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Nicotinamide adenine dinucleotide (NAD) serves as a cap-like structure on cellular RNAs (NAD-RNAs) in all domains of life including the bacterium Escherichia coli. NAD also acts as a key molecule in phage-host interactions, where bacterial immune systems deplete NAD to abort phage infection. Nevertheless, NAD-RNAs have not yet been identified during phage infections of bacteria and the mechanisms of their synthesis and degradation are unknown in this context. The T4 phage that specifically infects E. coli presents an important model to study phage infections, but a systematic analysis of the presence and dynamics of NAD-RNAs during T4 phage infection is lacking. Here, we investigate the presence of NAD-RNAs during T4 phage infection in a dual manner. By applying time-resolved NAD captureSeq, we identify NAD-capped host and phage transcripts and their dynamic regulation during phage infection. We provide evidence that NAD-RNAs are – as reported earlier – generated by the host RNA polymerase by initiating transcription with NAD at canonical transcription start sites. In addition, we characterize NudE.1 – a T4 phage-encoded Nudix hydrolase – as the first phage-encoded NAD-RNA decapping enzyme. T4 phages carrying inactive NudE.1 display a delayed lysis phenotype. This study investigates for the first time the dual epitranscriptome of a phage and its host, thereby introducing epitranscriptomics as an important field of phage research.
Interferon-stimulated gene-15 (ISG15) is an interferon-induced protein with two ubiquitin-like (Ubl) domains linked by a short peptide chain, and the conjugated protein of the ISGylation system. Similar to ubiquitin and other Ubls, ISG15 is ligated to its target proteins with a series of E1, E2, and E3 enzymes known as Uba7, Ube2L6/UbcH8, and HERC5, respectively. Ube2L6/UbcH8 plays a literal central role in ISGylation, underscoring it as an important drug target for boosting innate antiviral immunity. Depending on the type of conjugated protein and the ultimate target protein, E2 enzymes have been shown to function as monomers, dimers, or both. UbcH8 has been crystalized in both monomeric and dimeric forms, but the functional state is unclear. Here, we used a combined approach of small-angle X-ray scattering (SAXS) and nuclear magnetic resonance (NMR) spectroscopy to characterize UbcH8′s oligomeric state in solution. SAXS revealed a dimeric UbcH8 structure that could be dissociated when fused with an N-terminal glutathione S-transferase molecule. NMR spectroscopy validated the presence of a concentration-dependent monomer-dimer equilibrium and suggested a backside dimerization interface. Chemical shift perturbation and peak intensity analysis further suggest dimer-induced conformational dynamics at ISG15 and E3 interfaces - providing hypotheses for the protein′s functional mechanisms. Our study highlights the power of combining NMR and SAXS techniques in providing structural information about proteins in solution.
Interferon-stimulated gene-15 (ISG15) is an interferon-induced protein with two ubiquitin-like (Ubl) domains linked by a short peptide chain, and the conjugated protein of the ISGylation system. Similar to ubiquitin and other Ubls, ISG15 is ligated to its target proteins with a series of E1, E2, and E3 enzymes known as Uba7, Ube2L6/UbcH8, and HERC5, respectively. Ube2L6/UbcH8 plays a literal central role in ISGylation, underscoring it as an important drug target for boosting innate antiviral immunity. Depending on the type of conjugated protein and the ultimate target protein, E2 enzymes have been shown to function as monomers, dimers, or both. UbcH8 has been crystalized in both monomeric and dimeric forms, but the functional state is unclear. Here, we used a combined approach of small-angle X-ray scattering (SAXS) and nuclear magnetic resonance (NMR) spectroscopy to characterize UbcH8′s oligomeric state in solution. SAXS revealed a dimeric UbcH8 structure that could be dissociated when fused with an N-terminal glutathione S-transferase molecule. NMR spectroscopy validated the presence of a concentration-dependent monomer-dimer equilibrium and suggested a backside dimerization interface. Chemical shift perturbation and peak intensity analysis further suggest dimer-induced conformational dynamics at ISG15 and E3 interfaces - providing hypotheses for the protein′s functional mechanisms. Our study highlights the power of combining NMR and SAXS techniques in providing structural information about proteins in solution.
Interferon-stimulated gene-15 (ISG15) is an interferon-induced protein with two ubiquitin-like (Ubl) domains linked by a short peptide chain, and the conjugated protein of the ISGylation system. Similar to ubiquitin and other Ubls, ISG15 is ligated to its target proteins with a series of E1, E2, and E3 enzymes known as Uba7, Ube2L6/UbcH8, and HERC5, respectively. Ube2L6/UbcH8 plays a literal central role in ISGylation, underscoring it as an important drug target for boosting innate antiviral immunity. Depending on the type of conjugated protein and the ultimate target protein, E2 enzymes have been shown to function as monomers, dimers, or both. UbcH8 has been crystalized in both monomeric and dimeric forms, but the functional state is unclear. Here, we used a combined approach of small-angle X-ray scattering (SAXS) and nuclear magnetic resonance (NMR) spectroscopy to characterize UbcH8’s oligomeric state in solution. SAXS revealed a dimeric UbcH8 structure that could be dissociated when fused with an N-terminal glutathione S-transferase molecule. NMR spectroscopy validated the presence of a concentration-dependent monomer-dimer equilibrium and suggested a backside dimerization interface. Chemical shift perturbation and peak intensity analysis further suggest dimer-induced conformational dynamics at ISG15 and E3 interfaces - providing hypotheses for the protein’s functional mechanisms. Our study highlights the power of combining NMR and SAXS techniques in providing structural information about proteins in solution.
Interferon-stimulated gene-15 (ISG15) is an interferon-induced protein with two ubiquitin-like (Ubl) domains linked by a short peptide chain, and the conjugated protein of the ISGylation system. Similar to ubiquitin and other Ubls, ISG15 is ligated to its target proteins with a series of E1, E2, and E3 enzymes known as Uba7, Ube2L6/UbcH8, and HERC5, respectively. Ube2L6/UbcH8 plays a literal central role in ISGylation, underscoring it as an important drug target for boosting innate antiviral immunity. Depending on the type of conjugated protein and the ultimate target protein, E2 enzymes have been shown to function as monomers, dimers, or both. UbcH8 has been crystalized in both monomeric and dimeric forms, but the functional state is unclear. Here, we used a combined approach of small-angle X-ray scattering (SAXS) and nuclear magnetic resonance (NMR) spectroscopy to characterize UbcH8’s oligomeric state in solution. SAXS revealed a dimeric UbcH8 structure that could be dissociated when fused with an N-terminal glutathione S-transferase molecule. NMR spectroscopy validated the presence of a concentration-dependent monomer-dimer equilibrium and suggested a backside dimerization interface. Chemical shift perturbation and peak intensity analysis further suggest dimer-induced conformational dynamics at ISG15 and E3 interfaces - providing hypotheses for the protein’s functional mechanisms. Our study highlights the power of combining NMR and SAXS techniques in providing structural information about proteins in solution.
Interferon-stimulated gene-15 (ISG15) is an interferon-induced protein with two ubiquitin-like (Ubl) domains linked by a short peptide chain, and the conjugated protein of the ISGylation system. Similar to ubiquitin and other Ubls, ISG15 is ligated to its target proteins with a series of E1, E2, and E3 enzymes known as Uba7, Ube2L6/UbcH8, and HERC5, respectively. Ube2L6/UbcH8 plays a literal central role in ISGylation, underscoring it as an important drug target for boosting innate antiviral immunity. Depending on the type of conjugated protein and the ultimate target protein, E2 enzymes have been shown to function as monomers, dimers, or both. UbcH8 has been crystalized in both monomeric and dimeric forms, but the functional state is unclear. Here, we used a combined approach of small-angle X-ray scattering (SAXS) and nuclear magnetic resonance (NMR) spectroscopy to characterize UbcH8’s oligomeric state in solution. SAXS revealed a dimeric UbcH8 structure that could be dissociated when fused with an N-terminal glutathione S-transferase molecule. NMR spectroscopy validated the presence of a concentration-dependent monomer-dimer equilibrium and suggested a backside dimerization interface. Chemical shift perturbation and peak intensity analysis further suggest dimer-induced conformational dynamics at ISG15 and E3 interfaces - providing hypotheses for the protein’s functional mechanisms. Our study highlights the power of combining NMR and SAXS techniques in providing structural information about proteins in solution.
Interferon-stimulated gene-15 (ISG15) is an interferon-induced protein with two ubiquitin-like (Ubl) domains linked by a short peptide chain, and the conjugated protein of the ISGylation system. Similar to ubiquitin and other Ubls, ISG15 is ligated to its target proteins with a series of E1, E2, and E3 enzymes known as Uba7, Ube2L6/UbcH8, and HERC5, respectively. Ube2L6/UbcH8 plays a literal central role in ISGylation, underscoring it as an important drug target for boosting innate antiviral immunity. Depending on the type of conjugated protein and the ultimate target protein, E2 enzymes have been shown to function as monomers, dimers, or both. UbcH8 has been crystalized in both monomeric and dimeric forms, but the functional state is unclear. Here, we used a combined approach of small-angle X-ray scattering (SAXS) and nuclear magnetic resonance (NMR) spectroscopy to characterize UbcH8’s oligomeric state in solution. SAXS revealed a dimeric UbcH8 structure that could be dissociated when fused with an N-terminal glutathione S-transferase molecule. NMR spectroscopy validated the presence of a concentration-dependent monomer-dimer equilibrium and suggested a backside dimerization interface. Chemical shift perturbation and peak intensity analysis further suggest dimer-induced conformational dynamics at ISG15 and E3 interfaces - providing hypotheses for the protein’s functional mechanisms. Our study highlights the power of combining NMR and SAXS techniques in providing structural information about proteins in solution.
Targeted protein degradation (TPD) has recently emerged as an exciting new drug modality. However, the strategy of developing small molecule-based protein degraders has evolved over the past two decades and has now established molecular tags that are already in clinical use, as well as chimeric molecules, PROteolysis TArgeting Chimeras (PROTACs), based mainly on ligand systems developed for the two E3 ligases CRBN and VHL. The large size of the human E3 ligase family suggests that PROTACs can be developed by targeting a large diversity of E3 ligases, some of which have restricted expression patterns with the potential to design disease- or tissue-specific degraders. Indeed, many new E3 ligands have been published recently, confirming the druggability of E3 ligases. This review summarises recent data on E3 ligases and highlights the challenges in developing these molecules into efficient PROTACs rivalling the established degrader systems.
The Kinase Chemogenomic Set (KCGS): An open science resource for kinase vulnerability identification
(2019)
We describe the assembly and annotation of a chemogenomic set of protein kinase inhibitors as an open science resource for studying kinase biology. The set only includes inhibitors that show potent kinase inhibition and a narrow spectrum of activity when screened across a large panel of kinase biochemical assays. Currently, the set contains 187 inhibitors that cover 215 human kinases. The kinase chemogenomic set (KCGS) is the most highly annotated set of selective kinase inhibitors available to researchers for use in cell-based screens.
Die Zahl der gramnegativen Bakterien auf der WHO-Liste der Antibiotikaresistenzen hat in den letzten Jahrzehnten erheblich zugenommen. Schätzungen zufolge wird die Antibiotikaresistenz bis 2050 tödlicher sein als Krebs. Die äußere Membran gramnegativer Bakterien ist aufgrund ihres wichtigsten Strukturbestandteils, des Lipopolysaccharids (LPS), sehr anpassungsfähig an Umweltveränderungen. Das LPS macht gramnegative Bakterien von Natur aus resistent gegen viele Antibiotika und führt somit zu Antibiotikaresistenz. Der bakterielle ATP-bindende Kassettentransporter (ABC-Transporter) MsbA spielt eine entscheidende Rolle bei der Regulierung der bakteriellen Außenmembran, indem er das Kern-LPS durch ATP-Hydrolyse über die Innenmembran von gramnegativen Bakterien flockt. Darüber hinaus fungiert diese Floppase als Efflux-Pumpe, indem sie Medikamente durch die innere Membran transportiert, was sie zu einem interessanten Ziel für Medikamente macht. Vor kurzem wurden zwei verschiedene Klassen von MsbA-Inhibitoren entdeckt: (1) Tetrahydrobenzothiophene (TBT), die den LPS-Transport aufheben, und (2) Chinolinderivate, die sowohl die ATP-Hydrolyse als auch die LPS-Translokation blockieren. Darüber hinaus hat die Bestimmung der 3D-Struktur von MsbA durch Rontgen- und Kryo-EM mehrere interessante Zustände der Floppase ergeben. Die Kernspinresonanzspektroskopie ist eine hervorragende biophysikalische Methode zur Ergänzung der vorhandenen 3D-Strukturdaten. Insbesondere ermöglicht die Festkörper-NMR die Untersuchung von Membranproteinen in einer nativen Umgebung (z. B. in einer Lipiddoppelschicht). In der Vergangenheit hat unser Labor mithilfe der Festkörper-NMR einige detaillierte Mechanismen von MsbA aufgedeckt. Trotz der zahlreichen Fortschritte bei der Untersuchung der ABC-Transporterprotein-Superfamilie ist der spezifische Prozess der Substrattranslokation von MsbA noch immer unbekannt. Es wird angenommen, dass dieser Translokationsprozess über die Kopplungshelices (CHs) erfolgt, die sich zwischen der Transmembranregion (TMD) und der Nukleotidbindungsdomäne (NBD) befinden. Nukleotid-Bindungsdomäne (NBD). Zu diesem Zweck wird dem Zusammenspiel zwischen der TMD und der NBD über die CHs besondere Aufmerksamkeit gewidmet, mit dem Ziel, den Prozess der Substrattranslokation mithilfe von funktionellen Assays und Festkörper-NMR zu verstehen. Bei letzterem wurden spezifische Reporter in die CHs eingeführt, um Konformationsänderungen in 2D-spektroskopischen Daten zu verfolgen. Darüber hinaus wurde zeitaufgelöste NMR eingesetzt, um die Auswirkungen verschiedener Substrate in der TMD während der ATP-Hydrolyse in der NBD sichtbar zu machen. Die einzigartigen Reporter in den CHs haben Konformationsänderungen in bestimmten katalytischen Zuständen gezeigt. Darüber hinaus scheinen verschiedene Substrate die Kinetik der ATP-Hydrolyse zu beeinflussen. Die Ergebnisse zeigten, dass einige Substrate einen bevorzugten katalytischen Zustand innerhalb des ATP-Hydrolyse Zyklus aufweisen, der möglicherweise einen gekoppelten oder ungekoppelten Kinasemechanismus hat. Diese Ergebnisse könnten verschiedene Einblicke in die molekulare Struktur potenzieller neuer Antibiotika liefern.
G protein-coupled receptors (GPCRs) play a crucial role in modulating physiological responses and serve as the main drug target. Specifically, salmeterol and salbutamol which are used for the treatment of pulmonary diseases, exert their effects by activating the GPCR β2-adrenergic receptor (β2AR). In our study, we employed coarse-grained molecular dynamics simulations with the Martini 3 force field to investigate the dynamics of drug molecules in membranes in presence and absence of β2AR. Our simulations reveal that in more than 50% of the flip-flop events the drug molecules use the β2AR surface to permeate the membrane. The pathway along the GPCR surface is significantly more energetically favorable for the drug molecules, which was revealed by umbrella sampling simulations along spontaneous flip-flop pathways. Furthermore, we assessed the behavior of drugs with intracellular targets, such as kinase inhibitors, whose therapeutic efficacy could benefit from this observation. In summary, our results show that β2AR surface interactions can significantly enhance membrane permeation of drugs, emphasizing their potential for consideration in future drug development strategies.
The simultaneous inhibition of HDACs and BET proteins has shown promising anti-proliferative effects against different cancer types, including the difficult to treat pancreatic cancer. In this work, the strategy of concurrently targeting HDACs and BET proteins was pursued by developing different types of dual inhibitors.
By developing a novel scaffold that selectively inhibits HDAC1/2 together with BET proteins in cells, an effective tool for the investigation of pancreatic cancer, and other diseases which are sensitive to epigenetic processes, was created. The compound’s small size further gives the opportunity to further develop the inhibitor towards optimized pharmacokinetic properties, potentially resulting in a drug for cancer treatment.
A second novel approach that was pursued, was the development of a small-molecule degrader, targeting HDACs and BET proteins. Through synthesizing a variety of different molecules, a compound that was capable of lowering BRD4 levels and, at the same time, increasing histone acetylation was developed. While additional mechanistic investigations are needed to verify the degradation, the potent antiproliferative effects in pancreatic cancer cells encourage further studies following this alternative new strategy.
Molekulare Werkzeuge können in der Wissenschaft unter anderem dazu verwendet werden, biochemische Prozesse gezielt zu untersuchen, um sie somit besser zu verstehen. Dabei handelt es sich zum Beispiel, um kleine chemische Moleküle, die gezielt für ihr Anwendungsgebiet konzipiert worden sind. Mit Ihnen lassen sich z.B. Interaktionen zwischen (Makro-)Molekülen regulieren, chemische Gleichgewichte lokal verändern oder auch Botenstoffe zielgerichtet freisetzen. Die Effekte dieser temporären Einwirkung auf verschiedenste biologische Systeme können hilfreiche Erkenntnisse struktureller, funktioneller oder systematischer Art für die entsprechenden Forschungsgebiete liefern.
Um die interdisziplinären Problemstellungen zielgerichtet mit den entsprechend zugeschnittenen Werkzeugen zu adressieren, ist es dabei jedoch absolut notwendig, dass ein umfassendes und über die Grenzen der jeweiligen Fachgebiete hinaus gehendes Verständnis der jeweiligen Fragestellungen entwickelt wird.
Viele der bisher bekannten Werkzeuge benötigen für ihren Einsatz bis heute noch relativ harsche Reaktionsbedingungen, haben ein eingeschränktes Anwendungsfeld oder lassen sich nicht ausreichend Zeit- & Ortsaufgelöst „aktivieren“. Die Möglichkeit Licht als externes Trigger-Signal zu verwenden, um die entsprechenden molekularen Werkzeuge zu aktivieren (oder auch zu deaktivieren), überwindet genau diese Defizite und bringt neben der hohen zeitlichen und räumlichen Auflösung noch viele weitere Vorteile mit sich. Im Rahmen meiner Doktorarbeit ist es mir gelungen gemeinsam mit meinen Kooperationspartnern neue lichtaktivierbare molekulare Werkzeuge von Grund auf zu designen, zu synthetisieren, sie auf ihre photochemischen Eigenschaften zu untersuchen und sie anzuwenden. Durch die interdisziplinäre Zusammenarbeit mit Doktoranden aus der Organischen, Theoretischen und Physikalischen Chemie, konnte ein umfassendes Bild dieser neuen Substanzklassen aufgezeigt werden. Die verschiedenen Arten lichtaktivierbarer Werkzeuge sollen im Verlauf dieser Arbeit genauer herausgearbeitet werden. Generell kann man in drei grundlegenden Klassen von lichtaktivierbaren Werkzeugen unterscheiden: 1. irreversibel photolabile Schutzgruppen, 2. photoaktivierbare Label und 3. reversibel lichtschaltbare Photoschalter.
Auf dem Gebiet der photolabilen Schutzgruppen, auch photoaktivierbare Schutzgruppen oder Photocages genannt, ist es uns gelungen eine neue Spezies von Molekülen zu identifizieren, die dazu in der Lage sind, nach photochemischer Anregung eine spezifische Bindung innerhalb ihres molekularen Gerüsts zu spalten. Möglich gemacht wurde dies, indem wir den sog. „uncaging Prozess ganz neu gedacht“ haben und mit der Unterstützung von Theorie und Spektroskopie unsere Ergebnisse in einer Struktur-Aktivitäts-Beziehungs-Studie (SAR) festhalten konnten. Aus einer Substanzbibliothek von diversen theoretisch berechneten Kandidaten, wurden die vielversprechendsten Verbindungen anschließend synthetisiert und photochemisch charakterisiert. Nach initialen Untersuchungen und den daraus hervorgehenden Erkenntnissen, wurden weitere molekulare Struktur auf die Optimierungen der photochemischen Eigenschaften hin theoretisch berechnet und anschließend im Labor realisiert. Daraus resultierend entwickelten wir einen Photocage, der mit einer hohen Quantenausbeute mit Licht von über 450 nm photolysierbar ist und ebenfalls dazu in der Lage ist Neurotransmitter wie z.B. Glutamat zielgerichtet und lichtaktiviert freizusetzen. Eine weitere Struktur-Aktivitäts-Beziehungs-Studie wurde im Rahmen dieser Arbeit mit dem Isatin-Gerüst als potentiell neue photolabile Schutzgruppe durchgeführt.
Ebenfalls konnten in einer dritten Studie auf dem Gebiet der photolabilen Schutzgruppen Untersuchungen am Coumarin-Grundgerüst zeigen, dass eine systematische Einschränkung der Relaxationspfade im Molekül eine Verbesserung der photochemischen Eigenschaften mit sich bringen kann.
Photoaktivierbare Label werden in den verschiedensten Bereichen der Wissenschaft angewendet. Meist erlauben jedoch die chemischen Moleküle nur eine begrenzte „Beobachtungszeit“ der biochemischen Prozesse aufgrund der effizienten und damit schnellen Relaxationspfade zurück in den Grundzustand. Zu Beginn der durchgeführten Untersuchungen, bestand unsere Idee darin, die selektive Prä-IR-Anregung mit Hilfe eines UV/vis-Pulses (entsprechend der VIPER-Spektrokopie) in ein langlebiges Triplett-Signal eines geeigneten Chromophors zu überführen, welches anschließend für die Beobachtung vergleichsweise lang-lebiger biochemischer Prozesse verwendet werden könnte. Aus dieser Idee heraus entwickelten wir einen Chromophor, der neben einer Absorption im sichtbaren Bereich des elektromagnetischen Spektrums, zusätzlich eine IR-adressierbare funktionelle Gruppe, sowie die Eigenschaft, ein effizientes Inter-System-Crossing (ISC) nach photochemischer Anregung durchzuführen, besaß. Zu unserem Erstaunen zeigte dieses Derivat jedoch nach erfolgreicher Synthese nicht das erwartete Verhalten. Ein weiteres Beispiel für die hochgradige Komplexität der Photochemie.
Mit Hilfe von theoretischen und spektroskopischen Methoden konnten dennoch viele hilfreiche Erkenntnisse aus dieser Studie für zukünftige Untersuchungen aufgedeckt werden.
Ebenso war es während meiner Promotion eines der Ziele, den Schaltprozess des sog. Fulgid-Photoschalters genauer zu untersuchen und somit besser zu verstehen. Hierbei handelt es sich um ein ausgesprochen beständiges, photochemisch reversibel schaltbares Molekül, auch wenn dies vielleicht auf den ersten Blick ein Widerspruch in sich zu sein scheint. Es gelang uns diesen Photoschalter, genauer gesagt seine Photo-Isomere, auf dem Gebiet der chemischen Aktinometrie zu etablieren.
Dafür waren zahlreiche Messungen diverser Reaktivitäten (photochemische Reaktions-Quantenausbeuten) in verschiedenste Wellenlängenbereiche vom Nah-UV-Bereich bis hin zur 700 nm Grenze erforderlich. Außerdem wurden alle Werte mit der Referenzmessung einer Photodiode bzw. je nach Wellenlängenbereich auch mit der klassischen Ferri-Oxalat-Aktinometrie verglichen. Im Anschluss daran fokussierte ich mich weiter auf die einzelnen Photo-Isomere und ihre einzigartige chemische Struktur. Mit Hilfe der chiralen HPLC gelang es uns die einzelnen Photo-Isomere voneinander zu isolieren und diese mit verschiedensten photochemischen und theoretischen Methoden „genauer unter die Lupe“ zu nehmen. Die aus dieser Studie gewonnenen Erkenntnisse bereiten den Weg für diverse, zukünftige spektroskopische Anwendungen dieses Photoschalters.
The enzyme acetyl-CoA carboxylase (ACC) plays a crucial role in fatty acid metabolism. In recent years, ACC has been recognized as a promising drug target for treating different diseases. However, the role of ACC in vascular endothelial cells (ECs) has been neglected so far. To characterize the role of ACC, we used the ACC inhibitor, soraphen A, as a chemical tool, and also a gene silencing approach. We found that ACC1 was the predominant isoform in human umbilical vein ECs as well as in human microvascular ECs and that soraphen A reduced the levels of malonyl-CoA. We revealed that ACC inhibition shifted the lipid composition of EC membranes. Accordingly, membrane fluidity, filopodia formation, and migratory capacity were reduced. The antimigratory action of soraphen A depended on an increase in the cellular proportion of PUFAs and, most importantly, on a decreased level of phosphatidylglycerol. Our study provides a causal link between ACC, membrane lipid composition, and cell migration in ECs. Soraphen A represents a useful chemical tool to investigate the role of fatty acid metabolism in ECs and ACC inhibition offers a new and valuable therapeutic perspective for the treatment of EC migration-related diseases.
5-Lipoxygenase (5-LO) catalysis is positively regulated by Ca2+ ions and phospholipids that both act via the N-terminal C2-like domain of 5-LO. Previously, we have shown that 1-oleoyl-2-acetylglycerol (OAG) functions as an agonist for human polymorphonuclear leukocytes (PMNL) in stimulating 5-LO product formation. Here we have demonstrated that OAG directly stimulates 5-LO catalysis in vitro. In the absence of Ca2+ (chelated using EDTA), OAG strongly and concentration-dependently stimulated crude 5-LO in 100,000 x g supernatants as well as purified 5-LO enzyme from PMNL. Also, the monoglyceride 1-O-oleyl-rac-glycerol and 1,2-dioctanoyl-sn-glycerol were effective, whereas various phospholipids did not stimulate 5-LO. However, in the presence of Ca2+, OAG caused no stimulation of 5-LO. Also, phospholipids or cellular membranes abolished the effects of OAG. As found previously for Ca2+, OAG renders 5-LO activity resistant against inhibition by glutathione peroxidase activity, and this effect of OAG is reversed by phospholipids. Intriguingly, a 5-LO mutant lacking tryptophan residues (Trp-13, -75, and -102) important for the binding of the 5-LO C2-like domain to phospholipids was not stimulated by OAG. We conclude that OAG directly stimulates 5-LO by acting at a phospholipid binding site located within the C2-like domain.
Recently, we reported that in crude enzyme preparations, a monocyte-derived soluble protein (M-DSP) renders 5-lipoxygenase (5-LO) activity Ca2+-dependent. Here we provide evidence that this M-DSP is glutathione peroxidase (GPx)-1. Thus, the inhibitory effect of the M-DSP on 5-LO could be overcome by the GPx-1 inhibitor mercaptosuccinate and by the broad spectrum GPx inhibitor iodoacetate, as well as by addition of 13(S)-hydroperoxy-9Z,11E-octadecadienoic acid (13(S)-HPODE). Also, the chromatographic characteristics and the estimated molecular mass (80-100 kDa) of the M-DSP fit to GPx-1 (87 kDa), and GPx-1, isolated from bovine erythrocytes, mimicked the effects of the M-DSP. Intriguingly, only a trace amount of thiol (10 micro M GSH) was required for reduction of 5-LO activity by GPx-1 or the M-DSP. Moreover, the requirement of Ca2+ allowing 5-LO product synthesis in various leukocytes correlated with the respective GPx-1 activities. Mutation of the Ca2+ binding sites within the C2-like domain of 5-LO resulted in strong reduction of 5-LO activity by M-DSP and GPx-1, also in the presence of Ca2+. In summary, our data suggest that interaction of Ca2+ at the C2-like domain of 5-LO protects the enzyme against the effect of GPx-1. Apparently, in the presence of Ca2+, a low lipid hydroperoxide level is sufficient for 5-LO activation.
5-lipoxygenase (5-LO), the key enzyme in leukotriene biosynthesis, is expressed in a tissue- and cell differentiation-specific manner. The 5-LO core promoter required for basal promoter activity has a unique (G+C)-rich sequence that contains five tandem Sp1 consensus sequences. The mechanisms involved in the regulation of cell type-specific 5-LO expression are unknown. Here we show that 5-LO expression is regulated by DNA methylation. Treatment of the 5-LO-negative cell lines U937 and HL-60TB with the demethylating agent 5-aza-2'-deoxycytidine (AdC) up-regulated expression of 5-LO primary transcripts and mature mRNA in a similar fashion, indicating that AdC stimulates 5-LO gene transcription. Analysis of the methylation status of the 5-LO promoter revealed that the core promoter region was methylated in U937 and HL-60TB cells, whereas it was unmethylated in the 5-LO-positive parent HL-60 cell line. Reporter gene assays with 5-LO promoter constructs gave up to 68- and 655-fold repression of 5-LO promoter activity in HeLa and Mono Mac 6 cells by methylation. 1,25-dihydroxyvitamin D(3) and transforming growth factor-beta (TGFbeta), potent inducers of the 5-LO pathway in myeloid cell lines, increased 5-LO RNA expression in HL-60TB and U937 cells, but co-treatment with AdC was required to achieve 5-LO expression levels in HL-60TB cells that were comparable with wild-type HL-60 cells. In reporter gene assays, 1,25-dihydroxyvitamin D(3) and TGFbeta were unable to induce promoter activity when the 5-LO promoter constructs were methylated, which suggests that 5-LO promoter demethylation is a prerequisite for the high level induction of 5-LO gene expression by 1,25-dihydroxyvitamin D(3) and TGFbeta and that the effects of both agents on 5-LO mRNA expression are not related to DNA methylation.
Nukleinsäuren und Proteine bilden zusammen mit den Kohlenhydraten und Lipiden die vier großen Gruppen der Biomoleküle. Dabei setzen sich Nukleinsäuren aus einer variierenden Abfolge von Nukleotiden zusammen. Gleiches trifft auf die Proteine zu, wobei deren Bausteine als Aminosäuren bezeichnet werden. Die Reihenfolge der Bausteine bestimmt zusammen mit der Interaktion, die die einzelnen Bestandteile untereinander eingehen, deren Funktion. Um deren Wirkungsweise verstehen und nachverfolgen zu können, wurden unterschiedliche Methoden entwickelt, zu welchen auch die EPR-Spektroskopie gehört.
Durch den Einbau modifizierter Nukleotide oder Aminosäuren lassen sich Spinlabel in die sonst EPR-inaktiven Nukleinsäuren und Proteine einführen. Diese Marker lassen sich grundsätzlich in drei Klassen unterteilen (Metallionen, Nitroxidradikale und TAMs), weisen aber immer mindestens ein ungepaartes Elektronenpaar auf. Die Festphasensynthese ist eine Standardprozedur zur Herstellung von markierten Nukleinsäuren und Proteinen. Allerdings führen die Bedingungen dieser Methode zumindest teilweise zur Zersetzung der Nitroxidradikale, die dieser Arbeit zugrunde liegen, wenn sie direkt während der Synthese eingebaut werden. Der direkte Einbau ist aber in vielen Fällen essenziell, um bestimmte Eigenschaften zu erzielen.
Um den Abbau des Nitroxidradikals während der Festphasensynthese zu verhindern, kann dieses vorübergehend mit einer Schutzgruppe versehen werden, welche sich anschließend wieder abspalten lässt.
Der Schwerpunkt dieser Arbeit liegt hierbei auf der Darstellung neuer photolabil geschützter Spinlabel zur Synthese markierter Proteine und Nukleinsäuren.
Basierend auf den Nukleotiden Uridin und Cytidin konnten zwei für die RNA-Synthese vorgesehene Phosphoramidite synthetisiert werden, welche jeweils an der 5-Position des Pyrimidinrings mit einem photolabil geschützten Spinlabel auf Basis von TPA versehen waren. Durch Einbau des Uridinderivats in das Neomycin-Aptamer konnte zudem der Einfluss der Spinlabel auf die lokale Struktur mit Hilfe von in-line probing gezeigt werden.
Der gleiche TPA-Label konnte ebenfalls mit einem Lysin gekuppelt werden, welches später über ein orthogonales tRNA/Aminoacyl-tRNA Synthetase Paares in eine Polypeptid eingebaut werden sollte. In Kooperation mit dem AK Grininger ist auch ein nicht geschützter Spinlabel zur kupferfreien Markierung der Fettsäuresynthase entstanden. Abschließend war noch die Synthese eines auf Phenylalanin basierenden photolabil geschützten Spinlabel in Arbeit, welcher jedoch nicht beendet werden konnte. Dieser sollte mittels Festphasensynthese einbaubar sein, weswegen er am N-Terminus mit Fmoc geschützt ist.
Nuclear magnetic resonance (NMR) spectroscopy is a powerful and popular technique for probing the molecular structures, dynamics and chemical properties. However the conventional NMR spectroscopy is bottlenecked by its low sensitivity. Dynamic nuclear polarization (DNP) boosts NMR sensitivity by orders of magnitude and resolves this limitation. In liquid-state this revolutionizing technique has been restricted to a few specific non-biological model molecules in organic solvents. Here we show that the carbon polarization in small biological molecules, including carbohydrates and amino acids, can be enhanced sizably by in situ Overhauser DNP (ODNP) in water at room temperature and at high magnetic field. An observed connection between ODNP 13C enhancement factor and paramagnetic 13C NMR shift has led to the exploration of biologically relevant heterocyclic compound indole. The QM/MM MD simulation underscores the dynamics of intermolecular hydrogen bonds as the driving force for the scalar ODNP in a long-living radical-substrate complex. Our work reconciles results obtained by DNP spectroscopy, paramagnetic NMR and computational chemistry and provides new mechanistic insights into the high-field scalar ODNP.
Upon antibiotic stress Gram-negative pathogens deploy resistance-nodulation-cell division-type tripartite efflux pumps. These include a H+/drug antiporter module that recognizes structurally diverse substances, including antibiotics. Here, we show the 3.5 Å structure of subunit AdeB from the Acinetobacter baumannii AdeABC efflux pump solved by single-particle cryo-electron microscopy. The AdeB trimer adopts mainly a resting state with all protomers in a conformation devoid of transport channels or antibiotic binding sites. However, 10% of the protomers adopt a state where three transport channels lead to the closed substrate (deep) binding pocket. A comparison between drug binding of AdeB and Escherichia coli AcrB is made via activity analysis of 20 AdeB variants, selected on basis of side chain interactions with antibiotics observed in the AcrB periplasmic domain X-ray co-structures with fusidic acid (2.3 Å), doxycycline (2.1 Å) and levofloxacin (2.7 Å). AdeABC, compared to AcrAB-TolC, confers higher resistance to E. coli towards polyaromatic compounds and lower resistance towards antibiotic compounds.
Coronavirus disease 2019 (COVID-19) is a global pandemic posing significant health risks. The diagnostic test sensitivity of COVID-19 is limited due to irregularities in specimen handling. We propose a deep learning framework that identifies COVID-19 from medical images as an auxiliary testing method to improve diagnostic sensitivity. We use pseudo-coloring methods and a platform for annotating X-ray and computed tomography images to train the convolutional neural network, which achieves a performance similar to that of experts and provides high scores for multiple statistical indices (F1 scores > 96.72% (0.9307, 0.9890) and specificity >99.33% (0.9792, 1.0000)). Heatmaps are used to visualize the salient features extracted by the neural network. The neural network-based regression provides strong correlations between the lesion areas in the images and five clinical indicators, resulting in high accuracy of the classification framework. The proposed method represents a potential computer-aided diagnosis method for COVID-19 in clinical practice.
Single-particle tracking enables the analysis of the dynamics of biomolecules in living cells with nanometer spatial and millisecond temporal resolution. This technique reports on the mobility of membrane proteins and is sensitive to the molecular state of a biomolecule and to interactions with other biomolecules. Trajectories describe the mobility of single particles over time and provide information such as the diffusion coefficient and diffusion state. Changes in particle dynamics within single trajectories lead to segmentation, which allows to extract information on transitions of functional states of a biomolecule. Here, mean-squared displacement analysis is developed to classify trajectory segments into immobile, confined diffusing, and freely diffusing states, and to extract the occurrence of transitions between these modes. We applied this analysis to single-particle tracking data of the membrane receptor MET in live cells and analyzed state transitions in single trajectories of the un-activated receptor and the receptor bound to the ligand internalin B. We found that internalin B-bound MET shows an enhancement of transitions from freely and confined diffusing states into the immobile state as compared to un-activated MET. Confined diffusion acts as an intermediate state between immobile and free, as this state is most likely to change the diffusion state in the following segment. This analysis can be readily applied to single-particle tracking data of other membrane receptors and intracellular proteins under various conditions and contribute to the understanding of molecular states and signaling pathways.
The covalent conjugation of ubiquitin-fold modifier 1 (UFM1) to proteins generates a signal that regulates transcription, response to cell stress, and differentiation. Ufmylation is initiated by ubiquitin-like modifier activating enzyme 5 (UBA5), which activates and transfers UFM1 to ubiquitin-fold modifier-conjugating enzyme 1 (UFC1). The details of the interaction between UFM1 and UBA5 required for UFM1 activation and its downstream transfer are however unclear. In this study, we described and characterized a combined linear LC3-interacting region/UFM1-interacting motif (LIR/UFIM) within the C terminus of UBA5. This single motif ensures that UBA5 binds both UFM1 and light chain 3/γ-aminobutyric acid receptor-associated proteins (LC3/GABARAP), two ubiquitin (Ub)-like proteins. We demonstrated that LIR/UFIM is required for the full biological activity of UBA5 and for the effective transfer of UFM1 onto UFC1 and a downstream protein substrate both in vitro and in cells. Taken together, our study provides important structural and functional insights into the interaction between UBA5 and Ub-like modifiers, improving the understanding of the biology of the ufmylation pathway.
Die vorliegende Doktorarbeit beschäftigt sich mit der Untersuchung von molekularen Systemen, die aus mehreren Chromophoren bestehen und über einen Zweiphotonen-Prozess aktiviert werden können.
Die Zweiphotonen-Absorption (2PA) beschreibt die nahezu simultane Absorption zweier Photonen, deren Summe die Energie ergibt, die für den entsprechenden elektronischen Übergang nötig ist. Da für die Anregung somit zwei niederenergetische Photonen benötigt werden, kann für die 2PA Nahinfrarot-Licht (NIR-Licht) verwendet werden, welches eine geringe Phototoxizität aufweist und eine tiefe Gewebedurchdringung ermöglicht. Weiterhin wird durch die intrinsische dreidimensionale Auflösung der 2PA eine hohe Ortsauflösung der Photoaktivierung erzielt.
Photolabile Schutzgruppen (PPGs) bzw. Photocages sind chemische Verbindungen, die der vorübergehenden Maskierung der biologischen Funktion eines (Makro-)Moleküls dienen. Sie können durch Licht geeigneter Wellenlängen abgespalten werden (uncaging), wodurch die Aktivität des geschützten Substrats wiederhergestellt wird. Leider weisen viele der etablierten PPGs schlechte Zweiphotonen-Eigenschaften auf. Um die 2P-Aktivität einer PPG zu erhöhen, kann sie kovalent mit einem guten Zweiphotonen-Absorber verknüpft werden, der bei Bestrahlung das Licht über einen Zweiphotonen-Prozess absorbiert und anschließend mittels Energietransfer auf die photolabile Schutzgruppe überträgt. Dies führt schließlich zur Uncaging-Reaktion.
Im Zuge von Projekt I dieser Dissertation wurde eine solche molekulare Dyade für verbessertes Zweiphotonen-Uncaging bestehend aus einem Rhodamin-Fluorophor als Zweiphotonen-Absorber und einem Rotlicht-absorbierenden BODIPY als photolabile Schutzgruppe hergestellt und charakterisiert. Die Zweiphotonen-Aktivität des Fluorophors wurde mittels TPEF-Messungen (two-photon excited fluorescence) untersucht. Anschließend wurde das Rhodamin an einen 3,5-Distyryl-substituierten BODIPY-Photocage gekuppelt. Der Energietransfer innerhalb dieser Dyade wurde mithilfe von transienter Ultrakurzzeit-Spektroskopie und quantenmechanischen Berechnungen untersucht. Die Freisetzung der Abgangsgruppe para-Nitroanilin (PNA) bei Belichtung der Dyade konnte sowohl nach Einphotonen-Anregung des Rhodamins als auch des BODIPYs mithilfe von UV/vis-Absorptionsmessungen qualitativ nachgewiesen werden.
Da die Uncaging-Reaktion allerdings nicht besonders effektiv war, wurde für die Weiterführung des Projekts ein neuer BODIPY Photocage, der eine verbesserte Photolyse-Effizienz und eine höhere Photostabilität aufwies, verwendet und erneut an einen Rhodamin-Fluorophor geknüpft. Anhand dieser optimierten Dyade konnte die Einphotonen-Photolyse quantifiziert, d.h. eine Uncaging-Quantenausbeute für die Freisetzung von PNA bestimmt werden. Weiterhin wurde beobachtet, dass die Photolyse der Dyade mit einer deutlichen Änderung ihrer Fluoreszenzeigenschaften einherging. Dies ermöglichte einen Nachweis des Zweiphotonen-Uncagings mithilfe eines Fluoreszenzmikroskops. Die Dyaden-Moleküle wurden zur Immobilisierung in Liposomen eingeschlossen und unter dem konfokalen Fluoreszenzmikroskop belichtet. Sowohl nach Einphotonen- als auch nach Zweiphotonen-Anregung der Rhodamin-Einheit konnte die gewünschte Fluoreszenzänderung beobachtet und somit das Uncaging bestätigt werden.
In Projekt II der Dissertation wurde ein photoaktivierbarer Fluorophor (PAF) hergestellt. PAFs liegen in ihrer geschützten Form dunkel vor. Durch die Aktivierung mit Licht können sie Fluoreszenzsignale emittieren. Sie liefern somit ein direktes Feedback über die Lichtverteilung und –intensität innerhalb einer Probe und werden somit unter anderem für die Charakterisierung und Optimierung von Belichtungsapparaturen verwendet. Besonders wünschenswert ist hierbei eine Fluoreszenzaktivierung mit sichtbarem Licht bzw. mit NIR-Licht über einen Zweiphotonen-Prozess.
Im Zuge der Arbeit wurde ein Rhodamin-Derivat synthetisiert, das durch die Anbringung eines DEACM450-Photocages in seine nichtemittierende Form gezwungen wurde. Bei Bestrahlung mit 455 nm konnte die Abspaltung der Cumarin-Schutzgruppe und der damit verbundene Anstieg der Rhodamin-Fluoreszenz beobachtet und eine Uncaging-Quantenausbeute bestimmt werden. Für die Untersuchung der Zweiphotonen-Photolyse wurde der geschützte Fluorophor in einem Hydrogel immobilisiert und unter dem konfokalen Fluoreszenzmikroskop betrachtet werden. Anschließend wurden Fluoreszenzbilder vor und nach Photoanregung von bestimmten Regionen des Hydrogels aufgenommen. Durch das Uncaging der Probe konnten helle, definierte Muster geschrieben und ausgelesen werden. Die Photoaktivierung führte dabei sowohl über die Einphotonen-Anregung mit blauem Licht (488 nm) als auch über die Zweiphotonen-Anregung mit NIR-Licht (920 nm) zur Generierung von stabilen, gleichmäßigen Fluoreszenzmustern mit hohem Kontrast.
Isothermal titration calorimetry (ITC) is a widely used technique for the characterization of protein-protein and protein-ligand interactions. It provides information on the stoichiometry, affinity, and the thermodynamic driving forces of interactions. This chapter exemplifies the use of ITC to investigate interactions between human autophagy modifiers (LC3/GABARAP proteins) and their interaction partners, the LIR motif containing sequences. The purpose of this report is to present a detailed protocol for the production of LC3/GABARAP-interacting LIR peptides using E. coli expression systems. In addition, we outline the design of ITC experiments using the LC3/GABARAP:peptide interactions as an example. Comprehensive troubleshooting notes are provided to facilitate the adaptation of these protocols to different ligand-receptor systems. The methodology outlined for studying protein-ligand interactions will help to avoid common errors and misinterpretations of experimental results.
RcsF, a proposed auxiliary regulator of the regulation of capsule synthesis (rcs) phosphorelay system, is a key element for understanding the RcsC-D-A/B signaling cascade, which is responsible for the regulation of more than 100 genes and is involved in cell division, motility, biofilm formation, and virulence. The RcsC-D-A/B system is one of the most complex bacterial signal transduction pathways, consisting of several membrane-bound and soluble proteins. RcsF is a lipoprotein attached to the outer membrane and plays an important role in activating the RcsC-d-A/B pathway. The exact mechanism of activation of the rcs phosphorelay by RcsF, however, remains unknown. We have analyzed the sequence of RcsF and identified three structural elements: 1) an N-terminal membrane-anchored helix (residues 3-13), 2) a loop (residues 14-48), and 3) a C-terminal folded domain (residues 49-134). We have determined the structure of this C-terminal domain and started to investigate its interaction with potential partners. Important features of its structure are two disulfide bridges between Cys-74 and Cys-118 and between Cys-109 and Cys-124. To evaluate the importance of this RcsF disulfide bridge network in vivo, we have examined the ability of the full-length protein and of specific Cys mutants to initiate the rcs signaling cascade. The results indicate that the Cys-74/Cys-118 and the Cys-109/Cys-124 residues correlate pairwise with the activity of RcsF. Interaction studies showed a weak interaction with an RNA hairpin. However, no interaction could be detected with reagents that are believed to activate the rcs phosphorelay, such as lysozyme, glucose, or Zn(2+) ions.
Hypoxia potentiates palmitate-induced pro-inflammatory activation of primary human macrophages
(2015)
Pro-inflammatory cytokines secreted by adipose tissue macrophages (ATMs) contribute to chronic low-grade inflammation and obesity-induced insulin resistance. Recent studies have shown that adipose tissue hypoxia promotes an inflammatory phenotype in ATMs. However, our understanding of how hypoxia modulates the response of ATMs to free fatty acids within obese adipose tissue is limited. We examined the effects of hypoxia (1% O2) on the pro-inflammatory responses of human monocyte-derived macrophages to the saturated fatty acid palmitate. Compared with normoxia, hypoxia significantly increased palmitate-induced mRNA expression and protein secretion of IL-6 and IL-1β. Although palmitate-induced endoplasmic reticulum stress and nuclear factor κB pathway activation were not enhanced by hypoxia, hypoxia increased the activation of JNK and p38 mitogen-activated protein kinase signaling in palmitate-treated cells. Inhibition of JNK blocked the hypoxic induction of pro-inflammatory cytokine expression, whereas knockdown of hypoxia-induced transcription factors HIF-1α and HIF-2α alone or in combination failed to reduce IL-6 and only modestly reduced IL-1β gene expression in palmitate-treated hypoxic macrophages. Enhanced pro-inflammatory cytokine production and JNK activity under hypoxia were prevented by inhibiting reactive oxygen species generation. In addition, silencing of dual-specificity phosphatase 16 increased normoxic levels of IL-6 and IL-1β and reduced the hypoxic potentiation in palmitate-treated macrophages. The secretome of hypoxic palmitate-treated macrophages promoted IL-6 and macrophage chemoattractant protein 1 expression in primary human adipocytes, which was sensitive to macrophage JNK inhibition. Our results reveal that the coexistence of hypoxia along with free fatty acids exacerbates macrophage-mediated inflammation.
Einfache elektrochemische Methode zur Bestimmung von Chlorit in wässrigen und nicht-wässrigen Systemen Stoffe bzw. Verbindungen, welche nachweislich krebserregend oder fruchtbarkeitsschädigend sind, werden seit Jahren, insbesondere durch die WHO, streng reguliert. Zu diesen Stoffen zählt u. a. Chlorit, welches als Abbauprodukt in Desinfektionsmitteln, Poolwassern und im Rahmen von organischen Oxidationsprozessen vorkommt. Im Rahmen des Projektes sollte eine elektrochemische Methode zu Detektion von Chlorit in wässrigen und organischen Proben entwickelt werden, wobei auf eine Glaskohlenstoffelektrode in Kombination mit Li [NTf]2 im Wässrigen und [Bmpyrr][NTf]2/MeOH im Organischen als Elektrolyten zurückgegriffen wurden.
Bei der Methodenentwicklung wurde auf Differentielle-Puls-Voltammetrie zurückgegriffen, da diese im Vergleich zum Cyclovoltammetrie deutlich empfindlicher ist. Die Methodenvalidierung nach ICH-Guidelines konnte erfolgreich durchgeführt werden Dabei konnte im Wässrigen eine Nachweisgrenze von 0.07 mg L-1 (Organisch: 0.20 mg L-1) erhalten werden. Beide lagen deutlich unter den WHO-Grenzwerten von 0.7 mg L-1. Die Selektivität/Interferenz wurde gegenüber den übrigen Chlor-Spezies getestet; für alle Spezies, außer Hypochlorit, konnten für die Wiederfindungsrate von Chlorit Werte nahe 100% erhalten werden. Die entwickelte Methode konnte erfolgreich auf wässrige (Poolproben, Desinfektionsmittel) und organische Proben (aus Pinnick-Synthesen) angewendet werden. Insbesondere durch die Anwendung im Bereich der Pinnick-Oxidation war der Sensor für mögliche In-Line-Analytik geeignet. Bei den organischen Proben konnte zudem die ionische Flüssigkeit zu 92% zurückgewonnen werden, was den Elektrolyten in Hinblick auf Nachhaltigkeit und Wirtschaftlichkeit noch attraktiver macht.
Entwicklung ionenchromatographischer Methoden zur Detektion von Chloroxo-Spezies
Der Bedarf an schnellen, kostengünstigen Analysemethoden, welche den Vorgaben der einzelnen Behörden weltweit entsprechen, ist in den letzten Jahren enorm gestiegen. Im Rahmen des Projektes sollte eine ionenchromatographische Methode (IC) entwickelt werden, welche neben den Chloroxo-Spezies (Chlorid, Hypochlorit, Chlorit, Chlorat und Perchlorat) auch die bekannten Standardionen (Fluorid, Bromid, Nitrat, Phosphat, Sulfat, Iodid) nachweisbar macht. Zunächst gelang es, die Methodenparameter zu optimieren und so die Chloro-Spezies, außer Hypochlorit, von den übrigen Standardanionen innerhalb von 50 Minuten vollständig zu trennen. Die Methode konnte in der weiteren Entwicklung sogar noch um die Detergenzien-Anionen Acetat, Formiat, Oxalat und Tartrat erweitert werden. (ASupp 7, 45 °C, 0.8 mL min-1, 6 mmol L-1 Na2CO3 / 1 mmol L-1 NaHCO3 + 10% Acetonitril). Auch alle notwendigen Validierungsparameter konnten erfolgreich bestimmt werden. Zuletzt war es möglich, erfolgreich unterschiedliche Realproben zu vermessen.
Da ein Nachweis von Hypochlorit mittels IC nicht möglich war, wurden weitere Anstrengung unternommen, dieses Anion mittels IC-PCR (Nachsäulenderivatisierung) nachzuweisen. Als Detektionsprinzip wurde dabei auf eine Bromat-Nachweis-Methode mittels UV/VIS zurückgegriffen, welche im Rahmen des Projektes angepasst wurde. Da davon ausgegangen werden muss, dass das Hypochlorit mit reaktiven Stellen innerhalb des Säulenmaterials reagiert und somit nicht mehr detektiert werden kann, wurden Passivierungsexperimente an der Vorsäule und Säule für 24 h mit einer Hypochlorit-NaOH-Mischung durchgeführt. Nach 60 Stunden Passivierung konnten erstmals reproduzierbare Ergebnisse bei dem Nachweis von OCl- erhalten werden. Zuletzt konnten erfolgreich fünf unterschiedliche Realproben vermessen und der Hypochlorit-Gehalt mit bisher angewandten Methoden verglichen werden, wobei die erhaltenen Werte in der gleichen Größenordnung lagen.
Entwicklung eines Sensors unter Verwendung der Viologen-Grundstruktur auf metallischen Oberflächen
Früher fanden Viologene und deren Derivate Anwendung im Bereich der Schädlingsbekämpfung und wurden hauptsächlich als Kontaktherbizid verwendet. Mittlerweile hat sich das Anwendungsspektrum der Viologene deutlich verändert, u.a. werden die in organischen Redox-Fluss-Batterien als Elektrolyte eingesetzt. Im Rahmen diesen Projekts wurden mehrere bekannte Viologen-Grundkörper (u. A. Methylviologen (MV)) vollständig elektrochemisch charakterisiert Im Anschluss wurde MV mit unterschiedlichen Ankergruppen (Thiol-, Sulfonat, -Phosphonat-, Carboxylanker) modifiziert und auf metallische Oberfläche (u. A. Gold und Kupfer) abgeschieden mit dem Ziel ein neues Sensor-Motiv für die Analytik zu entwickeln. Der Thiolanker konnte erfolgreich auf Gold, der Carboxylanker erfolgreich auf Kupfer abgeschieden werden. Die anschließenden elektrochemischen Untersuchungen der abgeschiedenen Monolagen ergaben jedoch eine geringe Stabilität der Anker in wässriger und organischer Umgebung, sodass in Zukunft weitere Anstrengungen unternommen werden müssen, die Stabilität des Viologensystems auf der Oberfläche zu verbessern.
Glucokinase (GK) is a key enzyme of glucose metabolism in liver and pancreatic beta-cells, and small molecule activators of GK (GKAs) are under evaluation for the treatment of type 2 diabetes. In liver, GK activity is controlled by the GK regulatory protein (GKRP), which forms an inhibitory complex with the enzyme. Here, we performed isothermal titration calorimetry and surface plasmon resonance experiments to characterize GK-GKRP binding and to study the influence that physiological and pharmacological effectors of GK have on the protein-protein interaction. In the presence of fructose-6-phosphate, GK-GKRP complex formation displayed a strong entropic driving force opposed by a large positive enthalpy; a negative change in heat capacity was observed (Kd = 45 nm, DeltaH = 15.6 kcal/mol, TDeltaS = 25.7 kcal/mol, DeltaCp = -354 cal mol(-1) K(-1)). With k(off) = 1.3 x 10(-2) s(-1), the complex dissociated quickly. The thermodynamic profile suggested a largely hydrophobic interaction. In addition, effects of pH and buffer demonstrated the coupled uptake of one proton and indicated an ionic contribution to binding. Glucose decreased the binding affinity between GK and GKRP. This decrease was potentiated by an ATP analogue. Prototypical GKAs of the amino-heteroaryl-amide type bound to GK in a glucose-dependent manner and impaired the association of GK with GKRP. This mechanism might contribute to the antidiabetic effects of GKAs.
The β-subunits of Na,K-ATPase and H,K-ATPase have important functions in maturation and plasma membrane targeting of the catalytic α-subunit but also modulate the transport activity of the holoenzymes. In this study, we show that tryptophan replacement of two highly conserved tyrosines in the transmembrane domain of both Na,K- and gastric H,K-ATPase β-subunits resulted in considerable shifts of the voltage-dependent E1P/E2P distributions toward the E1P state as inferred from presteady-state current and voltage clamp fluorometric measurements of tetramethylrhodamine-6-maleimide-labeled ATPases. The shifts in conformational equilibria were accompanied by significant decreases in the apparent affinities for extracellular K+ that were moderate for the Na,K-ATPase β-(Y39W,Y43W) mutation but much more pronounced for the corresponding H,K-ATPase β-(Y44W,Y48W) variant. Moreover in the Na,K-ATPase β-(Y39W,Y43W) mutant, the apparent rate constant for reverse binding of extracellular Na+ and the subsequent E2P-E1P conversion, as determined from transient current kinetics, was significantly accelerated, resulting in enhanced Na+ competition for extracellular K+ binding especially at extremely negative potentials. Analogously the reverse binding of extracellular protons and subsequent E2P-E1P conversion was accelerated by the H,K-ATPase β-(Y44W,Y48W) mutation, and H+ secretion was strongly impaired. Remarkably tryptophan replacements of residues in the M7 segment of Na,K- and H,K-ATPase α-subunits, which are at interacting distance to the β-tyrosines, resulted in similar E1 shifts, indicating their participation in stabilization of E2. Thus, interactions between selected residues within the transmembrane regions of α- and β-subunits of P2C-type ATPases exert an E2-stabilizing effect, which is of particular importance for efficient H+ pumping by H,K-ATPase under in vivo conditions.
The Na+/K+-ATPase maintains the physiological Na+ and K+ gradients across the plasma membrane in most animal cells. The functional unit of the ion pump is comprised of two mandatory subunits including the α-subunit, which mediates ATP hydrolysis and ion translocation, as well as the β-subunit, which acts as a chaperone to promote proper membrane insertion and trafficking in the plasma membrane. To examine the conformational dynamics between the α- and β-subunits of the Na+/K+-ATPase during ion transport, we have used fluorescence resonance energy transfer, under voltage clamp conditions on Xenopus laevis oocytes, to differentiate between two models that have been proposed for the relative orientation of the α- and β-subunits. These experiments were performed by measuring the time constant of irreversible donor fluorophore destruction with fluorescein-5-maleimide as the donor fluorophore and in the presence or absence of tetramethylrhodamine-6-maleimide as the acceptor fluorophore following labeling on the M3-M4 or M5-M6 loop of the α-subunit and the β-subunit. We have also used fluorescence resonance energy transfer to investigate the relative movement between the two subunits as the ion pump shuttles between the two main conformational states (E1 and E2) as described by the Albers-Post scheme. The results from this study have identified a model for the orientation of the β-subunit in relation to the α-subunit and suggest that the α- and β-subunits move toward each other during the E2 to E1 conformational transition.
Macrophages respond to the Th2 cytokine IL-4 with elevated expression of arachidonate 15-lipoxygenase (ALOX15). Although IL-4 signaling elicits anti-inflammatory responses, 15-lipoxygenase may either support or inhibit inflammatory processes in a context-dependent manner. AMP-activated protein kinase (AMPK) is a metabolic sensor/regulator that supports an anti-inflammatory macrophage phenotype. How AMPK activation is linked to IL-4-elicited gene signatures remains unexplored. Using primary human macrophages stimulated with IL-4, we observed elevated ALOX15 mRNA and protein expression, which was attenuated by AMPK activation. AMPK activators, e.g. phenformin and aminoimidazole-4-carboxamide 1-β-d-ribofuranoside inhibited IL-4-evoked activation of STAT3 while leaving activation of STAT6 and induction of typical IL-4-responsive genes intact. In addition, phenformin prevented IL-4-induced association of STAT6 and Lys-9 acetylation of histone H3 at the ALOX15 promoter. Activating AMPK abolished cellular production of 15-lipoxygenase arachidonic acid metabolites in IL-4-stimulated macrophages, which was mimicked by ALOX15 knockdown. Finally, pretreatment of macrophages with IL-4 for 48 h increased the mRNA expression of the proinflammatory cytokines IL-6, IL-12, CXCL9, and CXCL10 induced by subsequent stimulation with lipopolysaccharide. This response was attenuated by inhibition of ALOX15 or activation of AMPK during incubation with IL-4. In conclusion, limiting ALOX15 expression by AMPK may promote an anti-inflammatory phenotype of IL-4-stimulated human macrophages.
By translocating proteasomal degradation products into the endoplasmic reticulum for loading of major histocompatibility complex I molecules, the ABC transporter TAP plays a focal role in the adaptive immunity against infected or malignantly transformed cells. A key question regarding the transport mechanism is how the quality of the incoming peptide is detected and how this information is transmitted to the ATPase domains. To identify residues involved in this process, we evolved a Trojan horse strategy in which a small artificial protease is inserted into antigenic epitopes. After binding, the TAP backbone in contact is cleaved, allowing the peptide sensor site to be mapped by mass spectrometry. Within this sensor site, we identified residues that are essential for tight coupling of peptide binding and transport. This sensor and transmission interface is restructured during the ATP hydrolysis cycle, emphasizing its important function in the cross-talk between the transmembrane and the nucleotide-binding domains. This allocrite sensor may be similarly positioned in other members of the ABC exporter family.
Biogenesis of mitochondrial cytochrome c oxidase (COX) relies on a large number of assembly factors, among them the transmembrane protein Surf1. The loss of human Surf1 function is associated with Leigh syndrome, a fatal neurodegenerative disorder caused by severe COX deficiency. In the bacterium Paracoccus denitrificans, two homologous proteins, Surf1c and Surf1q, were identified, which we characterize in the present study. When coexpressed in Escherichia coli together with enzymes for heme a synthesis, the bacterial Surf1 proteins bind heme a in vivo. Using redox difference spectroscopy and isothermal titration calorimetry, the binding of the heme cofactor to purified apo-Surf1c and apo-Surf1q is quantified: Each of the Paracoccus proteins binds heme a in a 1:1 stoichiometry and with Kd values in the submicromolar range. In addition, we identify a conserved histidine as a residue crucial for heme binding. Contrary to most earlier concepts, these data support a direct role of Surf1 in heme a cofactor insertion into COX subunit I by providing a protein-bound heme a pool.
Biological membranes are complex and dynamic assemblies of lipids and proteins. Poikilothermic organisms including bacteria, fungi, reptiles, and fish do not control their body temperature and must adapt their membrane lipid composition in order to maintain membrane fluidity in the cold. This adaptive response was termed homeoviscous adaptation and has been frequently studied with a specific focus on the acyl chain composition of membrane lipids. Mass spectrometry-based lipidomics can nowadays provide more comprehensive insights into the complexity of lipid remodeling during adaptive responses. Eukaryotic cells compartmentalize biochemical processes in organelles with characteristic surface properties, and the lipid composition of organelle membranes must be tightly controlled in order to maintain organelle function and identity during adaptive responses. Some highly differentiated cells such as neurons maintain unique lipid compositions with specific physicochemical properties. To date little is known about the sensory mechanisms regulating the acyl chain profile in such specialized cells or during adaptive responses. Here we summarize our current understanding of lipid metabolic networks with a specific focus on the role of physicochemical membrane properties for the regulation of the acyl chain profile during homeoviscous adaptation. By comparing the mechanisms of the bacterial membrane sensors with the prototypical eukaryotic lipid packing sensor Mga2 from Saccharomyces cerevisiae, we identify common operational principles that might guide our search for novel membrane sensors in different organelles, organisms, and highly specialized cells.
We demonstrated previously that 5-lipoxygenase (5-LO), a key enzyme in leukotriene biosynthesis, can be phosphorylated by p38 MAPK-regulated MAPKAP kinases (MKs). Here we show that mutation of Ser-271 to Ala in 5-LO abolished MK2 catalyzed phosphorylation and clearly reduced phosphorylation by kinases prepared from stimulated polymorphonuclear leukocytes and Mono Mac 6 cells. Compared with heat shock protein 27 (Hsp-27), 5-LO was a weak substrate for MK2. However, the addition of unsaturated fatty acids (i.e. arachidonate 1-50 microm) up-regulated phosphorylation of 5-LO, but not of Hsp-27, by active MK2 in vitro, resulting in a similar phosphorylation as for Hsp-27. 5-LO was phosphorylated also by other serine/threonine kinases recognizing the motif Arg-Xaa-Xaa-Ser (protein kinase A, Ca(2+)/calmodulin-dependent kinase II), but these activities were not increased by fatty acids. HeLa cells expressing wild type 5-LO or S271A-5-LO, showed prominent 5-LO activity when incubated with Ca(2+)-ionophore plus arachidonate. However, when stimulated with only exogenous arachidonic acid, activity for the S271A mutant was significantly lower as compared with wild type 5-LO. It appears that phosphorylation at Ser-271 is more important for 5-LO activity induced by a stimulus that does not prominently increase intracellular Ca(2+) and that arachidonic acid stimulates leukotriene biosynthesis also by promoting this MK2-catalyzed phosphorylation.
Malfunction of the actin cytoskeleton is linked to numerous human diseases including neurological disorders and cancer. LIMK1 (LIM domain kinase 1) and its paralogue LIMK2 are two closely related kinases that control actin cytoskeleton dynamics. Consequently, they are potential therapeutic targets for the treatment of such diseases. In the present review, we describe the LIMK conformational space and its dependence on ligand binding. Furthermore, we explain the unique catalytic mechanism of the kinase, shedding light on substrate recognition and how LIMK activity is regulated. The structural features are evaluated for implications on the drug discovery process. Finally, potential future directions for targeting LIMKs pharmacologically, also beyond just inhibiting the kinase domain, are discussed.
Epigenetic control of microsomal prostaglandin E synthase-1 by HDAC-mediated recruitment of p300
(2017)
Nonsteroidal anti-inflammatory drugs are the most widely used medicine to treat pain and inflammation, and to inhibit platelet function. Understanding the expression regulation of enzymes of the prostanoid pathway is of great medical relevance. Histone acetylation crucially controls gene expression. We set out to identify the impact of histone deacetylases (HDACs) on the generation of prostanoids and examine the consequences on vascular function. HDAC inhibition (HDACi) with the pan-HDAC inhibitor, vorinostat, attenuated prostaglandin (PG)E2 generation in the murine vasculature and in human vascular smooth muscle cells. In line with this, the expression of the key enzyme for PGE2 synthesis, microsomal PGE synthase-1 (PTGES1), was reduced by HDACi. Accordingly, the relaxation to arachidonic acid was decreased after ex vivo incubation of murine vessels with HDACi. To identify the underlying mechanism, chromatin immunoprecipitation (ChIP) and ChIP-sequencing analysis were performed. These results suggest that HDACs are involved in the recruitment of the transcriptional activator p300 to the PTGES1 gene and that HDACi prevented this effect. In line with the acetyltransferase activity of p300, H3K27 acetylation was reduced after HDACi and resulted in the formation of heterochromatin in the PTGES1 gene. In conclusion, HDAC activity maintains PTGES1 expression by recruiting p300 to its gene.
Der Fokus der Arbeit liegt auf der Untersuchung von Wechselwirkungen zwischen Molekülen in selbst-anordnenden Monolagen (SAMs) auf Goldoberflächen mittels Rastertunnelmikroskopie und komplementären Methoden wie z.B. Infrarot-Reflektions-Absorptions-Spektro-skopie.
In dieser Arbeit wurde das kürzlich etablierte Konzept von eingebetteten Dipolmomenten in aromatischen, SAM-bildenden Molekülen eingehender untersucht. Das Ausmaß des Dipol-moments und die Größe der SAM-bildenden Moleküle wurden synthetisch variiert und der Einfluss auf die Struktur und elektronischen Eigenschaften der SAMs untersucht. Binäre, gemischte Monolagen aus SAM-bildenden Molekülen mit "entgegen gerichteten", Dipolmomenten wurden hergestellt und charakterisiert. Zur Herstellung der binären, gemischten Monolagen wurden zwei Methoden verwendet: die Monolagen wurden a) aus bereits gemischten Lösungen der Moleküle abgeschieden oder b) eine reine SAM in die Lösung des anderen Moleküls eingelegt, so dass ein Austausch stattfand. Der Vergleich der beiden Methoden ermöglicht Rückschlüsse über die Abscheidungsprozesse. Die Charakterisierung der SAMs dieser Mischungsreihen gab Aufschluss über Eigenschaften wie Packungsdichte, Austrittsarbeit, elektronischen Ladungstransport in Monolagen und Orientierung der Moleküle relativ zur Oberfläche und erlaubte Schlussfolgerungen über die Mischbarkeit und das Ausmaß der Dipolwechselwirkungen der Moleküle in der Monolage. In einem ähnlichen Ansatz zu dem oben beschriebenen Vorgehen wurden Quadrupolwechselwirkungen zwischen SAM-bildenen, Benzol-, Naphtalin- und Anthracenderivaten untersucht. In Mischungsreihen wurden SAMs von nicht- und teilweise (hoch)fluorierten, SAM-bildenden Molekülen auf Goldoberflächen charakterisiert. Die Ergebnisse der Untersuchungen können bei der gezielten Einstellung der elektronischen Eigenschaften in elektronischen Bauteilen wie OFETs Anwendung finden.
In einem weiteren Projekt wurde der Einfluss von polaren Endgruppen auf die in situ Abspaltung von Schutzgruppen an Terphenylthiol-Derivaten untersucht, wobei die Ergebnisse zum Aufbau größerer, aus organischer Elektronik bestehender, Netzwerke verwendet werden können.
The role of USP22 in nucleic acid sensing pathways and interferon-induced necroptotic cell death
(2023)
Every day, living organisms are challenged by internal and external factors that threaten to bring imbalance to their tightly regulated systems and disrupt homeostasis, leading to degeneration, and ultimately death. More than ever, we face the challenge of combating diseases such as COVID-19 caused by infection with the SARS-CoV-2 coronavirus. It is therefore crucial to identify host factors that control antiviral defense mechanisms. In addition, in the fight against cancer, it is becoming increasingly important to identify markers that could be used for targeted therapy to influence cellular processes and determine cell fate.
As a deubiquitylating enzyme, ubiquitin specific peptidase 22 (USP22) mediates the removal of the small molecule ubiquitin, which is post-translationally added to target proteins, thereby regulating several important processes such as protein degradation, activation or localization. Through its deubiquitylating function, USP22 controls several biological processes such as cell cycle regulation, proliferation and cancer immunoresistance by modulating key proteins involved in these pathways. Lately, USP22 was reported to positively regulate TNFα-mediated necroptosis, an inflammatory type of programmed cell death, in various human tumor cell lines by affecting RIPK3 phosphorylation. In addition, USP22 as a part of the Spt-Ada-Gcn5 acetyltransferase (SAGA) transcription complex is known to regulate gene expression by removing ubiquitin from histones H2A and H2B. However, little is known about the role of USP22 in global gene expression.
In this study, we performed a genome-wide screen in the human colon carcinoma cell line HT-29 and identified USP22 as a key negative regulator of basal interferon (IFN) expression. We further demonstrated that the absence of USP22 results in increased STING activity and ubiquitylation, both basally and in response to stimulation with the STING agonist 2'3'-cGAMP, thereby affecting IFNλ1 expression and basal expression of antiviral ISGs. In addition, we were able to establish USP22 as a critical host factor in controlling SARS-CoV-2 infection by regulating infection, replication, and the generation of infectious virus particles, which we attribute in part to its role in regulating STING signaling.
In the second part of the study, we connected the findings of USP22-dependent regulation of IFN signaling and TNFα-induced necroptosis and investigated the role of USP22 during necroptosis induced by the synergistic action of IFN and the Smac mimetic BV6 in caspase-deficient settings. We identified USP22 as a negative regulator of IFN-induced necroptosis, which does not depend on STING expression, but relies on a yet unknown mechanism.
In summary, we identify USP22 as an important regulator of IFN signaling with important implications for the defense against viral infections and regulation of the necroptotic pathway that could be exploited for devising targeted therapeutic strategies against viral infections and related diseases like COVID-19, and advancing precision medicine in cancer treatment.
The accumulation and distribution of characteristic secondary products in the different organs of an Aloe plant (A. succotrina Lam.) were studied by high performance liquid chromatography for the first time. In the leaves of the Aloe plant, only anthrone-C-glycosyls of the 7-hydroxyaloin type and, for the first time in plant material, the free anthraquinone 7-hydroxyaloeemodin were found. In contrast to previous reports on the distribution of secondary products in Aloe plants, anthrone-C-glycosyls were also detected in flowers, bracts and the inflorescence axis of the species examined. Aloesaponol I, a tetrahydroanthracene aglycone, was only present in the underground organs and in the stem. The 2-alkylchromone-C-glucosyl aloeresin B showed no specific occurrence as it was found in every type of organ. Based on these results and the findings of recent studies on Aloe roots and flowers, a distribution scheme of polyketide types in the Aloe plant was established. It suggests a separate and independent anthranoid metabolism for underground Aloe organs and stem on the one hand, and for leaves and inflorescence organs on the other hand. In the latter structures anthranoid metabolism seems to be additionally compartmentalized as the anthranoid pro files of inflorescence organs and leaves differ in two points relevant to anthranoid biosynthe sis: firstly, the occurrence of anthrone aglycones and secondly, the individual content of corresponding anthrone-C-glucosyl diastereomers.
From the leaf exudate of Aloe lateritia ENGLER the C-glucosyl com pounds homonataloin, aloeresin A and aloesin (synon. aloeresin B) were isolated together with the anthraquinone nataloeem odin-8-methylether and spectroscopically identified. Hom onataloin, widely distributed in Aloe species, was separated into homonataloin A and B by combined TLC and DCCC. In their 1 D and 2D 1H NMR spectra only the shifts of the 2′-hydroxyl protons of both glucosyl residues differ significantly, indicative of 10 S (A) resp. 10 S (B) configurations. In both com pounds the anthrone is in β-position of the D-glucopyranosyl, as determined by the large coupling constants of the anomeric protons. The 13C NMR signals are unambiguously assigned by the use of DEPT, APT and gated-decoupling methods. Only the chemical shifts of C -11 and C -14 show significant differences between both diastereomers due to the adjacent 2′-sugar hydroxyls. The two homonataloins differ mostly in optical rotation and circulardichroism due to different configurations at C - 10 of the anthrone part. The absolute configurations of the diastereomers are determined by correlation of their CD spectra with the CD spectra of the structural analogues 7-hydroxyaloins A and B, which shows that hom onataloin A is the 10 S, 1′S-compound and that homonataloin B has 10 R, 1′S-configuration.
To better understand the role of sphingolipids in the multifactorial process of inflammatory bowel disease (IBD), we elucidated the role of CerS4 in colitis and colitis-associated cancer (CAC). For this, we utilized the azoxymethane/dextran sodium sulphate (AOM/DSS)-induced colitis model in global CerS4 knockout (CerS4 KO), intestinal epithelial (CerS4 Vil/Cre), or T-cell restricted knockout (CerS4 LCK/Cre) mice. CerS4 KO mice were highly sensitive to the toxic effect of AOM/DSS, leading to a high mortality rate. CerS4 Vil/Cre mice had smaller tumors than WT mice. In contrast, CerS4 LCK/Cre mice frequently suffered from pancolitis and developed more colon tumors. In vitro, CerS4-depleted CD8+ T-cells isolated from the thymi of CerS4 LCK/Cre mice showed impaired proliferation and prolonged cytokine production after stimulation in comparison with T-cells from WT mice. Depletion of CerS4 in human Jurkat T-cells led to a constitutively activated T-cell receptor and NF-κB signaling pathway. In conclusion, the deficiency of CerS4 in T-cells led to an enduring active status of these cells and prevents the resolution of inflammation, leading to a higher tumor burden in the CAC mouse model. In contrast, CerS4 deficiency in epithelial cells resulted in smaller colon tumors and seemed to be beneficial. The higher tumor incidence in CerS4 LCK/Cre mice and the toxic effect of AOM/DSS in CerS4 KO mice exhibited the importance of CerS4 in other tissues and revealed the complexity of general targeting CerS4.
Today, the term buchu refers to the two species in commerce, Agathosma betulina (P.J.Bergius) Pillans and Agathosma crenulata (L.) Pillans (Rutaceae). Its traditional use in urinary tract infections and related ailments made it a popular remedy, specifically in the US, in 19th century, but with the advent of antibiotics it became largely obsolete. Recent focus is on technological use and on the essential oil for use in the perfume and food-flavouring industry. A review of the scarce pharmacological research revealed moderate antimicrobial activity for a leaf extract but not the essential oil of both species in the MIC assay. In the 5-lipoxygenase (5-LO) assay the essential oil of both species revealed IC50 values of 50.37 ± 1.87 μg/ml and 59.15 ± 7.44 μg/ml, respectively. In another study 98% inhibitory activity was determined for 250 μg/ml of an ethanolic extract of A. betulina on cyclooxygenase (COX)-1 and a 25% inhibitory activity on COX-2. Analgesic activity of an ethanolic extract of A. betulina was shown in mice. Moderate antioxidant activity was determined for methanol:dichlormethane extracts of A. betulina and A. crenulata and an aqueous extract of A. betulina showed a Trolox equivalent antioxidant capacity (TEAC) of 11.8 µM Trolox. Recent in vitro studies with a commercial aqueous extract of buchu revealed increased uptake of glucose added to 3T3-L1 cell line, significant inhibition of the respiratory burst of neutrophils and monocytes, reduction in the expression of adhesion molecules and inhibition of the release of IL-6 and TNF-α. In diabetic rats the ingestion of aqueous buchu extract completely normalized the glucose level and in rats receiving a high fat diet the consumption of aqueous buchu extract resulted in less weight gain and less intraperitoneal fat gain as well as reduction of elevated blood pressure to normal associated with cardioprotective effects. Limitations in the hitherto conducted research lie in the undisclosed composition of the buchu extracts used and the difficulty in extrapolating data from animal studies to humans. Health claims for buchu products need to be substantiated by randomized, double-blind and placebo-controlled studies. Only then can they be promoted for their true therapeutic potential.
Necroptosis is an immunogenic form of programmed cell death characterized by plasma membrane accumulation of activated mixed lineage kinase domain-like (MLKL) that eventually leads to membrane disruption and release of danger-associated molecular patterns (DAMPs). Necroptotic cell death is tightly controlled by checkpoints, including compartmentalization as well as post-translational modifications (PTMs), like phosphorylation and ubiquitination of receptor-interacting protein kinase (RIPK) 1, RIPK3 and MLKL. Removal of plasma membrane-located activated MLKL via endocytosis or exocytosis can counteract necroptosis, but up till now, the exact mechanisms by which necroptosis is regulated downstream of MLKL activation and oligomerization are not fully understood.
Ubiquitination is a key post-translational modification that regulates various cellular processes including cell survival and cell death signaling via ubiquitination of RIPK1, RIPK3 and MLKL. M1-linked (linear) poly-ubiquitination is mediated exclusively by the linear ubiquitin chain assembly complex (LUBAC) which critically regulates cell fate and immune signaling via death receptors such as TNF receptor 1 (TNFR1).
In this study, we demonstrate that M1 poly-Ubiquitin (poly-Ub) increases during necroptosis which can be blocked by inhibition of LUBAC activity with the small-molecule HOIL-1-interacting protein (HOIP) inhibitor HOIPIN-8 or by loss of LUBAC catalytic subunit HOIP. Intriguingly, HOIPIN-8, as well as the HOIP inhibitor gliotoxin, and HOIP knockdown effectively prevent TNFα/smac mimetic/zVAD.fmk-induced necroptotic cell death in cells of human origin, without affecting necroptotic RIPK1 and RIPK3 phosphorylation, necrosome formation and oligomerization of phosphorylated MLKL. We demonstrate that HOIPIN-8 treatment inhibits MLKL translocation to intracellular membranes and accumulation in plasma membrane hotspots as well as MLKL exocytosis. We further confirm that HOIPIN-8 treatment suppresses necroptotic cell death in primary human pancreatic organoids (hPOs). Using time-lapse imaging and live/dead staining, we demonstrate loss of organoid structure and hPO cell death induced by smac mimetics and caspase inhibitors, thus providing a novel platform to investigate necroptosis in near physiological settings. Inhibition of LUBAC activity with HOIPIN-8 prevents hPO collapse and extends cell viability. Of note, loss of the M1 Ub-targeting deubiquitinating enzymes (DUBs) OTU DUB with linear linkage specificity (OTULIN) and cylindromatosis (CYLD) in human cell lines does not affect necroptosis induction and HOIPIN-8-mediated rescue of necroptosis. Intriguingly, inhibition of LUBAC activity with HOIPIN-8 does not block necroptotic cell death in murine cell lines.
Using massive analyses of cDNA ends (MACE)-seq-based global transcriptome analysis we confirm that necroptosis induces a pro-inflammatory cytokine profile which is dependent on LUBAC function and necroptotic signaling. Loss of LUBAC activity prevents the MLKL-dependent production and release of pro-inflammatory cytokines and chemokines.
Finally, we identify Flotillin-1 and -2 (FLOT1/2) as putative targets of necroptosis-induced M1 poly-Ub. Ubiquitin-binding in ABIN and NEMO (UBAN)-based pulldowns of M1 poly-ubiquitinated proteins revealed enrichment of FLOTs after necroptosis induction which is dependent on LUBAC activity and can be blocked with necroptosis inhibitors Nec-1s, GSK’872 and NSA, targeting RIPK1, RIPK3 and MLKL, respectively. Of note, loss of FLOT1/2 potentiates necroptosis suppression induced by LUBAC inhibition with HOIPIN-8.
Together, these findings identify LUBAC-mediated M1 poly-Ub as an important mediator of necroptosis and identify FLOTs as novel putative targets of LUBAC-mediated M1 poly-Ub during necroptosis. In addition, by modeling necroptosis in primary human organoids, we further expand the spectrum of experimental models to study necroptosis in human cellular settings.