic analysis of Fe–S proteins is often limited by low cluster occupancy in recombinantly produced proteins. In this work, we report a systematic comparison of different maturation strategies for three well-established [4Fe–4S] proteins. Aconitase B, HMBPP reductase (IspH), and quinolinate synthase (NadA) were used as model proteins as they have previously been characterized. The protein production strategies include expression of the gene of interest in BL21(DE3) cells, maturation of the apo protein using chemical or semi-enzymatic reconstitution, co-expression with two different plasmids containing the iron–sulfur cluster (isc) or sulfur formation (suf) operon, a cell strain lacking IscR, the transcriptional regulator of the ISC machinery, and an engineered “SufFeScient” derivative of BL21(DE3). Our results show that co-expression of a Fe–S biogenesis pathway influences the protein yield and the cluster content of the proteins. The presence of the Fe–S cluster is contributing to correct folding and structural stability of the proteins. In vivo maturation reduces the formation of Fe–S aggregates, which occur frequently when performing chemical reconstitution. Furthermore, we show that the in vivo strategies can be extended to the radical SAM protein ThnB, which was previously only maturated by chemical reconstitution. Our results shed light on the differences of in vitro and in vivo Fe–S cluster maturation and points out the pitfalls of chemical reconstitution. Graphical abstract

Published
2022

4. Time-resolved structural analysis of an RNA-cleaving DNA catalyst

Author

Jan Borggräfe, Julian Victor, Hannah Rosenbach, Aldino Viegas, Christoph G. W. Gertzen, Christine Wuebben, Helena Kovacs, Mohanraj Gopalswamy, Detlev Riesner, Gerhard Steger, Olav Schiemann, Holger Gohlke, Ingrid Span, and Manuel Etzkorn

Subjects
Models, Molecular, Kinetics, Time Factors, Multidisciplinary, Metals, Biocatalysis, DNA, Single-Stranded, RNA, ddc:500, DNA, Catalytic, Nuclear Magnetic Resonance, Biomolecular
Abstract

The 10–23 DNAzyme is one of the most prominent catalytically active DNA sequences1,2. Its ability to cleave a wide range of RNA targets with high selectivity entails a substantial therapeutic and biotechnological potential2. However, the high expectations have not yet been met, a fact that coincides with the lack of high-resolution and time-resolved information about its mode of action3. Here we provide high-resolution NMR characterization of all apparent states of the prototypic 10–23 DNAzyme and present a comprehensive survey of the kinetics and dynamics of its catalytic function. The determined structure and identified metal-ion-binding sites of the precatalytic DNAzyme–RNA complex reveal that the basis of the DNA-mediated catalysis is an interplay among three factors: an unexpected, yet exciting molecular architecture; distinct conformational plasticity; and dynamic modulation by metal ions. We further identify previously hidden rate-limiting transient intermediate states in the DNA-mediated catalytic process via real-time NMR measurements. Using a rationally selected single-atom replacement, we could considerably enhance the performance of the DNAzyme, demonstrating that the acquired knowledge of the molecular structure, its plasticity and the occurrence of long-lived intermediate states constitutes a valuable starting point for the rational design of next-generation DNAzymes.

Published
2021

5. The Asp1 pyrophosphatase from S. pombe hosts a [2Fe-2S]2+ cluster in vivo

Author

Hannah Rosenbach, George E. Cutsail, James A. Birrell, Serena DeBeer, Ingrid Span, Marina Pascual-Ortiz, Ursula Fleig, and Eva Walla

Subjects
Pyrophosphatase, biology, Cell morphogenesis, Chemistry, Kinase, Iron–sulfur cluster, biology.organism_classification, Biochemistry, Pyrophosphate, Cofactor, Inorganic Chemistry, chemistry.chemical_compound, Protein kinase domain, Schizosaccharomyces pombe, biology.protein
Abstract

TheSchizosaccharomyces pombeAsp1 protein is a bifunctional kinase/pyrophosphatase that belongs to the highly conserved eukaryotic diphosphoinositol pentakisphosphate kinase PPIP5K/Vip1 family. The N-terminal Asp1 kinase domain generates specific high-energy inositol pyrophosphate (IPP) molecules, which are hydrolyzed by the C-terminal Asp1 pyrophosphatase domain (Asp1365−920). Thus, Asp1 activities regulate the intracellular level of a specific class of IPP molecules, which control a wide number of biological processes ranging from cell morphogenesis to chromosome transmission. Recently, it was shown that chemical reconstitution of Asp1371−920leads to the formation of a [2Fe-2S] cluster; however, the biological relevance of the cofactor remained under debate. In this study, we provide evidence for the presence of the Fe–S cluster in Asp1365−920inside the cell. However, we show that the Fe–S cluster does not influence Asp1 pyrophosphatase activity in vitro or in vivo. Characterization of the as-isolated protein by electronic absorption spectroscopy, mass spectrometry, and X-ray absorption spectroscopy is consistent with the presence of a [2Fe-2S]2+cluster in the enzyme. Furthermore, we have identified the cysteine ligands of the cluster. Overall, our work reveals that Asp1 contains an Fe–S cluster in vivo that is not involved in its pyrophosphatase activity.

Published
2021

6. Stability and Activity of the 10-23 DNAzyme Under Molecular Crowding Conditions

Author

Nina, Kirchgässler, Hannah, Rosenbach, and Ingrid, Span

Subjects
Kinetics, Fluorescence Resonance Energy Transfer, Thermodynamics, Electrophoresis, Polyacrylamide Gel, DNA, Catalytic
Abstract

DNAzymes are biocatalysts that have been selected in vitro and their function inside cells (in vivo) is extremely low. Thus, almost all studies have been carried out in diluted solutions (in vitro). The cellular presence of molecules such as amino acids, polypeptides, alcohols, and sugars introduces forces that modify the kinetics and thermodynamics of DNAzyme-mediated catalysis. The crowded intracellular environment referred to as molecular crowding can be mimicked by adding high concentrations of natural or synthetic macromolecules to the reaction conditions. Here, we investigate the activity of the 10-23 DNAzyme and the stability of the DNAzyme:RNA complex under molecular crowding conditions. Therefore, we use a Förster resonance energy transfer (FRET)-based activity assay in combination with denaturing urea polyacrylamide gel electrophoresis and circular dichroism (CD) spectroscopy.

Published
2022

7. Fluorescence-Based Kinetic Measurements for RNA-Cleaving DNAzymes

Author

Hannah, Rosenbach and Gerhard, Steger

Subjects
RNA Cleavage, Kinetics, RNA, DNA, Catalytic, Fluorescence
Abstract

Studying the catalytic behavior of biocatalysts under different conditions including temperature, buffer conditions, and cofactor concentrations is an important tool to understand their reaction mechanism. We describe two protocols that allow for the investigation of the catalysis of RNA-cleaving DNAzymes. The techniques include the use of FRET-labeled RNA substrates for studying the RNA-cleavage reaction in real-time under high throughput as well as RNA substrates labeled with a fluorescein molecule at the 5' end for gel-based assays. Both methods allow for an accurate determination of rate constants given a reaction model.

Published
2022

10. Iron-sulfur clusters are involved in post-translational arginylation

Author

Ingrid Span, Hannah Rosenbach, Kelly N. Chacón, Nna-Emeka Ejimogu, Toan S. Bui, Veronika A. Szalai, Ijaz Mohamed, Janae B. Brown, Aaron T. Smith, and Verna Van

Subjects
chemistry.chemical_classification, Protein stability, Regulatory control, Enzyme, chemistry, Post translational, Mechanism (biology), Cluster (physics), Molecular mechanism, chemistry.chemical_element, Sulfur, Cell biology
Abstract

Eukaryotic arginylation is an essential post-translational modification that both modulates protein stability and regulates protein half-life through the N-degron pathway. Arginylation is catalyzed by a family of enzymes known as the arginyl-tRNA transferases (ATE1s), which are conserved across the eukaryotic domain. Despite its conservation and importance, little is known regarding the structure, mechanism, and regulation of ATE1s. In this work, we have discovered that ATE1s bind a previously unknown iron-sulfur cluster that is conserved across evolution. We have extensively characterized the nature of this iron-sulfur cluster, and we show that the presence of the iron-sulfur cluster is linked to alterations in arginylation efficacy. Finally, we demonstrate that the ATE1 iron-sulfur cluster is oxygen sensitive, which could be a molecular mechanism of the N-degron pathway to sense oxidative stress. Thus, our data provide the framework of a cluster-based paradigm of ATE1 regulatory control.

Published
2021

11. The Asp1 pyrophosphatase from S. pombe hosts a [2Fe-2S]

Author

Hannah, Rosenbach, Eva, Walla, George E, Cutsail, James A, Birrell, Marina, Pascual-Ortiz, Serena, DeBeer, Ursula, Fleig, and Ingrid, Span

Subjects
Iron-Sulfur Proteins, Original Paper, Iron–sulfur cluster, X-ray absorption spectroscopy, Multifunctional Enzymes, Cytoskeletal Proteins, Phosphotransferases (Alcohol Group Acceptor), Inositol phosphate metabolism, Schizosaccharomyces pombe, Mutation, Schizosaccharomyces, Pyrophosphatase, Biocatalysis, Cysteine, Schizosaccharomyces pombe Proteins, PPIP5K/Vip1, Pyrophosphatases
Abstract

The Schizosaccharomyces pombe Asp1 protein is a bifunctional kinase/pyrophosphatase that belongs to the highly conserved eukaryotic diphosphoinositol pentakisphosphate kinase PPIP5K/Vip1 family. The N-terminal Asp1 kinase domain generates specific high-energy inositol pyrophosphate (IPP) molecules, which are hydrolyzed by the C-terminal Asp1 pyrophosphatase domain (Asp1365−920). Thus, Asp1 activities regulate the intracellular level of a specific class of IPP molecules, which control a wide number of biological processes ranging from cell morphogenesis to chromosome transmission. Recently, it was shown that chemical reconstitution of Asp1371−920 leads to the formation of a [2Fe-2S] cluster; however, the biological relevance of the cofactor remained under debate. In this study, we provide evidence for the presence of the Fe–S cluster in Asp1365−920 inside the cell. However, we show that the Fe–S cluster does not influence Asp1 pyrophosphatase activity in vitro or in vivo. Characterization of the as-isolated protein by electronic absorption spectroscopy, mass spectrometry, and X-ray absorption spectroscopy is consistent with the presence of a [2Fe-2S]2+ cluster in the enzyme. Furthermore, we have identified the cysteine ligands of the cluster. Overall, our work reveals that Asp1 contains an Fe–S cluster in vivo that is not involved in its pyrophosphatase activity. Supplementary Information The online version contains supplementary material available at 10.1007/s00775-020-01840-w.

Published
2020

12. Influence of monovalent metal ions on metal binding and catalytic activity of the 10-23 DNAzyme

Author

Wolfgang Hoyer, Manuel Etzkorn, Olav Schiemann, Julian Victor, Ingrid Span, Hannah Rosenbach, Christine Wuebben, Jan Borggräfe, and Gerhard Steger

Subjects
0301 basic medicine, Metal ions in aqueous solution, Clinical Biochemistry, Deoxyribozyme, DNA, Single-Stranded, 010402 general chemistry, Cleavage (embryo), 01 natural sciences, Biochemistry, Divalent, 03 medical and health sciences, chemistry.chemical_compound, ddc:570, Molecule, Molecular Biology, chemistry.chemical_classification, Ions, Binding Sites, Sodium, RNA, DNA, Catalytic, Combinatorial chemistry, 0104 chemical sciences, 030104 developmental biology, chemistry, Biocatalysis, Potassium, RNA Cleavage, DNA
Abstract

Deoxyribozymes (DNAzymes) are single-stranded DNA molecules that catalyze a broad range of chemical reactions. The 10–23 DNAzyme catalyzes the cleavage of RNA strands and can be designed to cleave essentially any target RNA, which makes it particularly interesting for therapeutic and biosensing applications. The activity of this DNAzyme in vitro is considerably higher than in cells, which was suggested to be a result of the low intracellular concentration of bioavailable divalent cations. While the interaction of the 10–23 DNAzyme with divalent metal ions was studied extensively, the influence of monovalent metal ions on its activity remains poorly understood. Here, we characterize the influence of monovalent and divalent cations on the 10–23 DNAzyme utilizing functional and biophysical techniques. Our results show that Na+ and K+ affect the binding of divalent metal ions to the DNAzyme:RNA complex and considerably modulate the reaction rates of RNA cleavage. We observe an opposite effect of high levels of Na+ and K+ concentrations on Mg2+- and Mn2+-induced reactions, revealing a different interplay of these metals in catalysis. Based on these findings, we propose a model for the interaction of metal ions with the DNAzyme:RNA complex.

Published
2020

13. Expanding crystallization tools for nucleic acid complexes using U1A protein variants

Author

Hannah, Rosenbach, Julian, Victor, Jan, Borggräfe, Ralf, Biehl, Gerhard, Steger, Manuel, Etzkorn, and Ingrid, Span

Subjects
Magnetic Resonance Spectroscopy, X-Ray Diffraction, Nucleic Acids, Scattering, Small Angle, ddc:540, Crystallization, Ribonucleoprotein, U1 Small Nuclear
Abstract

Journal of structural biology 210(2), 107480 (1-9) (2020). doi:10.1016/j.jsb.2020.107480, The major bottlenecks in structure elucidation of nucleic acids are crystallization and phasing. Co-crystallization with proteins is a straight forward approach to overcome these challenges. The human RNA-binding protein U1A has previously been established as crystallization module, however, the absence of UV-active residues and the predetermined architecture in the asymmetric unit constitute clear limitations of the U1A system. Here, we report three crystal structures of tryptophan-containing U1A variants, which expand the crystallization toolbox for nucleic acids. Analysis of the structures complemented by SAXS, NMR spectroscopy, and optical spectroscopy allow for insights into the potential of the U1A variants to serve as crystallization modules for nucleic acids. In addition, we report a fast and efficient protocol for crystallization of RNA by soaking and present a fluorescence-based approach for detecting RNA-binding in crystallo. Our results provide a new tool set for the crystallization of RNA and RNA:DNA complexes., Published by Elsevier, San Diego, Calif.

Published
2020
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