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1. Pathologie der entzündungsbedingten Gewebeschädigung bei Verbrennungen – Identifikation einer kausalen Rolle von lokalisierten C-reaktiven Protein Ablagerungen

Author

Braig, D, Kaiser, B, Thiele, JR, Bannasch, H, Stark, GB, Peter, K, Koch, HG, and Eisenhardt, SU

Subjects
ddc: 610, 610 Medical sciences, Medicine
Abstract

Einleitung: Die auf das thermische Trauma folgende Entzündungsreaktion kann den initialen Gewebeschaden weiter vergrößern. C-reaktives Protein (CRP) ist ein Akut-Phase Protein, dessen Plasmaspiegel im Rahmen eines Verbrennungstraumas rasant ansteigt. Ablagerungen von zirkulierendem, pentamerem[for full text, please go to the a.m. URL], 132. Kongress der Deutschen Gesellschaft für Chirurgie

Published
2015
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3. Maligne infantile Osteopetrose bei einem zweijährigen Jungen – eine Kasuistik

Author

Scheer, J, Mudler, A, Müller, S, Eberl, W, and Koch, HG

Subjects
ddc: 610, 610 Medical sciences, Medicine
Abstract

Hintergrund: Als Osteopetrose (auch Marmorknochenkrankheit) wird eine Gruppe seltener vererbbarer Erkrankungen des Skeletts bezeichnet, die sich durch eine vermehrte Knochendichte im Röntgenbild auszeichnen. Der Erkrankung liegt eine Fehlfunktion der Osteoklasten zugrunde. Bisher konnten Mutationen[for full text, please go to the a.m. URL], 60. Jahrestagung der Norddeutschen Gesellschaft für Kinder- und Jugendmedizin

Published
2011
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4. Das Toxic Schock Syndrom: Variabilität des klinischen Verlaufs

Author

Junius, L, Zellmer, A, Mudler, A, Sandvoss, A, Eberl, W, and Koch, HG

Subjects
ddc: 610, 610 Medical sciences, Medicine
Abstract

Einleitung: Das Toxic Schock Syndrom ist eine seltene Erkrankung (Inzidenz ca. 1/100.000 aller Frauen im Alter von 15–44 Jahren), die fulminant verläuft und lebensbedrohlich sein kann (Letalität 2–4%). Pathogenese: Toxin-1 vermittelte Reaktion des Staphylococcus aureus[for full text, please go to the a.m. URL], 60. Jahrestagung der Norddeutschen Gesellschaft für Kinder- und Jugendmedizin

Published
2011
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5. Cystathionine beta-synthasemutations in homocystinuria

Author

Kraus JP, Janosík M, Kozich V, Mandell R, Shih V, Sperandeo MP, Sebastio G, de Franchis R, Kluijtmans LA, Blom H, Boers GH, Gordon RB, Kamoun P, Tsai MY, Kruger WD, Koch HG, Ohura T, Gaustadnes M., ANDRIA, GENEROSO, Kraus, Jp, Janosík, M, Kozich, V, Mandell, R, Shih, V, Sperandeo, Mp, Sebastio, G, de Franchis, R, Andria, Generoso, Kluijtmans, La, Blom, H, Boers, Gh, Gordon, Rb, Kamoun, P, Tsai, My, Kruger, Wd, Koch, Hg, Ohura, T, and Gaustadnes, M.

Subjects
Cystathionine beta-synthase
Published
1999

8. Cystathionine beta- synthase mutations in homocystinuria

Author

Kraus, JP, Janosik, M, Kozich, V, Mandell, R, Shih, V, Sperandeo, MP, Sebastio, G, de Franchis, R, Andria, G, Kluijtmans, LAJ, Blom, H, Boers, GHJ, Gordon, RB, Kamoun, P, Tsai, MY, Kruger, W, Koch, HG, Ohura, T, and Gaustadnes, Mette

Published
1999

14. Molecular cloning and physical mapping of the tupaia herpesvirus genome

Author

Hajo Delius, J Clarke, Rolf M. Flügel, Bertfried Matz, Gholamreza Darai, and Koch Hg

Subjects
viruses, Immunology, EcoRI, Molecular cloning, HindIII, Microbiology, Restriction fragment, Restriction map, Virology, Animals, Cloning, Molecular, Herpesviridae, Southern blot, Tupaia, Genetics, biology, Tupaiidae, Chromosome Mapping, Nucleic Acid Hybridization, DNA Restriction Enzymes, Molecular biology, Restriction enzyme, Insect Science, DNA, Viral, biology.protein, Restriction fragment length polymorphism, Research Article
Abstract

Purified virion DNA of about 200 kilobase pairs of tupaia herpesvirus strain 2 was cleaved with EcoRI or HindIII restriction endonuclease. Restriction fragments representing the complete viral genome including both termini were inserted into the EcoRI, HindIII, and EcoRI-HindIII sites of the bacterial plasmid pAT153. Restriction maps for the restriction endonucleases EcoRI and HindIII were constructed with data derived from Southern blot hybridizations of individual viral DNA fragments or cloned DNA fragments which were hybridized to either viral genome fragments or recombinant plasmids. The analysis revealed that the tupaia herpesvirus genome consists of a long unique sequence of 200 kilobase pairs and that inverted repeat DNA sequences of greater than 40 base pairs do not occur, in agreement with previous electron microscopic data. No DNA sequence homology was detectable between the tupaia herpesvirus DNA and the genome of murine cytomegalovirus, which was reported to have a similar structure. In addition, seven individual isolates of tupaia herpesvirus were characterized. The isolates can be grouped into five strains by their DNA cleavage patterns.

Published
1985
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16. Cloned HBV DNA causes hepatitis in chimpanzees

Author

Hans Will, Koch Hg, H Schellekens, Heinz Schaller, Roberto Cattaneo, Deinhardt F, van Eerd Pm, and Gholamreza Darai

Subjects
Hepatitis B virus, Time Factors, Pan troglodytes, Hepatitis B virus DNA polymerase, viruses, Biology, medicine.disease_cause, Virus Replication, Hepatitis B virus PRE beta, DNA sequencing, chemistry.chemical_compound, Structure-Activity Relationship, Viral Proteins, medicine, Animals, Cloning, Molecular, Multidisciplinary, virus diseases, Hepatitis B, medicine.disease, Virology, digestive system diseases, Viral replication, chemistry, DNA, Viral, Viral hepatitis, DNA
Abstract

Most of our knowledge of the structure and function of the hepatitis B virus (HBV) genome comes from the analysis of the viral DNA sequences cloned in bacteria1–3. Because the physical state of cloned HBV DNA differs from HBV DNA encapsidated in the virion—for example, it lacks the nick-gap structure4, and a covalently linked protein5—the question arises as to whether it can initiate HBV replication in vitro6 or in vivo. We describe here the development of typical acute viral hepatitis, and the detection of HBV-specific DNA sequences in the serum and liver, in a chimpanzee inoculated with cloned HBV DNA. This demonstrates that neither the virion proteins nor the nick-gap structure of the virion DNA are needed for the initiation of replication of HBV in vivo.

Published
1982

17. Synthetisches Oestrogen und Gestagen zur Bahnung der Coli-Pyelonephritis im Tierexperiment

Author

K. Sack, W. Henkel, Koch Hg, and R. Commichau

Subjects
medicine.medical_specialty, Kidney, medicine.anatomical_structure, business.industry, medicine.medical_treatment, Urology, Medicine, business, Electrocoagulation
Abstract

In rats coli-pyelonephritis does not persist without temporary ureterligation or electrocoagulation of the kidney. After weekly injections of hydroxyprogesteronecapronate (1–25 mg) or oestradiolundecylate (0,01–2 mg) and endovesicle instillation of approximately 108 E. coli 0 25: K 19: H 12/ml a significant rate of pyelonephritis after 3 weeks is to be found.

Published
1969
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18. Prospektive Verlaufsstudie zur Langzeittherapie der chronischen Pyelonephritis

Author

Commichau R, Henkel W, and Koch Hg

Abstract

Die Haufigkeit chronischer Pyelonephritiden (Pn) als Ursache der Uramie und diagnostische Probleme infolge oligosymptomatischer oder atypischer Verlaufsformen haben in den letzten Jahren den Ausbau differenzierter nephrologischer Untersuchungsmethoden wesentlich mitbestimmt und die therapeutischen Bemuhungen intensiviert. Da mit der temporaren Sulfonamid- und Antibioticamedikation bei dieser bakteriellen, meist doppelseitigen herdformigen Nierenerkrankung keine befriedigenden Resultate zu erzielen waren [5, 12, 15, 24], forderte Haschen [8] die Langzeitbehandlung (LZB). Gegen diese Chemotherapie mit reduzierter Erhaltungsdosis wurde eingewandt, das sie den interstitiellen Entzundungsprozes auf Grund unzureichender Blut- und Gewebespiegel nicht wirksam beeinflusse und lediglich die Resistenzentwicklung pathogener Harnkeime fordere, zumal bei Niereninsuffizienz keine bakteriostatischen Harnkonzentrationen erreichbar sind [7]. Deshalb empfahlen Brod [3] sowie Thiel u Spuhler [22] die hochdosierte antibiotische Intervallbehandlung. Dieser Therapieform wird entgegengehalten, das abgekapselte pyelonephritische Herde in der vernarbten minderdurchbluteten Niere auch von hohen Antibioticakonzentrationen nicht erreicht werden und die intermittierende Medikation Rezidiven Vorschub leiste [20, 23].

Published
1968
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21. Diversity of cystathionine β-synthase haplotypes bearing the most common homocystinuria mutation c.833T>C: a possible role for gene conversion

Author

Michael Krawczak, Mette Gaustadnes, Gianfranco Sebastio, Viktor Kozich, Hans G. Koch, Jitka Sokolová, Michael Linnebank, David Neil Cooper, Bridget Wilcken, Toshihiro Ohura, Ewa Pronicka, Generoso Andria, Guglielmina Pepe, Olga Rickards, Sufin Yap, Leo A. J. Kluijtmans, David E.L. Wilcken, E. R. Naughten, Petr Vyletal, Henk J. Blom, Godfried H.J. Boers, Jan P. Kraus, Flemming Skovby, Aranka László, Vyletal, P, Sokolov, J, Cooper, Dn, Kraus, Jp, Krawczak, M, Pepe, G, Rickards, O, Koch, Hg, Linnebank, M, Kluijtmans, La, Blom, Hj, Boers, Gh, Gaustadnes, M, Skovby, F, Wilcken, B, Wilcken, De, Andria, Generoso, Sebastio, Gianfranco, Naughten, Er, Yap, S, Ohura, T, Pronicka, E, Laszlo, A, and Kozich, V.

Subjects
haplotype, Energy and redox metabolism [NCMLS 4], Molecular Sequence Data, Cystathionine beta-Synthase, Homocystinuria, Vascular medicine and diabetes [UMCN 2.2], Biology, Compound heterozygosity, CBS, homocystinuria, Genomic disorders and inherited multi-system disorders [IGMD 3], 03 medical and health sciences, 0302 clinical medicine, Gene Frequency, Genetics, medicine, Humans, pyridoxal 5′phosphate, Genetic Testing, Gene conversion, Allele, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Cystathionine beta-synthase, Haplotype, Homocysteine, Pyridoxal 5′phosphate, Base Sequence, gene conversion, Cardiovascular diseases [NCEBP 14], Transition (genetics), Genetic Variation, homocysteine, medicine.disease, Cystathionine beta synthase, 3. Good health, Europe, Settore BIO/18 - Genetica, Haplotypes, Africa, Mutation (genetic algorithm), biology.protein, 030217 neurology & neurosurgery, Research Article
Abstract

Contains fulltext : 52383.pdf (Publisher’s version ) (Closed access) Homozygosity or compound heterozygosity for the c.833T>C transition (p.I278 T) in the cystathionine beta-synthase (CBS) gene represents the most common cause of pyridoxine-responsive homocystinuria in Western Eurasians. However, the frequency of the pathogenic c.833C allele, as observed in healthy newborns from several European countries (q(c.833C) approximately equals 3.3 x 10(-3)), is approximately 20-fold higher than expected on the basis of the observed number of symptomatic homocystinuria patients carrying this mutation (q(c.833C) approximately equals 0.18 x 10(-3)), implying clinical underascertainment. Intriguingly, the c.833C mutation is also present in combination with a 68-bp insertion, c.[833C; 844_845ins68], in a substantial proportion of chromosomes from nonhomocystinuric individuals worldwide. We have sought to study the relationship between the pathogenic and nonpathogenic c.833C-bearing chromosomes and to determine whether the pathogenic c.[833C; -] chromosomes are identical-by-descent or instead arose by recurrent mutation. Initial haplotype analysis of 780 randomly selected Czech and sub-Saharan African wild-type chromosomes, employing 12 intragenic markers, revealed 29 distinct CBS haplotypes, of which 10 carried the c.[833C; 844_845ins68] combination; none carried an isolated c.833C or c.844_845ins68 mutation. Subsequent examination of 69 pathogenic c.[833C; -] chromosomes, derived from homocystinuria patients of predominantly European origin, disclosed three unrelated haplotypes that differed from their wild-type counterparts by virtue of the presence of c.833C, thereby indicating that c.833T>C transition has occurred repeatedly and independently in the past. Since c.833T does not reside within an obvious mutational hotspot, we surmise that the three pathogenic and comparatively prevalent c.[833C; -] chromosomes may have originated by recurrent gene conversion employing the common nonpathogenic c.[833C; 844_845ins68] chromosomes as templates.

Published
2007
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22. The small membrane protein CcoS is involved in cofactor insertion into the cbb 3 -type cytochrome c oxidase.

Author

Rauch J, Kurscheidt K, Shen KW, Andrei A, Daum N, Öztürk Y, Melin F, Layer G, Hellwig P, Daldal F, and Koch HG

Abstract

Respiratory complexes, such as cytochrome oxidases, are cofactor-containing multi-subunit protein complexes that are critically important for energy metabolism in all domains of life. Their intricate assembly strictly depends on accessory proteins, which coordinate subunit associations and cofactor deliveries. The small membrane protein CcoS was previously identified as an essential assembly factor to produce an active cbb 3 -type cytochrome oxidase (cbb 3 -Cox) in Rhodobacter capsulatus, but its function remained unknown. Here we show that the ΔccoS strain assembles a heme b deficient cbb 3 -Cox, in which the CcoN-CcoO subunit association is impaired. Chemical crosslinking demonstrates that CcoS interacts with the CcoN and CcoP subunits of cbb 3 -Cox, and that it stabilizes the interaction of the Cu-chaperone SenC with cbb 3 -Cox. CcoS lacks heme- or Cu-binding motifs, and we did not find evidence for direct heme or Cu binding; rather our data indicate that CcoS, together with SenC, coordinates heme and Cu insertion into cbb 3 -Cox., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: Petra Hellwig reports financial support was provided by Institute Universitaire de France. If there are other authors, they 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 © 2024 The Authors. Published by Elsevier B.V. All rights reserved.)

Published
2024
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23. A nanoengineered tandem nitroreductase: designing a robust prodrug-activating nanoreactor.

Author

Zmyslia M, Capper MJ, Grimmeisen M, Sartory K, Deuringer B, Abdelsalam M, Shen K, Jung M, Sippl W, Koch HG, Kaul L, Süss R, Köhnke J, and Jessen-Trefzer C

Abstract

Nitroreductases are important enzymes for a variety of applications, including cancer therapy and bioremediation. They often require encapsulation to improve stability and activity. We focus on genetically encoded encapsulation of nitroreductases within protein capsids, like encapsulins. Our study showcases the encapsulation of nitroreductase NfsB as functional dimers within encapsulins, which enhances protein activity and stability in diverse conditions. Mutations within the pore region are beneficial for activity of the encapsulated enzyme, potentially by increasing diffusion rates. Cryogenic electron microscopy reveals the overall architecture of the encapsulated dimeric NfsB within the nanoreactor environment and identifies multiple pore states in the shell. These findings highlight the potential of encapsulins as versatile tools for enhancing enzyme performance across various fields., Competing Interests: There are no conflicts to declare., (This journal is © The Royal Society of Chemistry.)

Published
2024
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24. The contribution of mRNA targeting to spatial protein localization in bacteria.

Author

Shang W, Lichtenberg E, Mlesnita AM, Wilde A, and Koch HG

Subjects
Protein Sorting Signals genetics, Cell Membrane metabolism, Protein Biosynthesis, Membrane Proteins metabolism, Membrane Proteins genetics, RNA, Bacterial metabolism, RNA, Bacterial genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Bacterial Proteins metabolism, Bacterial Proteins genetics, Protein Transport, Bacteria metabolism, Bacteria genetics
Abstract

About 30% of all bacterial proteins execute their function outside of the cytosol and must be inserted into or translocated across the cytoplasmic membrane. This requires efficient targeting systems that recognize N-terminal signal sequences in client proteins and deliver them to protein transport complexes in the membrane. While the importance of these protein transport machineries for the spatial organization of the bacterial cell is well documented in multiple studies, the contribution of mRNA targeting and localized translation to protein transport is only beginning to emerge. mRNAs can exhibit diverse subcellular localizations in the bacterial cell and can accumulate at sites where new protein is required. This is frequently observed for mRNAs encoding membrane proteins, but the physiological importance of membrane enrichment of mRNAs and the consequences it has for the insertion of the encoded protein have not been explored in detail. Here, we briefly highlight some basic concepts of signal sequence-based protein targeting and describe in more detail strategies that enable the monitoring of mRNA localization in bacterial cells and potential mechanisms that route mRNAs to particular positions within the cell. Finally, we summarize some recent developments that demonstrate that mRNA targeting and localized translation can sustain membrane protein insertion under stress conditions when the protein-targeting machinery is compromised. Thus, mRNA targeting likely acts as a back-up strategy and complements the canonical signal sequence-based protein targeting., (© 2024 The Authors. The FEBS Journal published by John Wiley & Sons Ltd on behalf of Federation of European Biochemical Societies.)

Published
2024
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25. Ribosome-inactivation by a class of widely distributed C-tail anchored membrane proteins.

Author

Njenga RK, Boele J, Drepper F, Sinha K, Marouda E, Huesgen PF, Blaby-Haas C, and Koch HG

Abstract

Ribosome hibernation is a commonly used strategy that protects ribosomes under unfavorable conditions and regulates developmental processes. Multiple ribosome-hibernation factors have been identified in all domains of life, but due to their structural diversity and the lack of a common inactivation mechanism, it is currently unknown how many different hibernation factors exist. Here, we show that the YqjD/ElaB/YgaM paralogs, initially discovered as membrane-bound ribosome binding proteins in E. coli, constitute an abundant class of ribosome-hibernating proteins, which are conserved across all proteobacteria and some other bacterial phyla. Our data demonstrate that they inhibit in vitro protein synthesis by interacting with the 50S ribosomal subunit. In vivo cross-linking combined with mass spectrometry revealed their specific interactions with proteins surrounding the ribosomal tunnel exit and even their penetration into the ribosomal tunnel. Thus, YqjD/ElaB/YgaM inhibit translation by blocking the ribosomal tunnel and thus mimic the activity of antimicrobial peptides and macrolide antibiotics., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published
2024
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26. Control of a chemical chaperone by a universally conserved ATPase.

Author

Jiang H, Milanov M, Jüngert G, Angebauer L, Flender C, Smudde E, Gather F, Vogel T, Jessen HJ, and Koch HG

Abstract

The universally conserved YchF/Ola1 ATPases regulate stress response pathways in prokaryotes and eukaryotes. Deletion of YchF/Ola1 leads to increased resistance against environmental stressors, such as reactive oxygen species, while their upregulation is associated with tumorigenesis in humans. The current study shows that in E. coli , the absence of YchF stimulates the synthesis of the alternative sigma factor RpoS by a transcription-independent mechanism. Elevated levels of RpoS then enhance the transcription of major stress-responsive genes. In addition, the deletion of ychF increases the levels of polyphosphate kinase, which in turn boosts the production of the evolutionary conserved and ancient chemical chaperone polyphosphate. This potentially provides a unifying concept for the increased stress resistance in bacteria and eukaryotes upon YchF/Ola1 deletion. Intriguingly, the simultaneous deletion of ychF and the polyphosphate-degrading enzyme exopolyphosphatase causes synthetic lethality in E. coli , demonstrating that polyphosphate production needs to be fine-tuned to prevent toxicity., Competing Interests: The authors declare no competing interests., (© 2024 The Authors.)

Published
2024
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27. YidC from Escherichia coli Forms an Ion-Conducting Pore upon Activation by Ribosomes.

Author

Knyazev DG, Winter L, Vogt A, Posch S, Öztürk Y, Siligan C, Goessweiner-Mohr N, Hagleitner-Ertugrul N, Koch HG, and Pohl P

Subjects
Membrane Transport Proteins metabolism, Ribosomes metabolism, Arginine metabolism, Cell Membrane metabolism, Escherichia coli metabolism, Escherichia coli Proteins metabolism
Abstract

The universally conserved protein YidC aids in the insertion and folding of transmembrane polypeptides. Supposedly, a charged arginine faces its hydrophobic lipid core, facilitating polypeptide sliding along YidC's surface. How the membrane barrier to other molecules may be maintained is unclear. Here, we show that the purified and reconstituted E. coli YidC forms an ion-conducting transmembrane pore upon ribosome or ribosome-nascent chain complex (RNC) binding. In contrast to monomeric YidC structures, an AlphaFold parallel YidC dimer model harbors a pore. Experimental evidence for a dimeric assembly comes from our BN-PAGE analysis of native vesicles, fluorescence correlation spectroscopy studies, single-molecule fluorescence photobleaching observations, and crosslinking experiments. In the dimeric model, the conserved arginine and other residues interacting with nascent chains point into the putative pore. This result suggests the possibility of a YidC-assisted insertion mode alternative to the insertase mechanism.

Published
2023
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28. Coping with stress: How bacteria fine-tune protein synthesis and protein transport.

Author

Njenga R, Boele J, Öztürk Y, and Koch HG

Subjects
Adaptation, Psychological, Escherichia coli genetics, Escherichia coli metabolism, Heat-Shock Proteins metabolism, Escherichia coli Proteins metabolism, Protein Biosynthesis, Protein Transport
Abstract

Maintaining a functional proteome under different environmental conditions is challenging for every organism, in particular for unicellular organisms, such as bacteria. In order to cope with changing environments and stress conditions, bacteria depend on strictly coordinated proteostasis networks that control protein production, folding, trafficking, and degradation. Regulation of ribosome biogenesis and protein synthesis are cornerstones of this cellular adaptation in all domains of life, which is rationalized by the high energy demand of both processes and the increased resistance of translationally silent cells against internal or external poisons. Reduced protein synthesis ultimately also reduces the substrate load for protein transport systems, which are required for maintaining the periplasmic, inner, and outer membrane subproteomes. Consequences of impaired protein transport have been analyzed in several studies and generally induce a multifaceted response that includes the upregulation of chaperones and proteases and the simultaneous downregulation of protein synthesis. In contrast, generally less is known on how bacteria adjust the protein targeting and transport machineries to reduced protein synthesis, e.g., when cells encounter stress conditions or face nutrient deprivation. In the current review, which is mainly focused on studies using Escherichia coli as a model organism, we summarize basic concepts on how ribosome biogenesis and activity are regulated under stress conditions. In addition, we highlight some recent developments on how stress conditions directly impair protein targeting to the bacterial membrane. Finally, we describe mechanisms that allow bacteria to maintain the transport of stress-responsive proteins under conditions when the canonical protein targeting pathways are impaired., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2023 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2023
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29. Central role of Tim17 in mitochondrial presequence protein translocation.

Author

Fielden LF, Busch JD, Merkt SG, Ganesan I, Steiert C, Hasselblatt HB, Busto JV, Wirth C, Zufall N, Jungbluth S, Noll K, Dung JM, Butenko L, von der Malsburg K, Koch HG, Hunte C, van der Laan M, and Wiedemann N

Subjects
Mitochondrial Membranes metabolism, Protein Transport, Mitochondria metabolism, Mitochondrial Precursor Protein Import Complex Proteins metabolism, Saccharomyces cerevisiae cytology, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism
Abstract

The presequence translocase of the mitochondrial inner membrane (TIM23) represents the major route for the import of nuclear-encoded proteins into mitochondria 1,2 . About 60% of more than 1,000 different mitochondrial proteins are synthesized with amino-terminal targeting signals, termed presequences, which form positively charged amphiphilic α-helices 3,4 . TIM23 sorts the presequence proteins into the inner membrane or matrix. Various views, including regulatory and coupling functions, have been reported on the essential TIM23 subunit Tim17 (refs. 5-7 ). Here we mapped the interaction of Tim17 with matrix-targeted and inner membrane-sorted preproteins during translocation in the native membrane environment. We show that Tim17 contains conserved negative charges close to the intermembrane space side of the bilayer, which are essential to initiate presequence protein translocation along a distinct transmembrane cavity of Tim17 for both classes of preproteins. The amphiphilic character of mitochondrial presequences directly matches this Tim17-dependent translocation mechanism. This mechanism permits direct lateral release of transmembrane segments of inner membrane-sorted precursors into the inner membrane., (© 2023. The Author(s).)

Published
2023
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30. mRNA targeting eliminates the need for the signal recognition particle during membrane protein insertion in bacteria.

Author

Sarmah P, Shang W, Origi A, Licheva M, Kraft C, Ulbrich M, Lichtenberg E, Wilde A, and Koch HG

Subjects
Signal Recognition Particle genetics, Signal Recognition Particle metabolism, Bacterial Proteins metabolism, Escherichia coli genetics, Escherichia coli metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Bacteria metabolism, SEC Translocation Channels genetics, SEC Translocation Channels metabolism, Protein Transport, Ribosomes metabolism, Membrane Transport Proteins metabolism, Membrane Proteins genetics, Membrane Proteins metabolism, Escherichia coli Proteins metabolism
Abstract

Signal-sequence-dependent protein targeting is essential for the spatiotemporal organization of eukaryotic and prokaryotic cells and is facilitated by dedicated protein targeting factors such as the signal recognition particle (SRP). However, targeting signals are not exclusively contained within proteins but can also be present within mRNAs. By in vivo and in vitro assays, we show that mRNA targeting is controlled by the nucleotide content and by secondary structures within mRNAs. mRNA binding to bacterial membranes occurs independently of soluble targeting factors but is dependent on the SecYEG translocon and YidC. Importantly, membrane insertion of proteins translated from membrane-bound mRNAs occurs independently of the SRP pathway, while the latter is strictly required for proteins translated from cytosolic mRNAs. In summary, our data indicate that mRNA targeting acts in parallel to the canonical SRP-dependent protein targeting and serves as an alternative strategy for safeguarding membrane protein insertion when the SRP pathway is compromised., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2023 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published
2023
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31. Metabolic Sensing of Extracytoplasmic Copper Availability via Translational Control by a Nascent Exported Protein.

Author

Öztürk Y, Andrei A, Blaby-Haas CE, Daum N, Daldal F, and Koch HG

Subjects
Binding Sites, Ribosomes metabolism, Gene Expression Regulation, Copper metabolism, Oxidoreductases metabolism
Abstract

Metabolic sensing is a crucial prerequisite for cells to adjust their physiology to rapidly changing environments. In bacteria, the response to intra- and extracellular ligands is primarily controlled by transcriptional regulators, which activate or repress gene expression to ensure metabolic acclimation. Translational control, such as ribosomal stalling, can also contribute to cellular acclimation and has been shown to mediate responses to changing intracellular molecules. In the current study, we demonstrate that the cotranslational export of the Rhodobacter capsulatus protein CutF regulates the translation of the downstream cutO -encoded multicopper oxidase CutO in response to extracellular copper (Cu). Our data show that CutF, acting as a Cu sensor, is cotranslationally exported by the signal recognition particle pathway. The binding of Cu to the periplasmically exposed Cu-binding motif of CutF delays its cotranslational export via its C-terminal ribosome stalling-like motif. This allows for the unfolding of an mRNA stem-loop sequence that shields the ribosome-binding site of cutO , which favors its subsequent translation. Bioinformatic analyses reveal that CutF-like proteins are widely distributed in bacteria and are often located upstream of genes involved in transition metal homeostasis. Our overall findings illustrate a highly conserved control mechanism using the cotranslational export of a protein acting as a sensor to integrate the changing availability of extracellular nutrients into metabolic acclimation. IMPORTANCE Metabolite sensing is a fundamental biological process, and the perception of dynamic changes in the extracellular environment is of paramount importance for the survival of organisms. Bacteria usually adjust their metabolisms to changing environments via transcriptional regulation. Here, using Rhodobacter capsulatus, we describe an alternative translational mechanism that controls the bacterial response to the presence of copper, a toxic micronutrient. This mechanism involves a cotranslationally secreted protein that, in the presence of copper, undergoes a process resembling ribosomal stalling. This allows for the unfolding of a downstream mRNA stem-loop and enables the translation of the adjacent Cu-detoxifying multicopper oxidase. Bioinformatic analyses reveal that such proteins are widespread, suggesting that metabolic sensing using ribosome-arrested nascent secreted proteins acting as sensors may be a common strategy for the integration of environmental signals into metabolic adaptations.

Published
2023
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32. A common evolutionary origin reveals fundamental principles of protein insertases.

Author

Vögtle FN, Koch HG, and Meisinger C

Subjects
Hydrophobic and Hydrophilic Interactions, Lipid Bilayers chemistry, Membrane Proteins genetics, Membrane Proteins metabolism
Abstract

Membrane proteins require protein machineries to insert their hydrophobic transmembrane domains (TMDs) into the lipid bilayer. A functional analysis of protein insertases in this issue of PLOS Biology reveals that the fundamental mechanism of membrane protein insertion is universally conserved., Competing Interests: The authors declare that there are no conflicts of interest.

Published
2022
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33. Inhibition of SRP-dependent protein secretion by the bacterial alarmone (p)ppGpp.

Author

Czech L, Mais CN, Kratzat H, Sarmah P, Giammarinaro P, Freibert SA, Esser HF, Musial J, Berninghausen O, Steinchen W, Beckmann R, Koch HG, and Bange G

Subjects
Bacterial Proteins metabolism, Escherichia coli metabolism, Guanosine Pentaphosphate metabolism, Protein Binding, Receptors, Cytoplasmic and Nuclear metabolism, Escherichia coli Proteins metabolism, Signal Recognition Particle metabolism
Abstract

The stringent response enables bacteria to respond to nutrient limitation and other stress conditions through production of the nucleotide-based second messengers ppGpp and pppGpp, collectively known as (p)ppGpp. Here, we report that (p)ppGpp inhibits the signal recognition particle (SRP)-dependent protein targeting pathway, which is essential for membrane protein biogenesis and protein secretion. More specifically, (p)ppGpp binds to the SRP GTPases Ffh and FtsY, and inhibits the formation of the SRP receptor-targeting complex, which is central for the coordinated binding of the translating ribosome to the SecYEG translocon. Cryo-EM analysis of SRP bound to translating ribosomes suggests that (p)ppGpp may induce a distinct conformational stabilization of the NG domain of Ffh and FtsY in Bacillus subtilis but not in E. coli., (© 2022. The Author(s).)

Published
2022
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34. Symptom Burden and Factors Associated with Acute Respiratory Infections in the First Two Years of Life-Results from the LoewenKIDS Cohort.

Author

Langer S, Horn J, Gottschick C, Klee B, Purschke O, Caputo M, Dorendorf E, Meyer-Schlinkmann KM, Raupach-Rosin H, Karch A, Rübsamen N, Aydogdu M, Buhles M, Dressler F, Eberl W, Koch FEV, Frambach T, Franz H, Guthmann F, Guzman CA, Haase R, Hansen G, Heselich V, Hübner J, Koch HG, Oberhoff C, Riese P, Schild R, Seeger S, Tchirikov M, Trittel S, von Kaisenberg C, and Mikolajczyk R

Abstract

Acute respiratory infections (ARIs) are the most common childhood illnesses worldwide whereby the reported frequency varies widely, often depending on type of assessment. Symptom diaries are a powerful tool to counteract possible under-reporting, particularly of milder infections, and thus offer the possibility to assess the full burden of ARIs. The following analyses are based on symptom diaries from participants of the German birth cohort study LoewenKIDS. Primary analyses included frequencies of ARIs and specific symptoms. Factors, which might be associated with an increased number of ARIs, were identified using the Poisson regression. A subsample of two hundred eighty-eight participants were included. On average, 13.7 ARIs (SD: 5.2 median: 14.0 IQR: 10-17) were reported in the first two years of life with an average duration of 11 days per episode (SD: 5.8, median: 9.7, IQR: 7-14). The median age for the first ARI episode was 91 days (IQR: 57-128, mean: 107, SD: 84.5). Childcare attendance and having siblings were associated with an increased frequency of ARIs, while exclusive breastfeeding for the first three months was associated with less ARIs, compared to exclusive breastfeeding for a longer period. This study provides detailed insight into the symptom burden of ARIs in German infants.

Published
2022
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35. The Role of the Universally Conserved ATPase YchF/Ola1 in Translation Regulation during Cellular Stress.

Author

Landwehr V, Milanov M, Hong J, and Koch HG

Abstract

The ability to respond to metabolic or environmental changes is an essential feature in all cells and involves both transcriptional and translational regulators that adjust the metabolic activity to fluctuating conditions. While transcriptional regulation has been studied in detail, the important role of the ribosome as an additional player in regulating gene expression is only beginning to emerge. Ribosome-interacting proteins are central to this translational regulation and include universally conserved ribosome interacting proteins, such as the ATPase YchF (Ola1 in eukaryotes). In both eukaryotes and bacteria, the cellular concentrations of YchF/Ola1 determine the ability to cope with different stress conditions and are linked to several pathologies in humans. The available data indicate that YchF/Ola1 regulates the stress response via controlling non-canonical translation initiation and via protein degradation. Although the molecular mechanisms appear to be different between bacteria and eukaryotes, increased non-canonical translation initiation is a common consequence of YchF/Ola1 regulated translational control in E. coli and H. sapiens . In this review, we summarize recent insights into the role of the universally conserved ATPase YchF/Ola1 in adapting translation to unfavourable conditions.

Published
2021
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36. The largely unexplored biology of small proteins in pro- and eukaryotes.

Author

Steinberg R and Koch HG

Subjects
Eukaryota cytology, Antimicrobial Peptides metabolism, Eukaryota metabolism
Abstract

The large abundance of small open reading frames (smORFs) in prokaryotic and eukaryotic genomes and the plethora of smORF-encoded small proteins became only apparent with the constant advancements in bioinformatic, genomic, proteomic, and biochemical tools. Small proteins are typically defined as proteins of < 50 amino acids in prokaryotes and of less than 100 amino acids in eukaryotes, and their importance for cell physiology and cellular adaptation is only beginning to emerge. In contrast to antimicrobial peptides, which are secreted by prokaryotic and eukaryotic cells for combatting pathogens and competitors, small proteins act within the producing cell mainly by stabilizing protein assemblies and by modifying the activity of larger proteins. Production of small proteins is frequently linked to stress conditions or environmental changes, and therefore, cells seem to use small proteins as intracellular modifiers for adjusting cell metabolism to different intra- and extracellular cues. However, the size of small proteins imposes a major challenge for the cellular machinery required for protein folding and intracellular trafficking and recent data indicate that small proteins can engage distinct trafficking pathways. In the current review, we describe the diversity of small proteins in prokaryotes and eukaryotes, highlight distinct and common features, and illustrate how they are handled by the protein trafficking machineries in prokaryotic and eukaryotic cells. Finally, we also discuss future topics of research on this fascinating but largely unexplored group of proteins., (© 2021 The Authors. The FEBS Journal published by John Wiley & Sons Ltd on behalf of Federation of European Biochemical Societies.)

Published
2021
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37. Quantitative proteomics identifies the universally conserved ATPase Ola1p as a positive regulator of heat shock response in Saccharomyces cerevisiae.

Author

Dannenmaier S, Desroches Altamirano C, Schüler L, Zhang Y, Hummel J, Milanov M, Oeljeklaus S, Koch HG, Rospert S, Alberti S, and Warscheid B

Subjects
Adenosine Triphosphatases genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins genetics, Adenosine Triphosphatases metabolism, Gene Expression Regulation, Fungal, Heat-Shock Response, Protein Biosynthesis, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism
Abstract

The universally conserved P-loop ATPase Ola1 is implicated in various cellular stress response pathways, as well as in cancer and tumor progression. However, Ola1p functions are divergent between species, and the involved mechanisms are only poorly understood. Here, we studied the role of Ola1p in the heat shock response of the yeast Saccharomyces cerevisiae using a combination of quantitative and pulse labeling-based proteomics approaches, in vitro studies, and cell-based assays. Our data show that when heat stress is applied to cells lacking Ola1p, the expression of stress-protective proteins is enhanced. During heat stress Ola1p associates with detergent-resistant protein aggregates and rapidly forms assemblies that localize to stress granules. The assembly of Ola1p was also observed in vitro using purified protein and conditions, which resembled those in living cells. We show that loss of Ola1p results in increased protein ubiquitination of detergent-insoluble aggregates recovered from heat-shocked cells. When cells lacking Ola1p were subsequently relieved from heat stress, reinitiation of translation was delayed, whereas, at the same time, de novo synthesis of central factors required for protein refolding and the clearance of aggregates was enhanced when compared with wild-type cells. The combined data suggest that upon acute heat stress, Ola1p is involved in the stabilization of misfolded proteins, which become sequestered in cytoplasmic stress granules. This function of Ola1p enables cells to resume translation in a timely manner as soon as heat stress is relieved., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2021
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38. The missing enzymatic link in syntrophic methane formation from fatty acids.

Author

Agne M, Estelmann S, Seelmann CS, Kung J, Wilkens D, Koch HG, van der Does C, Albers SV, von Ballmoos C, Simon J, and Boll M

Subjects
Acetates metabolism, Acyl Coenzyme A metabolism, Archaea metabolism, Electron Transport physiology, Fermentation physiology, Formates metabolism, Oxidation-Reduction, Oxidoreductases metabolism, Bacterial Proteins metabolism, Deltaproteobacteria metabolism, Fatty Acids metabolism, Methane metabolism
Abstract

The microbial production of methane from organic matter is an essential process in the global carbon cycle and an important source of renewable energy. It involves the syntrophic interaction between methanogenic archaea and bacteria that convert primary fermentation products such as fatty acids to the methanogenic substrates acetate, H 2 , CO 2 , or formate. While the concept of syntrophic methane formation was developed half a century ago, the highly endergonic reduction of CO 2 to methane by electrons derived from β-oxidation of saturated fatty acids has remained hypothetical. Here, we studied a previously noncharacterized membrane-bound oxidoreductase (EMO) from Syntrophus aciditrophicus containing two heme b cofactors and 8-methylmenaquinone as key redox components of the redox loop-driven reduction of CO 2 by acyl-coenzyme A (CoA). Using solubilized EMO and proteoliposomes, we reconstituted the entire electron transfer chain from acyl-CoA to CO 2 and identified the transfer from a high- to a low-potential heme b with perfectly adjusted midpoint potentials as key steps in syntrophic fatty acid oxidation. The results close our gap of knowledge in the conversion of biomass into methane and identify EMOs as key players of β-oxidation in (methyl)menaquinone-containing organisms., Competing Interests: The authors declare no competing interest.

Published
2021
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39. The CopA2-Type P 1B -Type ATPase CcoI Serves as Central Hub for cbb 3 -Type Cytochrome Oxidase Biogenesis.

Author

Andrei A, Di Renzo MA, Öztürk Y, Meisner A, Daum N, Frank F, Rauch J, Daldal F, Andrade SLA, and Koch HG

Abstract

Copper (Cu)-transporting P 1B -type ATPases are ubiquitous metal transporters and crucial for maintaining Cu homeostasis in all domains of life. In bacteria, the P 1B -type ATPase CopA is required for Cu-detoxification and exports excess Cu(I) in an ATP-dependent reaction from the cytosol into the periplasm. CopA is a member of the CopA1-type ATPase family and has been biochemically and structurally characterized in detail. In contrast, less is known about members of the CopA2-type ATPase family, which are predicted to transport Cu(I) into the periplasm for cuproprotein maturation. One example is CcoI, which is required for the maturation of cbb 3 -type cytochrome oxidase ( cbb 3 -Cox) in different species. Here, we reconstituted purified CcoI of Rhodobacter capsulatus into liposomes and determined Cu transport using solid-supported membrane electrophysiology. The data demonstrate ATP-dependent Cu(I) translocation by CcoI, while no transport is observed in the presence of a non-hydrolysable ATP analog. CcoI contains two cytosolically exposed N-terminal metal binding sites (N-MBSs), which are both important, but not essential for Cu delivery to cbb 3 -Cox. CcoI and cbb 3 -Cox activity assays in the presence of different Cu concentrations suggest that the glutaredoxin-like N-MBS1 is primarily involved in regulating the ATPase activity of CcoI, while the CopZ-like N-MBS2 is involved in Cu(I) acquisition. The interaction of CcoI with periplasmic Cu chaperones was analyzed by genetically fusing CcoI to the chaperone SenC. The CcoI-SenC fusion protein was fully functional in vivo and sufficient to provide Cu for cbb 3 -Cox maturation. In summary, our data demonstrate that CcoI provides the link between the cytosolic and periplasmic Cu chaperone networks during cbb 3 -Cox assembly., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Andrei, Di Renzo, Öztürk, Meisner, Daum, Frank, Rauch, Daldal, Andrade and Koch.)

Published
2021
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40. Maturation of Rhodobacter capsulatus Multicopper Oxidase CutO Depends on the CopA Copper Efflux Pathway and Requires the cutF Product.

Author

Öztürk Y, Blaby-Haas CE, Daum N, Andrei A, Rauch J, Daldal F, and Koch HG

Abstract

Copper (Cu) is an essential cofactor required for redox enzymes in all domains of life. Because of its toxicity, tightly controlled mechanisms ensure Cu delivery for cuproenzyme biogenesis and simultaneously protect cells against toxic Cu. Many Gram-negative bacteria contain extracytoplasmic multicopper oxidases (MCOs), which are involved in periplasmic Cu detoxification. MCOs are unique cuproenzymes because their catalytic center contains multiple Cu atoms, which are required for the oxidation of Cu 1+ to the less toxic Cu 2+ . Hence, Cu is both substrate and essential cofactor of MCOs. Here, we investigated the maturation of Rhodobacter capsulatus MCO CutO and its role in periplasmic Cu detoxification. A survey of CutO activity of R. capsulatus mutants with known defects in Cu homeostasis and in the maturation of the cuproprotein cbb 3 -type cytochrome oxidase ( cbb 3 -Cox) was performed. This revealed that CutO activity is largely independent of the Cu-delivery pathway for cbb 3 -Cox biogenesis, except for the cupric reductase CcoG, which is required for full CutO activity. The most pronounced decrease of CutO activity was observed with strains lacking the cytoplasmic Cu chaperone CopZ, or the Cu-exporting ATPase CopA, indicating that CutO maturation is linked to the CopZ-CopA mediated Cu-detoxification pathway. Our data demonstrate that CutO is important for cellular Cu resistance under both aerobic and anaerobic growth conditions. CutO is encoded in the cutFOG operon, but only CutF, and not CutG, is essential for CutO activity. No CutO activity is detectable when cutF or its putative Cu-binding motif are mutated, suggesting that the cutF product serves as a Cu-binding component required for active CutO production. Bioinformatic analyses of CutF-like proteins support their widespread roles as putative Cu-binding proteins for several Cu-relay pathways. Our overall findings show that the cytoplasmic CopZ-CopA dependent Cu detoxification pathway contributes to providing Cu to CutO maturation, a process that strictly relies on cutF ., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Öztürk, Blaby-Haas, Daum, Andrei, Rauch, Daldal and Koch.)

Published
2021
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41. Cysteine Mutants of the Major Facilitator Superfamily-Type Transporter CcoA Provide Insight into Copper Import.

Author

Khalfaoui-Hassani B, Trasnea PI, Steimle S, Koch HG, and Daldal F

Subjects
Bacterial Proteins chemistry, Bacterial Proteins genetics, Biological Transport, Cysteine metabolism, Cytoplasm metabolism, Escherichia coli genetics, Escherichia coli metabolism, Homeostasis, Membrane Transport Proteins genetics, Oxidation-Reduction, Rhodobacter capsulatus genetics, Rhodobacter capsulatus metabolism, Bacterial Proteins metabolism, Copper metabolism, Cysteine genetics, Membrane Transport Proteins metabolism, Mutation
Abstract

CcoA belongs to the widely distributed bacterial copper (Cu) importer subfamily CalT ( C co A - l ike T ransporters) of the Major Facilitator Superfamily (MFS) and provides cytoplasmic Cu needed for cbb 3 -type cytochrome c oxidase ( cbb 3 -Cox) biogenesis. Earlier studies have supported a 12-transmembrane helix (TMH) topology of CcoA with the well-conserved Met 233 xxxMet 237 and His 261 xxxMet 265 motifs in its TMH7 and TMH8, respectively. Of these residues, Met 233 and His 261 are essential for Cu uptake and cbb 3 -Cox production, whereas Met 237 and Met 265 contribute partly to these processes. CcoA also contains five Cys residues of unknown role and, remarkably, its structural models predict that three of these are exposed to the highly oxidizing periplasm. Here, we first demonstrate that elimination of both Met 237 and Met 265 completely abolishes Cu uptake and cbb 3 -Cox production, indicating that CcoA requires at least one of these two Met residues for activity. Second, using scanning mutagenesis to probe plausible metal-interacting Met, His, and Cys residues of CcoA, we found that the periplasm-exposed Cys 49 located at the end of TMH2, the Cys 247 on a surface loop between TMH7 and THM8, and the C 367 located at the end of TMH11 are important for CcoA function. Analyses of the single and double Cys mutants revealed the occurrence of a disulfide bond in CcoA in vivo , possibly related to conformational changes it undergoes during Cu import as MFS-type transporter. Our overall findings suggest a model linking Cu import for cbb 3 -Cox biogenesis with a thiol:disulfide oxidoreduction step, advancing our understanding of the mechanisms of CcoA function. IMPORTANCE Copper (Cu) is a redox-active micronutrient that is both essential and toxic. Its cellular homeostasis is critical for supporting cuproprotein maturation while avoiding excessive oxidative stress. The Cu importer CcoA is the prototype of the widespread CalT subfamily of the MFS-type transporters. Hence, understanding its molecular mechanism of function is significant. Here, we show that CcoA undergoes a thiol:disulfide oxidoreduction cycle, which is important for its Cu import activity.

Published
2021
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42. Pyridinium Modified Anthracenes and Their Endoperoxides Provide a Tunable Scaffold with Activity against Gram-Positive and Gram-Negative Bacteria.

Author

Wang X, Bittner T, Milanov M, Kaul L, Mundinger S, Koch HG, Jessen-Trefzer C, and Jessen HJ

Subjects
Anthracenes pharmacology, Gram-Positive Bacteria, Microbial Sensitivity Tests, Staphylococcus epidermidis, Anti-Bacterial Agents pharmacology, Gram-Negative Bacteria
Abstract

Due to the emergence of multidrug resistant bacteria, the development of new antibiotics is required. We introduce here asymmetrically modified positively charged bis(methylpyridinium) anthracenes as a novel tunable scaffold, in which the two positive charges can be placed at a defined distance and angle. Our structure-activity relationship reveals that coupling the methylpyridiniums with alkynyl linkers to the central anthracene unit yields antibacterial compounds against a wide range of bacteria, including Escherichia coli , Staphylococcus aureus , and Staphylococcus epidermidis . Also, different mycobacteria, such as Mycobacterium smegmatis and Mycobacterium tuberculosis , are efficiently targeted by these compounds. The antibacterial activity depends on the number of alkynyl linkers and consequently also on the distance of the positive charges in the rigid anthracene scaffold. Additionally, the formation of an anthracene endoperoxide further increases the antibacterial activity, likely due to the release of toxic singlet oxygen that converts the endoperoxide back to the antibacterial anthracene scaffold with half-lives of several hours.

Published
2021
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43. The Universally Conserved ATPase YchF Regulates Translation of Leaderless mRNA in Response to Stress Conditions.

Author

Landwehr V, Milanov M, Angebauer L, Hong J, Jüngert G, Hiersemenzel A, Siebler A, Schmit F, Öztürk Y, Dannenmaier S, Drepper F, Warscheid B, and Koch HG

Abstract

The universally conserved P-loop GTPases control diverse cellular processes, like signal transduction, ribosome assembly, cell motility, and intracellular transport and translation. YchF belongs to the Obg-family of P-loop GTPases and is one of the least characterized member of this family. It is unique because it preferentially hydrolyses ATP rather than GTP, but its physiological role is largely unknown. Studies in different organisms including humans suggest a possible role of YchF in regulating the cellular adaptation to stress conditions. In the current study, we explored the role of YchF in the model organism Escherichia coli . By western blot and promoter fusion experiments, we demonstrate that YchF levels decrease during stress conditions or when cells enter stationary phase. The decline in YchF levels trigger increased stress resistance and cells lacking YchF are resistant to multiple stress conditions, like oxidative stress, replication stress, or translational stress. By in vivo site directed cross-linking we demonstrate that YchF interacts with the translation initiation factor 3 (IF3) and with multiple ribosomal proteins at the surface of the small ribosomal subunit. The absence of YchF enhances the anti-association activity of IF3, stimulates the translation of leaderless mRNAs, and increases the resistance against the endoribonuclease MazF, which generates leaderless mRNAs during stress conditions. In summary, our data identify YchF as a stress-responsive regulator of leaderless mRNA translation., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Landwehr, Milanov, Angebauer, Hong, Jüngert, Hiersemenzel, Siebler, Schmit, Öztürk, Dannenmaier, Drepper, Warscheid and Koch.)

Published
2021
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44. The Dynamic SecYEG Translocon.

Author

Oswald J, Njenga R, Natriashvili A, Sarmah P, and Koch HG

Abstract

The spatial and temporal coordination of protein transport is an essential cornerstone of the bacterial adaptation to different environmental conditions. By adjusting the protein composition of extra-cytosolic compartments, like the inner and outer membranes or the periplasmic space, protein transport mechanisms help shaping protein homeostasis in response to various metabolic cues. The universally conserved SecYEG translocon acts at the center of bacterial protein transport and mediates the translocation of newly synthesized proteins into and across the cytoplasmic membrane. The ability of the SecYEG translocon to transport an enormous variety of different substrates is in part determined by its ability to interact with multiple targeting factors, chaperones and accessory proteins. These interactions are crucial for the assisted passage of newly synthesized proteins from the cytosol into the different bacterial compartments. In this review, we summarize the current knowledge about SecYEG-mediated protein transport, primarily in the model organism Escherichia coli , and describe the dynamic interaction of the SecYEG translocon with its multiple partner proteins. We furthermore highlight how protein transport is regulated and explore recent developments in using the SecYEG translocon as an antimicrobial target., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Oswald, Njenga, Natriashvili, Sarmah and Koch.)

Published
2021
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45. Regulatory Control of Rishirilide(s) Biosynthesis in Streptomyces bottropensis .

Author

Tsypik O, Makitrynskyy R, Yan X, Koch HG, Paululat T, and Bechthold A

Abstract

Streptomycetes are well-known producers of numerous bioactive secondary metabolites widely used in medicine, agriculture, and veterinary. Usually, their genomes encode 20-30 clusters for the biosynthesis of natural products. Generally, the onset and production of these compounds are tightly coordinated at multiple regulatory levels, including cluster-situated transcriptional factors. Rishirilides are biologically active type II polyketides produced by Streptomyces bottropensis . The complex regulation of rishirilides biosynthesis includes the interplay of four regulatory proteins encoded by the rsl -gene cluster: three SARP family regulators (RslR1-R3) and one MarR-type transcriptional factor (RslR4). In this work, employing gene deletion and overexpression experiments we revealed RslR1-R3 to be positive regulators of the biosynthetic pathway. Additionally, transcriptional analysis indicated that rslR2 is regulated by RslR1 and RslR3. Furthermore, RslR3 directly activates the transcription of rslR2 , which stems from binding of RslR3 to the rslR2 promoter. Genetic and biochemical analyses demonstrated that RslR4 represses the transcription of the MFS transporter rslT4 and of its own gene. Moreover, DNA-binding affinity of RslR4 is strictly controlled by specific interaction with rishirilides and some of their biosynthetic precursors. Altogether, our findings revealed the intricate regulatory network of teamworking cluster-situated regulators governing the biosynthesis of rishirilides and strain self-immunity.

Published
2021
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46. Eeyarestatin 24 impairs SecYEG-dependent protein trafficking and inhibits growth of clinically relevant pathogens.

Author

Steenhuis M, Koningstein GM, Oswald J, Pick T, O'Keefe S, Koch HG, Cavalié A, Whitehead RC, Swanton E, High S, and Luirink J

Subjects
Anti-Bacterial Agents metabolism, Endoplasmic Reticulum metabolism, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Hydrazones chemistry, Hydroxyurea chemistry, Hydroxyurea pharmacology, Membrane Proteins metabolism, Nitroreductases metabolism, Protein Transport drug effects, SEC Translocation Channels drug effects, Hydrazones pharmacology, Hydroxyurea analogs & derivatives, SEC Translocation Channels metabolism
Abstract

Eeyarestatin 1 (ES1) is an inhibitor of endoplasmic reticulum (ER) associated protein degradation, Sec61-dependent Ca 2+ homeostasis and protein translocation into the ER. Recently, evidence was presented showing that a smaller analog of ES1, ES24, targets the Sec61-translocon, and captures it in an open conformation that is translocation-incompetent. We now show that ES24 impairs protein secretion and membrane protein insertion in Escherichia coli via the homologous SecYEG-translocon. Transcriptomic analysis suggested that ES24 has a complex mode of action, probably involving multiple targets. Interestingly, ES24 shows antibacterial activity toward clinically relevant strains. Furthermore, the antibacterial activity of ES24 is equivalent to or better than that of nitrofurantoin, a known antibiotic that, although structurally similar to ES24, does not interfere with SecYEG-dependent protein trafficking. Like nitrofurantoin, we find that ES24 requires activation by the NfsA and NfsB nitroreductases, suggesting that the formation of highly reactive nitroso intermediates is essential for target inactivation in vivo., (© 2020 The Authors. Molecular Microbiology published by John Wiley & Sons Ltd.)

Published
2021
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47. Four Phosphates at One Blow: Access to Pentaphosphorylated Magic Spot Nucleotides and Their Analysis by Capillary Electrophoresis.

Author

Haas TM, Qiu D, Häner M, Angebauer L, Ripp A, Singh J, Koch HG, Jessen-Trefzer C, and Jessen HJ

Abstract

The complex phosphorylation pattern of natural and modified pentaphosphorylated magic spot nucleotides is generated in a highly efficient way. A cyclic pyrophosphoryl phosphoramidite (cPyPA) reagent is used to introduce four phosphates on nucleosides regioselectively in a one-flask key transformation. The obtained magic spot nucleotides are used to develop a capillary electrophoresis UV detection method, enabling nucleotide assignment in complex bacterial extracts.

Published
2020
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48. SecY-mediated quality control prevents the translocation of non-gated porins.

Author

Jung S, Bader V, Natriashvili A, Koch HG, Winklhofer KF, and Tatzelt J

Subjects
Bacterial Outer Membrane Proteins metabolism, Protein Transport physiology, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Periplasm metabolism, Porins metabolism, SEC Translocation Channels metabolism
Abstract

OmpC and OmpF are among the most abundant outer membrane proteins in E. coli and serve as hydrophilic channels to mediate uptake of small molecules including antibiotics. Influx selectivity is controlled by the so-called constriction zone or eyelet of the channel. Mutations in the loop domain forming the eyelet can disrupt transport selectivity and thereby interfere with bacterial viability. In this study we show that a highly conserved motif of five negatively charged amino acids in the eyelet, which is critical to regulate pore selectivity, is also required for SecY-mediated transport of OmpC and OmpF into the periplasm. Variants with a deleted or mutated motif were expressed in the cytosol and translocation was initiated. However, after signal peptide cleavage, import into the periplasm was aborted and the mutated proteins were redirected to the cytosol. Strikingly, reducing the proof-reading capacity of SecY by introducing the PrlA4 substitutions restored transport of OmpC with a mutated channel domain into the periplasm. Our study identified a SecY-mediated quality control pathway to restrict transport of outer membrane porin proteins with a deregulated channel activity into the periplasm.

Published
2020
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49. Posttranslational insertion of small membrane proteins by the bacterial signal recognition particle.

Author

Steinberg R, Origi A, Natriashvili A, Sarmah P, Licheva M, Walker PM, Kraft C, High S, Luirink J, Shi WQ, Helmstädter M, Ulbrich MH, and Koch HG

Subjects
Amino Acid Sequence, Escherichia coli metabolism, Escherichia coli Proteins chemistry, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Models, Biological, Protein Binding, Protein Biosynthesis, Protein Transport, RNA, Messenger genetics, RNA, Messenger metabolism, SEC Translocation Channels metabolism, Membrane Proteins metabolism, Protein Processing, Post-Translational, Signal Recognition Particle metabolism
Abstract

Small membrane proteins represent a largely unexplored yet abundant class of proteins in pro- and eukaryotes. They essentially consist of a single transmembrane domain and are associated with stress response mechanisms in bacteria. How these proteins are inserted into the bacterial membrane is unknown. Our study revealed that in Escherichia coli, the 27-amino-acid-long model protein YohP is recognized by the signal recognition particle (SRP), as indicated by in vivo and in vitro site-directed cross-linking. Cross-links to SRP were also observed for a second small membrane protein, the 33-amino-acid-long YkgR. However, in contrast to the canonical cotranslational recognition by SRP, SRP was found to bind to YohP posttranslationally. In vitro protein transport assays in the presence of a SecY inhibitor and proteoliposome studies demonstrated that SRP and its receptor FtsY are essential for the posttranslational membrane insertion of YohP by either the SecYEG translocon or by the YidC insertase. Furthermore, our data showed that the yohP mRNA localized preferentially and translation-independently to the bacterial membrane in vivo. In summary, our data revealed that YohP engages an unique SRP-dependent posttranslational insertion pathway that is likely preceded by an mRNA targeting step. This further highlights the enormous plasticity of bacterial protein transport machineries., Competing Interests: The authors have declared that no competing interests exist.

Published
2020
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50. Cu Homeostasis in Bacteria: The Ins and Outs.

Author

Andrei A, Öztürk Y, Khalfaoui-Hassani B, Rauch J, Marckmann D, Trasnea PI, Daldal F, and Koch HG

Abstract

Copper (Cu) is an essential trace element for all living organisms and used as cofactor in key enzymes of important biological processes, such as aerobic respiration or superoxide dismutation. However, due to its toxicity, cells have developed elaborate mechanisms for Cu homeostasis, which balance Cu supply for cuproprotein biogenesis with the need to remove excess Cu. This review summarizes our current knowledge on bacterial Cu homeostasis with a focus on Gram-negative bacteria and describes the multiple strategies that bacteria use for uptake, storage and export of Cu. We furthermore describe general mechanistic principles that aid the bacterial response to toxic Cu concentrations and illustrate dedicated Cu relay systems that facilitate Cu delivery for cuproenzyme biogenesis. Progress in understanding how bacteria avoid Cu poisoning while maintaining a certain Cu quota for cell proliferation is of particular importance for microbial pathogens because Cu is utilized by the host immune system for attenuating pathogen survival in host cells.

Published
2020
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