TY - JOUR A1 - Reuter, Christian A1 - Hauf, Laura A1 - Imdahl, Fabian A1 - Sen, Rituparno A1 - Vafadarnejad, Ehsan A1 - Fey, Philipp A1 - Finger, Tamara A1 - Jones, Nicola G. A1 - Walles, Heike A1 - Barquist, Lars A1 - Saliba, Antoine-Emmanuel A1 - Groeber-Becker, Florian A1 - Engstler, Markus T1 - Vector-borne Trypanosoma brucei parasites develop in artificial human skin and persist as skin tissue forms JF - Nature Communications N2 - Transmission of Trypanosoma brucei by tsetse flies involves the deposition of the cell cycle-arrested metacyclic life cycle stage into mammalian skin at the site of the fly’s bite. We introduce an advanced human skin equivalent and use tsetse flies to naturally infect the skin with trypanosomes. We detail the chronological order of the parasites’ development in the skin by single-cell RNA sequencing and find a rapid activation of metacyclic trypanosomes and differentiation to proliferative parasites. Here we show that after the establishment of a proliferative population, the parasites enter a reversible quiescent state characterized by slow replication and a strongly reduced metabolism. We term these quiescent trypanosomes skin tissue forms, a parasite population that may play an important role in maintaining the infection over long time periods and in asymptomatic infected individuals. KW - mechanisms of disease KW - parasitology KW - transcriptomics Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-358142 VL - 14 ER - TY - JOUR A1 - Ramírez-Zavala, Bernardo A1 - Krüger, Ines A1 - Wollner, Andreas A1 - Schwanfelder, Sonja A1 - Morschhäuser, Joachim T1 - The Ypk1 protein kinase signaling pathway is rewired and not essential for viability in \(Candida\) \(albicans\) JF - PLoS Genetics N2 - Abstract Protein kinases are central components of almost all signaling pathways that control cellular activities. In the model organism Saccharomyces cerevisiae, the paralogous protein kinases Ypk1 and Ypk2, which control membrane lipid homeostasis, are essential for viability, and previous studies strongly indicated that this is also the case for their single ortholog Ypk1 in the pathogenic yeast Candida albicans. Here, using FLP-mediated inducible gene deletion, we reveal that C. albicans ypk1Δ mutants are viable but slow-growing, explaining prior failures to obtain null mutants. Phenotypic analyses of the mutants showed that the functions of Ypk1 in regulating sphingolipid biosynthesis and cell membrane lipid asymmetry are conserved, but the consequences of YPK1 deletion are milder than in S. cerevisiae. Mutational studies demonstrated that the highly conserved PDK1 phosphorylation site T548 in its activation loop is essential for Ypk1 function, whereas the TORC2 phosphorylation sites S687 and T705 at the C-terminus are important for Ypk1-dependent resistance to membrane stress. Unexpectedly, Pkh1, the single C. albicans orthologue of Pkh1/Pkh2, which mediate Ypk1 phosphorylation at the PDK1 site in S. cerevisiae, was not required for normal growth of C. albicans under nonstressed conditions, and Ypk1 phosphorylation at T548 was only slightly reduced in pkh1Δ mutants. We found that another protein kinase, Pkh3, whose ortholog in S. cerevisiae cannot substitute Pkh1/2, acts redundantly with Pkh1 to activate Ypk1 in C. albicans. No phenotypic effects were observed in cells lacking Pkh3 alone, but pkh1Δ pkh3Δ double mutants had a severe growth defect and Ypk1 phosphorylation at T548 was completely abolished. These results establish that Ypk1 is not essential for viability in C. albicans and that, despite its generally conserved function, the Ypk1 signaling pathway is rewired in this pathogenic yeast and includes a novel upstream kinase to activate Ypk1 by phosphorylation at the PDK1 site. Author summary Protein kinases are key components of cellular signaling pathways, and elucidating the specific roles of individual kinases is important to understand how organisms adapt to changes in their environment. The protein kinase Ypk1 is highly conserved in eukaryotic organisms and crucial for the maintenance of cell membrane homeostasis. It was previously thought that Ypk1 is essential for viability in the pathogenic yeast Candida albicans, as in the model organism Saccharomyces cerevisiae. Here, by using forced, inducible gene deletion, we reveal that C. albicans mutants lacking Ypk1 are viable but have a strong growth defect. The phenotypes of the mutants indicate that the known functions of Ypk1 are conserved in C. albicans, but loss of this kinase has less severe consequences than in S. cerevisiae. We also unravel the puzzling previous observation that C. albicans mutants lacking the Ypk1-activating kinase Pkh1, which is essential in S. cerevisiae, have no obvious growth defects. We show that the protein kinase Pkh3, which has not previously been implicated in the Ypk1 signaling pathway, can substitute Pkh1 and activate Ypk1 in C. albicans. These findings provide novel insights into this conserved signaling pathway and how it is rewired in a human-pathogenic fungus. KW - Ypk1 KW - protein kinase KW - signaling pathway KW - Candida albicans Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350076 VL - 19 IS - 8 ER - TY - THES A1 - Masota, Nelson Enos T1 - The Search for Novel Effective Agents Against Multidrug-Resistant Enterobacteriaceae T1 - Die Suche nach neuen wirksamen Wirkstoffen gegen multiresistente Enterobacteriaceae N2 - This thesis aimed at searching for new effective agents against Multidrug-Resistant Enterobacteriaceae. This is necessitated by the urgent need for new and innovative antibacterial agents addressing the critical priority pathogens prescribed by the World Health Organization (WHO). Among the available means for antibiotics discovery and development, nature has long remained a proven, innovative, and highly reliable gateway to successful antibacterial agents. Nevertheless, numerous challenges surrounding this valuable source of antibiotics among other drugs are limiting the complete realization of its potential. These include the availability of good quality data on the highly potential natural sources, limitations in methods to prepare and screen crude extracts, bottlenecks in reproducing biological potentials observed in natural sources, as well as hurdles in isolation, purification, and characterization of natural compounds with diverse structural complexities. Through an extensive review of the literature, it was possible to prepare libraries of plant species and phytochemicals with reported high potentials against Escherichia coli and Klebsiella pneumnoniae. The libraries were profiled to highlight the existing patterns and relationships between the reported antibacterial activities and studied plants’ families and parts, the type of the extracting solvent, as well as phytochemicals’ classes, drug-likeness and selected parameters for enhanced accumulation within the Gram-negative bacteria. In addition, motivations, objectives, the role of traditional practices and other crucial experimental aspects in the screening of plant extracts for antibacterial activities were identified and discussed. Based on the implemented strict inclusion criteria, the created libraries grant speedy access to well-evaluated plant species and phytochemicals with potential antibacterial activities. This way, further studies in yet unexplored directions can be pursued from the indicated or related species and compounds. Moreover, the availability of compound libraries focusing on related bacterial species serves a great role in the ongoing efforts to develop the rules of antibiotics penetrability and accumulation, particularly among Gram-negative bacteria. Here, in addition to hunting for potential scaffolds from such libraries, detailed evaluations of large pool compounds with related antibacterial potential can grant a better understanding of structural features crucial for their penetration and accumulation. Based on the scarcity of compounds with broad structural diversity and activity against Gram-negative bacteria, the creation and updating of such libraries remain a laborious but important undertaking. A Pressurized Microwave Assisted Extraction (PMAE) method over a short duration and low-temperature conditions was developed and compared to the conventional cold maceration over a prolonged duration. This method aimed at addressing the key challenges associated with conventional extraction methods which require long extraction durations, and use more energy and solvents, in addition to larger quantities of plant materials. Furthermore, the method was intended to replace the common use of high temperatures in most of the current MAE applications. Interestingly, the yields of 16 of 18 plant samples under PMAE over 30 minutes were found to be within 91–139% of those obtained from the 24h extraction by maceration. Additionally, different levels of selectivity were observed upon an analytical comparison of the extracts obtained from the two methods. Although each method indicated selective extraction of higher quantities or additional types of certain phytochemicals, a slightly larger number of additional compounds were observed under maceration. The use of this method allows efficient extraction of a large number of samples while sparing heat-sensitive compounds and minimizing chances for cross-reactions between phytochemicals. Moreover, findings from another investigation highlighted the low likelihood of reproducing antibacterial activities previously reported among various plant species, identified the key drivers of poor reproducibility, and proposed possible measures to mitigate the challenge. The majority of extracts showed no activities up to the highest tested concentration of 1024 µg/mL. In the case of identical plant species, some activities were observed only in 15% of the extracts, in which the Minimum Inhibitory Concentrations (MICs) were 4 – 16-fold higher than those in previous reports. Evaluation of related plant species indicated better outcomes, whereby about 18% of the extracts showed activities in a range of 128–512 μg/mL, some of the activities being superior to those previously reported in related species. Furthermore, solubilizing plant crude extracts during the preparation of test solutions for Antibacterial Susceptibility Testing (AST) assays was outlined as a key challenge. In trying to address this challenge, some studies have used bacteria-toxic solvents or generally unacceptable concentrations of common solubilizing agents. Both approaches are liable to give false positive results. In line with this challenge, this study has underscored the suitability of acetone in the solubilization of crude plant extracts. Using acetone, better solubility profiles of crude plant extracts were observed compared to dimethyl sulfoxide (DMSO) at up to 10 %v/v. Based on lacking toxicity against many bacteria species at up to 25 %v/v, its use in the solubilization of poorly water-soluble extracts, particularly those from less polar solvents is advocated. In a subsequent study, four galloylglucoses were isolated from the leaves of Paeonia officinalis L., whereby the isolation of three of them from this source was reported for the first time. The isolation and characterization of these compounds were driven by the crucial need to continually fill the pre-clinical antibiotics pipeline using all available means. Application of the bioautography-guided isolation and a matrix of extractive, chromatographic, spectroscopic, and spectrometric techniques enabled the isolation of the compounds at high purity levels and the ascertainment of their chemical structures. Further, the compounds exhibited the Minimum Inhibitory Concentrations (MIC) in a range of 2–256 µg/mL against Multidrug-Resistant (MDR) strains of E. coli and K. pneumonia exhibiting diverse MDR phenotypes. In that, the antibacterial activities of three of the isolated compounds were reported for the first time. The observed in vitro activities of the compounds resonated with their in vivo potentials as determined using the Galleria mellonella larvae model. Additionally, the susceptibility of the MDR bacteria to the galloylglucoses was noted to vary depending on the nature of the resistance enzymes expressed by the MDR bacteria. In that, the bacteria expressing enzymes with higher content of aromatic amino acids and zero or positive net charges were generally more susceptible. Following these findings, a plausible hypothesis for the observed patterns was put forward. The generally challenging pharmacokinetic properties of galloylglucoses limit their further development into therapeutic agents. However, the compounds can replace or reduce the use of antibiotics in livestock keeping as well as in the treatment of septic wounds and topical or oral cavity infections, among other potential uses. Using nature-inspired approaches, a series of glucovanillin derivatives were prepared following feasible synthetic pathways which in most cases ensured good yields and high purity levels. Some of the prepared compounds showed MIC values in a range of 128 – 512 μg/mL against susceptible and MDR strains of Klebsiella pneumoniae, Methicillin-Resistant Staphylococcus aureus (MRSA) and Vancomycin-Resistant Enterococcus faecium (VRE). These findings emphasize the previously reported essence of small molecular size, the presence of protonatable amino groups and halogen atoms, as well as an amphiphilic character, as crucial features for potential antibacterial agents. Due to the experienced limited success in the search for new antibacterial agents using purely synthetic means, pursuing semi-synthetic approaches as employed in this study are highly encouraged. This way, it is possible to explore broader chemical spaces around natural scaffolds while addressing their inherent limitations such as solubility, toxicity, and poor pharmacokinetic profiles. N2 - Ziel dieser Arbeit war die Suche nach neuen wirksamen Antiinfektiva gegen multiresistente Enterobacteriaceae. Grund dafür ist der dringende Bedarf an neuen und innovativen antibakteriellen Wirkstoffen gegen die von der Weltgesundheitsorganisation (WHO) als vorrangig eingestuften Krankheitserreger. Unter den verfügbaren Methoden zur Entdeckung und Entwicklung von Antibiotika ist die Natur seit langem ein bewährtes, innovatives und äußerst zuverlässiges Mittel, um erfolgreich zu antibakteriellen Wirkstoffen zu gelangen. Dennoch stehen dieser wertvollen Quelle von Antibiotika und anderen Arzneimitteln zahlreiche Herausforderungen gegenüber, die die vollständige Ausschöpfung ihres Potenzials einschränken. Dazu gehören die Verfügbarkeit qualitativ hochwertiger Daten über die hochpotenten natürlichen Quellen, Einschränkungen bei den Methoden zur Herstellung und zum Screening von Rohextrakten, Engpässe bei der Reproduktion des in natürlichen Quellen beobachteten biologischen Potenzials sowie Hürden bei der Isolierung, Reinigung und Charakterisierung von Naturstoffen mit unterschiedlicher struktureller Komplexität. Mittels einer umfassenden Durchsicht der Literatur war es möglich, Bibliotheken mit Pflanzenarten und Phytochemikalien zu erstellen, die ein hohes Potenzial gegen Escherichia coli und Klebsiella pneumnonia aufweisen. Die Bibliotheken wurden profiliert, um die bestehenden Muster und Beziehungen zwischen den berichteten antibakteriellen Aktivitäten und den untersuchten Pflanzenfamilien und -teilen, der Art des Extraktionslösungsmittels sowie den Klassen der Phytochemikalien, der Wirkstoffähnlichkeit und ausgewählten Parametern für eine verstärkte Akkumulation in den gramnegativen Bakterien aufzuzeigen. Darüber hinaus wurden Motivationen, Ziele, die Rolle traditioneller Methoden und andere wichtige experimentelle Aspekte beim Screening von Pflanzenextrakten auf antibakterielle Aktivitäten identifiziert und diskutiert. Auf der Grundlage der strengen Aufnahmekriterien bieten die erstellten Bibliotheken einen schnellen Zugang zu gut bewerteten Pflanzenarten und Phytochemikalien mit potenziellen antibakteriellen Aktivitäten. Auf diese Weise können weitere Studien in noch unerforschten Richtungen mit den angegebenen oder ähnlichen Arten und Verbindungen durchgeführt werden. Darüber hinaus spielt die Verfügbarkeit von Substanzbibliotheken, die sich auf verwandte Bakterienarten konzentrieren, eine große Rolle bei den laufenden Bemühungen, die Regeln für die Penetration und Akkumulation von Antibiotika zu entwickeln, insbesondere bei gramnegativen Bakterien. Neben der Suche nach potenziellen Molekülgerüsten aus solchen Bibliotheken können detaillierte Bewertungen großer Pools von Verbindungen mit antibakteriellem Potenzial ein besseres Verständnis der strukturellen Merkmale ermöglichen, die für ihre Penetration und Akkumulation entscheidend sind. Da es kaum Verbindungen mit breiter struktureller Vielfalt und Aktivität gegen gramnegative Bakterien gibt, ist die Erstellung und Aktualisierung solcher Bibliotheken nach wie vor ein mühsames, aber wichtiges Unterfangen. Es wurde eine schnelle mikrowellenunterstützte Extraktionsmethode unter Druck (PMAE) und bei niedrigen Temperaturen entwickelt und mit der herkömmlichen Kaltmazeration mit längerer andauernd verglichen. Mit der PMAE-Methode sollten die wichtigsten Probleme herkömmlicher Extraktionsmethoden gelöst werden, die eine lange Extraktionsdauer erfordern, mehr Energie und Lösungsmittel verbrauchen und zudem größere Mengen an Pflanzenmaterial benötigen. Darüber hinaus sollte die Methode die übliche Verwendung hoher Temperaturen in den meisten der derzeitigen MAE-Anwendungen ersetzen. Interessanterweise lag die Ausbeute von 16 der 18 Pflanzenproben bei der 30-minütigen PMAE zwischen 91 und 139 % der jenigen, die bei der 24-stündigen Extraktion durch Mazeration erzielt wurde. Darüber hinaus wurden bei einem analytischen Vergleich der mit den beiden Methoden gewonnenen Extrakte unterschiedliche Selektivitätsgrade festgestellt. Obwohl jede Methode eine selektive Extraktion größere Mengen oder zusätzlicher Arten bestimmter Phytochemikalien anzeigte, wurde bei der Mazeration eine etwas größere Anzahl an Verbindungen beobachtet. Die Anwendung dieser PMAE-Methode ermöglicht eine effiziente Extraktion einer großen Anzahl von Proben, wobei hitzeempfindliche Verbindungen geschont werden und die Wahrscheinlichkeit von Kreuzreaktionen zwischen Phytochemikalien minimiert wird. Die weitere Untersuchung von Pflanzenextraktionen haben die geringe Reproduzierbarkeit von antibakteriellen Aktivitäten, die zuvor für verschiedene Pflanzenarten berichtet wurden, aufgedeckt, die Hauptursachen für die schlechte Reproduzierbarkeit identifiziert und mögliche Maßnahmen zur Minimierung dieser Herausforderung vorgeschlagen. Die Mehrheit der Extrakte zeigte bis zur höchsten getesteten Konzentration von 1024 µg/ml keine Aktivitäten. Bei identischen Pflanzenarten wurden nur bei 15 % der Extrakte gewisse Aktivitäten beobachtet, wobei die minimalen Hemmkonzentrationen (MHK) um das Vier- bis 16-fache höher waren als in früheren Berichten. Die Auswertung verwandter Pflanzenarten zeigte geringfügig bessere Ergebnisse, wobei etwa lagen 18 % der Extrakte Aktivitäten in einem Bereich von 128-512 µg/ml aufwiesen; dabei einige der Aktivitäten über denen, die zuvor bei verwandten Arten berichtet wurden. Darüber hinaus wurde die Löslichkeit von Pflanzenrohextrakten bei der Herstellung von Testlösungen für die Bestimmung der Antimikrobischen Suszeptibilität (AST) als eine der größten Herausforderungen bezeichnet. Bei dem Versuch, diese Herausforderung zu bewältigen, wurden in einigen Studien bakterientoxische Lösungsmittel oder allgemein inakzeptable Konzentrationen gängiger Lösungsvermittler verwendet. Beide Ansätze können zu falsch-positiven Ergebnissen führen. Deshalb hat diese Studie die Eignung von Aceton für die Solubilisierung von Pflanzenrohextrakten unterstrichen. Bei Verwendung von Aceton wurden eine bessere Löslichkeit der Pflanzenrohextrakten im Vergleich zu Dimethylsulfoxid (DMSO) bei bis zu 10 % v/v beobachtet. Aufgrund der fehlenden Toxizität gegen viele Bakterienarten bei bis zu 25 % v/v wird die Verwendung von Aceton für die Solubilisierung schwer wasserlöslicher Extrakte, insbesondere solcher aus weniger polaren Lösungsmitteln, befürwortet. In der nachfolgenden Untersuchung wurden vier Galloylglucosen aus den Blättern von Paeonia officinalis L. isoliert, wobei von drei Substanzen aus dieser Quelle zum ersten Mal berichtet wurde. Die Isolierung und Charakterisierung dieser Verbindungen wurden durch die dringende Notwendigkeit vorangetrieben, die präklinische Antibiotika-Pipeline mit allen verfügbaren Methoden zu füllen. Die Anwendung der bioautographisch gesteuerten Isolierung und einer Matrix aus extraktiven, chromatographischen, spektroskopischen und spektrometrischen Techniken ermöglichte die Isolierung der Verbindungen mit hohem Reinheitsgrad und die Bestimmung ihrer chemischen Strukturen. Darüber hinaus wiesen die Verbindungen minimale Hemmkonzentrationen (MHK) in einem Bereich von 2-256 µg/ml gegen multiresistente (MDR) Stämme von E. coli und K. pneumonia auf, die verschiedene MDR-Phänotypen aufweisen. Über die antibakteriellen Aktivitäten von drei der isolierten Verbindungen wurde zum ersten Mal berichtet. Die beobachteten In-vitro-Aktivitäten der Verbindungen stimmten mit ihren In-vivo-Potenzialen überein, die anhand des Galleria mellonella-Larvenmodells ermittelt wurden. Darüber hinaus wurde festgestellt, dass die Empfindlichkeit der MDR-Bakterien gegenüber den Galloylglucosen von der Art der von den MDR-Bakterien exprimierten Resistenzenzyme abhängt. So waren die Bakterien, die Enzyme mit einem höheren Gehalt an aromatischen Aminosäuren und null oder positiven Nettoladungen exprimieren, im Allgemeinen anfälliger. Nach diesen Erkenntnissen wurde eine plausible Hypothese für die beobachteten Muster aufgestellt. Die allgemein schwierigen pharmakokinetischen Eigenschaften von Galloylglucosen schränken ihre weitere Entwicklung als therapeutischen Wirkstoffen ein. Die Verbindungen können jedoch den Einsatz von Antibiotika in der Tierhaltung sowie bei der Behandlung von septischen Wunden und Infektionen der Haut oder der Mundhöhle ersetzen oder reduzieren, neben anderen potenziellen Anwendungen. Mit von der Natur inspirierten Ansätzen wurde eine Reihe von Glucovanillin-Derivaten synthetisch hergestellt. Einige der neuen Verbindungen wiesen MHK-Werte im Bereich von 128 - 512 μg/ml gegen empfindliche und MDR-Stämme von Klebsiella pneumoniae, Methicillin-resistentem Staphylococcus aureus (MRSA) und Vancomycin-resistentem Enterococcus faecium (VRE) auf. Diese Ergebnisse unterstreichen die bereits früher berichtete Bedeutung einer kleinen Molekülgröße, des Vorhandenseins protonierbarer Aminogruppen und Halogenatome sowie eines amphiphilen Charakters als entscheidende Merkmale für potenzielle antibakterielle Wirkstoffe. Da die Suche nach neuen antibakteriellen Wirkstoffen mit rein synthetischen Mitteln bisher nur begrenzt erfolgreich war, sind halbsynthetische Ansätze, wie sie in dieser Studie verwendet wurden, sehr zu empfehlen. Auf diese Weise ist es möglich, größere chemische Räume um natürliche Molekülgerüste herum zu erforschen und gleichzeitig deren inhärente Einschränkungen wie Löslichkeit, Toxizität und schlechte pharmakokinetische Profile zu überwinden. KW - Enterobacteriaceae KW - Pflanzen KW - Synthese KW - Multidrugresistant KW - Plant extracts KW - Isolation and Characterization KW - Microwave Assisted Extraction KW - Nature-Insipired Synthesis KW - Reproducibility challenges KW - Library of Phytochemicals KW - Library of plant species KW - Plants KW - Characterization KW - Synthesis Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-302632 ER - TY - JOUR A1 - Ramírez-Zavala, Bernardo A1 - Betsova, Darina A1 - Schwanfelder, Sonja A1 - Krüger, Ines A1 - Mottola, Austin A1 - Krüger, Thomas A1 - Kniemeyer, Olaf A1 - Brakhage, Axel A. A1 - Morschhäuser, Joachim T1 - Multiple phosphorylation sites regulate the activity of the repressor Mig1 in \(Candida\) \(albicans\) JF - mSphere N2 - ABSTRACT The highly conserved heterotrimeric protein kinase SNF1 is important for metabolic adaptations in the pathogenic yeast Candida albicans. A key function of SNF1 is to inactivate the repressor protein Mig1 and thereby allow the expression of genes that are required for the utilization of alternative carbon sources when the preferred carbon source, glucose, is absent or becomes limiting. However, how SNF1 controls Mig1 activity in C. albicans has remained elusive. Using a phosphoproteomics approach, we found that Mig1 is phosphorylated at multiple serine residues. Replacement of these serine residues by nonphosphorylatable alanine residues strongly increased the repressor activity of Mig1 in cells lacking a functional SNF1 complex, indicating that additional protein kinases are involved in the regulation of Mig1. Unlike wild-type Mig1, whose levels strongly decreased when the cells were grown on sucrose or glycerol instead of glucose, the levels of a mutant Mig1 protein lacking nine phosphorylation sites remained high under these conditions. Despite the increased protein levels and the absence of multiple phosphorylation sites, cells with a functional SNF1 complex could still sufficiently inhibit the hyperactive Mig1 to enable wild-type growth on alternative carbon sources. In line with this, phosphorylated forms of the mutant Mig1 were still detected in the presence and absence of a functional SNF1, demonstrating that Mig1 contains additional, unidentified phosphorylation sites and that downstream protein kinases are involved in the control of Mig1 activity by SNF1. IMPORTANCE The SNF1 protein kinase signaling pathway, which is highly conserved in eukaryotic cells, is important for metabolic adaptations in the pathogenic yeast Candida albicans. However, so far, it has remained elusive how SNF1 controls the activity of one of its main effectors, the repressor protein Mig1 that inhibits the expression of genes required for the utilization of alternative carbon sources when glucose is available. In this study, we have identified multiple phosphorylation sites in Mig1 that contribute to its inactivation. Mutation of these sites strongly increased Mig1 repressor activity in the absence of SNF1, but SNF1 could still sufficiently inhibit the hyperactive Mig1 to enable growth on alternative carbon sources. These findings reveal features of Mig1 that are important for controlling its repressor activity. Furthermore, they demonstrate that both SNF1 and additional protein kinases regulate Mig1 in this pathogenic yeast. KW - Candida albicans KW - SNF1 KW - Mig1 KW - protein kinase KW - signaling pathway Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350060 VL - 8 IS - 6 ER - TY - JOUR A1 - Groh, Janos A1 - Abdelwahab, Tassnim A1 - Kattimani, Yogita A1 - Hörner, Michaela A1 - Loserth, Silke A1 - Gudi, Viktoria A1 - Adalbert, Robert A1 - Imdahl, Fabian A1 - Saliba, Antoine-Emmanuel A1 - Coleman, Michael A1 - Stangel, Martin A1 - Simons, Mikael A1 - Martini, Rudolf T1 - Microglia-mediated demyelination protects against CD8\(^+\) T cell-driven axon degeneration in mice carrying PLP defects JF - Nature Communications N2 - Axon degeneration and functional decline in myelin diseases are often attributed to loss of myelin but their relation is not fully understood. Perturbed myelinating glia can instigate chronic neuroinflammation and contribute to demyelination and axonal damage. Here we study mice with distinct defects in the proteolipid protein 1 gene that develop axonal damage which is driven by cytotoxic T cells targeting myelinating oligodendrocytes. We show that persistent ensheathment with perturbed myelin poses a risk for axon degeneration, neuron loss, and behavioral decline. We demonstrate that CD8\(^+\) T cell-driven axonal damage is less likely to progress towards degeneration when axons are efficiently demyelinated by activated microglia. Mechanistically, we show that cytotoxic T cell effector molecules induce cytoskeletal alterations within myelinating glia and aberrant actomyosin constriction of axons at paranodal domains. Our study identifies detrimental axon-glia-immune interactions which promote neurodegeneration and possible therapeutic targets for disorders associated with myelin defects and neuroinflammation. KW - diseases of the nervous system KW - myelin biology and repair KW - neuroimmunology Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-357641 VL - 14 ER - TY - THES A1 - Ponath, Falk Fred Finn T1 - Investigating the molecular biology of \(Fusobacterium\) \(nucleatum\) T1 - Untersuchung der Molekularbiologie von \(Fusobacterium\) \(nucleatum\) N2 - The anaerobe Fusobacterium nucleatum (F. nucleatum) is an important member of the oral microbiome but can also colonize different tissues of the human body. In particular, its association with multiple human cancers has drawn much attention. This association has prompted growing interest into the interaction of F. nucleatum with cancer, with studies focusing primarily on the host cells. At the same time, F. nucleatum itself remains poorly understood, which includes its transcriptomic architecture but also gene regulation such as global stress responses that typically enable survival of bacteria in new environments. An important aspect of such regulatory networks is the post-transcriptional regulation, which is entirely unknown in F. nucleatum. This paucity extents to any knowledge on small regulatory RNAs (sRNAs), despite their important role as post-transcriptional regulators of the bacterial physiology. Investigating the above stated aspects is further complicated by the fact that F. nucleatum is phylogenetically distant from all other bacteria, displays very limited genetic tractability and lacks genetic tools for dissecting gene function. This leaves many open questions on basic gene regulation in F. nucleatum, such as if the bacterium combines transcriptional and post-transcriptional regulation in its adaptation to a changing environment. To begin answering this question, this works elucidated the transcriptomic landscape of F. nucleatum by performing differential RNA-seq (dRNA-seq). Conducted for five representative strains of all F. nucleatum subspecies and the closely related F. periodonticum, the analysis globally uncovered transcriptional start sites (TSS), 5'untranslated regions (UTRs) and improved the existing annotation. Importantly, the dRNA-seq analysis also identified a conserved suite of sRNAs specific to Fusobacterium. The development of five genetic tools enabled further investigations of gene functions in F. nucleatum. These include vectors that enable the expression of different fluorescent proteins, inducible gene expression and scarless gene deletion in addition to transcriptional and translational reporter systems. These tools enabled the dissection of a Sigma E response and uncovered several commonalities with its counterpart in the phylogenetically distant Proteobacteria. The similarities include the upregulation of genes involved in membrane homeostasis but also a Simga E-dependent regulatory sRNA. Surprisingly, oxygen was found to activated Sigma E in F. nucleatum contrasting the typical role of the factor in envelope stress. The non-coding Sigma E-dependent sRNA, named FoxI, was shown to repress the translation of several envelope proteins which represented yet another parallel to the envelope stress response in Proteobacteria. Overall, this work sheds light on the RNA landscape of the cancer-associated bacterium leading to the discovery of a conserved global stress response consisting of a coding and a non-coding arm. The development of new genetic tools not only aided the latter discovery but also provides the means for further dissecting the molecular and infection biology of this enigmatic bacterium. N2 - Das anaerobe Bakterium Fusobacterium nucleatum (F. nucleatum) ist ein wichtiger Bestandteil des oralen Mikrobioms, kann aber auch verschiedene Gewebe des menschlichen Körpers besiedeln. Insbesondere seine Verbindung mit mehreren menschlichen Krebsarten hat viel Aufmerksamkeit auf sich gezogen. Diese Assoziation hat zu einem wachsenden Interesse an der Interaktion von F. nucleatum} mit Krebs geführt, wobei sich die Untersuchungen in erster Linie auf die Wirtszellen konzentrieren. Gleichzeitig ist F. nucleatum selbst nach wie vor schlecht verstanden, einschließlich seiner transkriptomischen Architektur, als auch der Genregulation, wie z. B. globale Stressreaktionen, die typischerweise das Überleben von Bakterien in neuen Umgebungen ermöglichen. Ein wichtiger Aspekt solcher regulatorischer Netzwerke ist die post-transkriptionelle Regulation, die bei F. nucleatum völlig unbekannt ist. Diese Unkenntnis erstreckt sich auch auf das Wissen über kleine regulatorische RNAs, trotz ihrer wichtigen Rolle als post-transkriptionelle Regulatoren der bakteriellen Physiologie. Die Untersuchung der oben genannten Aspekte wird zusätzlich durch die Tatsache erschwert, dass F. nucleatum phylogenetisch von allen anderen Bakterien weit entfernt ist, eine sehr begrenzte genetische Traktabilität aufweist und keine genetischen Werkzeuge zur Untersuchung der Genfunktion vorliegen. Dies führt zu vielen offenen Fragen bezüglich grundlegendener Genregulation in F. nucleatum, z. B. ob das Bakterium transkriptionelle und post-transkriptionelle Regulation kombiniert, um sich an eine sich verändernde Umwelt anzupassen. Als erster Schritt zur Beantwortung dieser Frage wurde in dieser Arbeit die transkriptomische Landschaft von F. nucleatum durch differential RNA-seq (dRNA-seq) aufgeklärt. Anhand von fünf repräsentativen Stämmen aller Unterarten von F. nucleatum und dem eng verwandten F. periodonticum wurden durch die Analyse global transkriptionelle Startstellen (TSS) und 5'untranslatierte Regionen (5'UTRs) aufgedeckt als auch die bestehende Annotation verbessert. Weiterhin konnte die dRNA-seq-Analyse auch eine konservierte Anzahl von Fusobacterium-spezifischen sRNAs identifizieren. Die Entwicklung von fünf genetischen Werkzeugen ermöglichte weitere Untersuchungen der Genfunktionen in F. nucleatum. Dazu gehören Vektoren, welche die Expression verschiedener fluoreszierender Proteine ermöglichen als auch Systeme für die induzierbare Genexpression, narbenlose Gendeletion sowie transkriptionelle und translationale Reportersysteme. Mit diesen Werkzeugen konnte die Sigma E Antwort entschlüsselt werden, welche mehrere Gemeinsamkeiten mit ihrem Gegenstück in den phylogenetisch entfernten Proteobakterien aufweist. Zu diesen Gemeinsamkeiten gehört die Hochregulierung von Genen, die an der Membranhomöostase beteiligt sind, aber auch eine Sigma E-abhängige regulatorische sRNA. Überraschenderweise wurde festgestellt, dass Sauerstoff Sigma E in F. nucleatum aktiviert, was im Gegensatz zu der typischen Rolle des $\sigma$-Faktors bei Membranstress steht. Die nicht-kodierende sRNA mit dem Namen FoxI, die von Sigma E abhängt, unterdrückt nachweislich die Translation verschiedener Membranproteine, was eine weitere Parallele zur Membranstressreaktion in Proteobakterien darstellt. Insgesamt wirft diese Arbeit Licht auf die RNA-Landschaft des krebsassoziierten Bakteriums und führt zur Entdeckung einer konservierten globalen Stressantwort, die aus einem kodierenden und einem nicht-kodierenden Arm besteht. Die Entwicklung neuer genetischer Werkzeuge hat nicht nur zu dieser Entdeckung beigetragen, sondern bietet auch die Möglichkeit, die Molekular- und Infektionsbiologie dieses rätselhaften Bakteriums weiter zu entschlüsseln. KW - Fusobacterium nucleatum KW - regulatory RNA KW - genetic modification KW - sigma factor Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-303516 ER - TY - JOUR A1 - Homberger, Christina A1 - Hayward, Regan J. A1 - Barquist, Lars A1 - Vogel, Jörg T1 - Improved bacterial single-cell RNA-seq through automated MATQ-seq and Cas9-based removal of rRNA reads JF - mBio N2 - Bulk RNA sequencing technologies have provided invaluable insights into host and bacterial gene expression and associated regulatory networks. Nevertheless, the majority of these approaches report average expression across cell populations, hiding the true underlying expression patterns that are often heterogeneous in nature. Due to technical advances, single-cell transcriptomics in bacteria has recently become reality, allowing exploration of these heterogeneous populations, which are often the result of environmental changes and stressors. In this work, we have improved our previously published bacterial single-cell RNA sequencing (scRNA-seq) protocol that is based on multiple annealing and deoxycytidine (dC) tailing-based quantitative scRNA-seq (MATQ-seq), achieving a higher throughput through the integration of automation. We also selected a more efficient reverse transcriptase, which led to reduced cell loss and higher workflow robustness. Moreover, we successfully implemented a Cas9-based rRNA depletion protocol into the MATQ-seq workflow. Applying our improved protocol on a large set of single Salmonella cells sampled over different growth conditions revealed improved gene coverage and a higher gene detection limit compared to our original protocol and allowed us to detect the expression of small regulatory RNAs, such as GcvB or CsrB at a single-cell level. In addition, we confirmed previously described phenotypic heterogeneity in Salmonella in regard to expression of pathogenicity-associated genes. Overall, the low percentage of cell loss and high gene detection limit makes the improved MATQ-seq protocol particularly well suited for studies with limited input material, such as analysis of small bacterial populations in host niches or intracellular bacteria. IMPORTANCE: Gene expression heterogeneity among isogenic bacteria is linked to clinically relevant scenarios, like biofilm formation and antibiotic tolerance. The recent development of bacterial single-cell RNA sequencing (scRNA-seq) enables the study of cell-to-cell variability in bacterial populations and the mechanisms underlying these phenomena. Here, we report a scRNA-seq workflow based on MATQ-seq with increased robustness, reduced cell loss, and improved transcript capture rate and gene coverage. Use of a more efficient reverse transcriptase and the integration of an rRNA depletion step, which can be adapted to other bacterial single-cell workflows, was instrumental for these improvements. Applying the protocol to the foodborne pathogen Salmonella, we confirmed transcriptional heterogeneity across and within different growth phases and demonstrated that our workflow captures small regulatory RNAs at a single-cell level. Due to low cell loss and high transcript capture rates, this protocol is uniquely suited for experimental settings in which the starting material is limited, such as infected tissues. KW - MATQ-seq KW - single-cell RNA-seq KW - Salmonella enterica KW - rRNA depletion KW - gene expression heterogeneity KW - DASH KW - Cas9 Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-350059 VL - 14 IS - 2 ER - TY - JOUR A1 - Maichl, Daniela Simone A1 - Kirner, Julius Arthur A1 - Beck, Susanne A1 - Cheng, Wen-Hui A1 - Krug, Melanie A1 - Kuric, Martin A1 - Ade, Carsten Patrick A1 - Bischler, Thorsten A1 - Jakob, Franz A1 - Hose, Dirk A1 - Seckinger, Anja A1 - Ebert, Regina A1 - Jundt, Franziska T1 - Identification of NOTCH-driven matrisome-associated genes as prognostic indicators of multiple myeloma patient survival JF - Blood Cancer Journal N2 - No abstract available. KW - cancer microenvironment KW - myeloma Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-357598 VL - 13 ER - TY - JOUR A1 - Michaux, Charlotte A1 - Gerovac, Milan A1 - Hansen, Elisabeth E. A1 - Barquist, Lars A1 - Vogel, Jörg T1 - Grad-seq analysis of Enterococcus faecalis and Enterococcus faecium provides a global view of RNA and protein complexes in these two opportunistic pathogens JF - microLife N2 - Enterococcus faecalis and Enterococcus faecium are major nosocomial pathogens. Despite their relevance to public health and their role in the development of bacterial antibiotic resistance, relatively little is known about gene regulation in these species. RNA–protein complexes serve crucial functions in all cellular processes associated with gene expression, including post-transcriptional control mediated by small regulatory RNAs (sRNAs). Here, we present a new resource for the study of enterococcal RNA biology, employing the Grad-seq technique to comprehensively predict complexes formed by RNA and proteins in E. faecalis V583 and E. faecium AUS0004. Analysis of the generated global RNA and protein sedimentation profiles led to the identification of RNA–protein complexes and putative novel sRNAs. Validating our data sets, we observe well-established cellular RNA–protein complexes such as the 6S RNA–RNA polymerase complex, suggesting that 6S RNA-mediated global control of transcription is conserved in enterococci. Focusing on the largely uncharacterized RNA-binding protein KhpB, we use the RIP-seq technique to predict that KhpB interacts with sRNAs, tRNAs, and untranslated regions of mRNAs, and might be involved in the processing of specific tRNAs. Collectively, these datasets provide departure points for in-depth studies of the cellular interactome of enterococci that should facilitate functional discovery in these and related Gram-positive species. Our data are available to the community through a user-friendly Grad-seq browser that allows interactive searches of the sedimentation profiles (https://resources.helmholtz-hiri.de/gradseqef/). KW - Enterococcus faecalis KW - Enterococcus faecium KW - Grad-seq KW - KhpB protein Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-313311 VL - 4 ER - TY - JOUR A1 - Soundararajan, Manonmani A1 - Marincola, Gabriella A1 - Liong, Olivia A1 - Marciniak, Tessa A1 - Wencker, Freya D. R. A1 - Hofmann, Franka A1 - Schollenbruch, Hannah A1 - Kobusch, Iris A1 - Linnemann, Sabrina A1 - Wolf, Silver A. A1 - Helal, Mustafa A1 - Semmler, Torsten A1 - Walther, Birgit A1 - Schoen, Christoph A1 - Nyasinga, Justin A1 - Revathi, Gunturu A1 - Boelhauve, Marc A1 - Ziebuhr, Wilma T1 - Farming practice influences antimicrobial resistance burden of non-aureus staphylococci in pig husbandries JF - Microorganisms N2 - Non-aureus staphylococci (NAS) are ubiquitous bacteria in livestock-associated environments where they may act as reservoirs of antimicrobial resistance (AMR) genes for pathogens such as Staphylococcus aureus. Here, we tested whether housing conditions in pig farms could influence the overall AMR-NAS burden. Two hundred and forty porcine commensal and environmental NAS isolates from three different farm types (conventional, alternative, and organic) were tested for phenotypic antimicrobial susceptibility and subjected to whole genome sequencing. Genomic data were analysed regarding species identity and AMR gene carriage. Seventeen different NAS species were identified across all farm types. In contrast to conventional farms, no AMR genes were detectable towards methicillin, aminoglycosides, and phenicols in organic farms. Additionally, AMR genes to macrolides and tetracycline were rare among NAS in organic farms, while such genes were common in conventional husbandries. No differences in AMR detection existed between farm types regarding fosfomycin, lincosamides, fusidic acid, and heavy metal resistance gene presence. The combined data show that husbandry conditions influence the occurrence of resistant and multidrug-resistant bacteria in livestock, suggesting that changing husbandry practices may be an appropriate means of limiting the spread of AMR bacteria on farms. KW - non-aureus staphylococci KW - NAS KW - alternative pig farming KW - antimicrobial resistance KW - one-health approach KW - intervention strategies KW - livestock-associated staphylococci KW - organic farming KW - pig farming methods Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-312750 SN - 2076-2607 VL - 11 IS - 1 ER -