TY - JOUR A1 - Kaltdorf, Martin A1 - Breitenbach, Tim A1 - Karl, Stefan A1 - Fuchs, Maximilian A1 - Kessie, David Komla A1 - Psota, Eric A1 - Prelog, Martina A1 - Sarukhanyan, Edita A1 - Ebert, Regina A1 - Jakob, Franz A1 - Dandekar, Gudrun A1 - Naseem, Muhammad A1 - Liang, Chunguang A1 - Dandekar, Thomas T1 - Software JimenaE allows efficient dynamic simulations of Boolean networks, centrality and system state analysis JF - Scientific Reports N2 - The signal modelling framework JimenaE simulates dynamically Boolean networks. In contrast to SQUAD, there is systematic and not just heuristic calculation of all system states. These specific features are not present in CellNetAnalyzer and BoolNet. JimenaE is an expert extension of Jimena, with new optimized code, network conversion into different formats, rapid convergence both for system state calculation as well as for all three network centralities. It allows higher accuracy in determining network states and allows to dissect networks and identification of network control type and amount for each protein with high accuracy. Biological examples demonstrate this: (i) High plasticity of mesenchymal stromal cells for differentiation into chondrocytes, osteoblasts and adipocytes and differentiation-specific network control focusses on wnt-, TGF-beta and PPAR-gamma signaling. JimenaE allows to study individual proteins, removal or adding interactions (or autocrine loops) and accurately quantifies effects as well as number of system states. (ii) Dynamical modelling of cell–cell interactions of plant Arapidopsis thaliana against Pseudomonas syringae DC3000: We analyze for the first time the pathogen perspective and its interaction with the host. We next provide a detailed analysis on how plant hormonal regulation stimulates specific proteins and who and which protein has which type and amount of network control including a detailed heatmap of the A.thaliana response distinguishing between two states of the immune response. (iii) In an immune response network of dendritic cells confronted with Aspergillus fumigatus, JimenaE calculates now accurately the specific values for centralities and protein-specific network control including chemokine and pattern recognition receptors. KW - cellular signalling networks KW - computer modelling Y1 - 2023 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-313303 VL - 13 ER - TY - THES A1 - Kessie, David Komla T1 - Characterisation of Bordetella pertussis virulence mechanisms using engineered human airway tissue models T1 - Charakterisierung der Virulenzmechanismen von Bordetella pertussis mit humanen Gewebemodellen der Atemwege N2 - Pertussis is a highly contagious acute respiratory disease of humans which is mainly caused by the gram-negative obligate human pathogen Bordetella pertussis. Despite the availability and extensive use of vaccines, the disease persists and has shown periodic re-emergence resulting in an estimated 640,000 deaths worldwide in 2014. The pathogen expresses various virulence factors that enable it to modulate the host immune response, allowing it to colonise the ciliated airway mucosa. Many of these factors also directly interfere with host signal transduction systems, causing damage to the ciliated airway mucosa and increase mucous production. Of the many virulence factors of B. pertussis, only the tracheal cytotoxin (TCT) is able to recapitulate the pathophysiology of ciliated cell extrusion and blebbing in animal models and in human nasal biopsies. Furthermore, due to the lack of appropriate human models and donor materials, the role of bacterial virulence factors has been extrapolated from studies using animal models infected with either B. pertussis or with the closely related species B. bronchiseptica which naturally causes respiratory infections in these animals and produces many similar virulence factors. Thus, in the present work, in vitro airway mucosa models developed by co-culturing human airway epithelia cells and fibroblasts from the conduction zone of the respiratory tract on a decellularized porcine small intestine submucosa scaffold (SISser®) were used, since these models have a high correlation to native human conducting zone respiratory epithelia. The major aim was to use the engineered airway mucosa models to elucidate the contribution of B. pertussis TCT in the pathophysiology of the disease as well as the virulence mechanism of B. pertussis in general. TCT and lipopolysaccharide (LPS) either alone or in combination were observed to induce epithelial cell blebbing and necrosis in the in vitro airway mucosa model. Additionally, the toxins induced viscous hyper-mucous secretion and significantly disrupted barrier properties of the in vitro airway mucosa models. This work also sought to assess the invasion and intracellular survival of B. pertussis in the polarised epithelia, which has been critically discussed for many years in the literature. Infection of the models with B. pertussis showed that the bacteria can adhere to the models and invade the epithelial cells as early as 6 hours post inoculation. Invasion and intracellular survival assays indicated the bacteria could invade and persist intracellularly in the epithelial cells for up to 3 days. Due to the novelty of the in vitro airway mucosa models, this work also intended to establish a method for isolating individual cells for scRNA-seq after infection with B. pertussis. Cold dissociation with Bacillus licheniformis subtilisin A was found to be capable of dissociating the cells without inducing a strong fragmentation, a problem which occurs when collagenase and trypsin/EDTA are used. In summary, the present work showed that TCT acts possibly in conjunction with LPS to disrupt the human airway mucosa much like previously shown in the hamster tracheal ring models and thus appears to play an important role during the natural B. pertussis infection. Furthermore, we established a method for infecting and isolating infected cells from the airway mucosa models in order to further investigate the effect of B. pertussis infection on the different cell populations in the airway by single cell analytics in the future. N2 - Pertussis ist eine hoch ansteckende akute Atemwegserkrankung des Menschen, die durch das gramnegative obligat humanpathogene Bakterium Bordetella pertussis verursacht wird. Obwohl seit langer Zeit effektive Impfstoffe verfügbar sind und weltweit eingesetzt werden, stellt die Krankheit nach wie vor ein großes Problem dar und tritt seit einiger Zeit auch in Ländern mit guten Impfraten wieder vermehrt auf. Allein in den letzten 10 Jahren wurden weltweit etwa 24 Millionen Neuinfektionen mit 640,000 Todesfällen pro Jahr gezählt. Die Bakterien exprimieren verschiedene Virulenzfaktoren, die es ihnen ermöglichen, die Immunantwort des Wirts zu modulieren, wodurch sie die Schleimhaut der oberen Atemwege besiedeln können. Viele dieser Faktoren stören auch direkt die Signaltransduktionssysteme des Zellen der oberen Atemwege, was zu einer Schädigung des Flimmerepithels der Atemwege und zu einer starken Erhöhung der Schleimproduktion führt. Von den vielen bekannten Virulenzfaktoren von B. pertussis kann soweit bekannt nur das Tracheale Cytotoxin (TCT) die typische Pathophysiologie des Flimmerepithels verursachen, die durch massive Gewebszerstörung gekennzeichnet ist und z.B. das Herauslösen von Epithelzellen aus der Epithelschicht oder die Ausbildung von bläschenförmigen Epithelzellen beinhaltet. Aufgrund des Mangels an geeigneten menschlichen Modellsystemen bzw. an Spendermaterialien wurden die Virulenzeigenschaften des Erregers entweder mit Hilfe von einfachen Zellkultursystemen oder in Tiermodellen untersucht, die keine natürlichen Wirte für B. pertussis darstellen. Alternativ hierzu wurden auch Daten, die mit dem eng verwandten tierpathogenen Bakterium B. bronchiseptica, das viele aus B. pertussis bekannte Virulenzfaktoren produziert, in entsprechenden Tiermodellen erhoben wurden, genutzt, um auf die Virulenzeigenschaften von B. pertussis zu schließen. Die vorliegende Arbeit verwendet In-vitro-Atemwegsschleimhautmodelle, die durch Co-Kultivierung von menschlichen Atemwegsepithelzellen und Fibroblasten auf einem dezellularisierten Schweine-Dünndarm-Submukosa-Gerüst (SISser®) entwickelt wurden. Die in-vitro-Atemwegsschleimhautmodelle weisen eine hohe Korrelation mit nativen menschlichen Epithelien der oberen Atemwege auf. Mithilfe dieser neuartigen Atemwegsschleimhautmodelle sollte der Beitrag von B. pertussis TCT zur Pathophysiologie der Krankheit und die Bedeutung von TCT als relevanter Virulenzfaktor aufgeklärt werden. Es wurde beobachtet, dass TCT und das bakterielle Lipopolysaccharid (LPS) entweder alleine oder in Kombination die Bildung von Epithelzellbläschen und Nekrose in diesen in-vitro-Atemwegsschleimhautmodellen induzieren. Zusätzlich induzierten diese Toxine eine viskose Hyperschleimsekretion und störten die Barriereeigenschaften der in-vitro-Atemwegsschleimhautmodelle signifikant. Zudem wurde in dieser Arbeit versucht, die Invasion und das intrazelluläre Überleben von B. pertussis in den polarisierten Epithelien zu bewerten, das in der einschlägigen Fachliteratur kritisch diskutiert wird. Die Infektion der Modelle mit B. pertussis zeigte, dass die Bakterien bereits 6 Stunden nach der Inokulation an den Modellen adhärieren und in diese eindringen können. Invasions- und intrazelluläre Überlebenstests zeigten, dass die Bakterien bis zu 3 Tage intrazellulär in die Epithelzellen überleben können. Aufgrund der Neuheit der in dieser Arbeit entwickelten in-vitro-Atemwegsschleimhautmodelle sollte auch eine Methode zur Isolierung einzelner Zellen für scRNA-seq Analysen nach Infektion mit B. pertussis etabliert werden. Dabei wurde festgestellt, dass die Inkubation der Modelle mit Subtilisin A von Bacillus licheniformis in der Kälte eine sehr gute Methode darstellt, um die Zellen zu dissoziieren, ohne eine starke Fragmentierung zu induzieren, wie sie unter Verwendung von Kollagenase und Trypsin / EDTA auftritt. Zusammenfassend wird in der vorliegenden Arbeit gezeigt, dass TCT gemeinsam mit LPS eine extrem destruktive Wirkung auf die menschliche Atemwegsschleimhaut besitzt, die der früher gezeigten Wirkung in Tiermodellen stark ähnelt. TCT sollte deshalb tatsächlich als ein wichtiger Virulenzfaktor von B. pertussis eingeschätzt werden. Darüber hinaus wurden Methoden zur Infektion und Isolierung von infizierten Zellen aus den Atemwegsschleimhautmodellen entwickelt, um künftig die Auswirkung einer B. pertussis Infektion auf die verschiedenen Zellpopulationen in den Atemwegen durch Einzelzellanalytik noch besser erforschen zu können. KW - Tissue engineering KW - Pertussis KW - Airway epithelia KW - Bordetella KW - tracheal cytotoxin KW - 3D models Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-235717 ER - TY - JOUR A1 - Stelzner, Kathrin A1 - Boyny, Aziza A1 - Hertlein, Tobias A1 - Sroka, Aneta A1 - Moldovan, Adriana A1 - Paprotka, Kerstin A1 - Kessie, David A1 - Mehling, Helene A1 - Potempa, Jan A1 - Ohlsen, Knut A1 - Fraunholz, Martin J. A1 - Rudel, Thomas T1 - Intracellular Staphylococcus aureus employs the cysteine protease staphopain A to induce host cell death in epithelial cells JF - PLoS Pathogens N2 - Staphylococcus aureus is a major human pathogen, which can invade and survive in non-professional and professional phagocytes. Uptake by host cells is thought to contribute to pathogenicity and persistence of the bacterium. Upon internalization by epithelial cells, cytotoxic S. aureus strains can escape from the phagosome, replicate in the cytosol and induce host cell death. Here, we identified a staphylococcal cysteine protease to induce cell death after translocation of intracellular S. aureus into the host cell cytoplasm. We demonstrated that loss of staphopain A function leads to delayed onset of host cell death and prolonged intracellular replication of S. aureus in epithelial cells. Overexpression of staphopain A in a non-cytotoxic strain facilitated intracellular killing of the host cell even in the absence of detectable intracellular replication. Moreover, staphopain A contributed to efficient colonization of the lung in a mouse pneumonia model. In phagocytic cells, where intracellular S. aureus is exclusively localized in the phagosome, staphopain A did not contribute to cytotoxicity. Our study suggests that staphopain A is utilized by S. aureus to exit the epithelial host cell and thus contributes to tissue destruction and dissemination of infection. Author summary Staphylococcus aureus is an antibiotic-resistant pathogen that emerges in hospital and community settings and can cause a variety of diseases ranging from skin abscesses to lung inflammation and blood poisoning. The bacterium can asymptomatically colonize the upper respiratory tract and skin of humans and take advantage of opportune conditions, like immunodeficiency or breached barriers, to cause infection. Although S. aureus was not regarded as intracellular bacterium, it can be internalized by human cells and subsequently exit the host cells by induction of cell death, which is considered to cause tissue destruction and spread of infection. The bacterial virulence factors and underlying molecular mechanisms involved in the intracellular lifestyle of S. aureus remain largely unknown. We identified a bacterial cysteine protease to contribute to host cell death of epithelial cells mediated by intracellular S. aureus. Staphopain A induced killing of the host cell after translocation of the pathogen into the cell cytosol, while bacterial proliferation was not required. Further, the protease enhanced survival of the pathogen during lung infection. These findings reveal a novel, intracellular role for the bacterial protease staphopain A. KW - Staphylococcus aureus KW - Staphylococcal infection KW - host cells KW - HeLa cells KW - cytotoxicity KW - intracellular pathogens KW - apoptosis KW - epithelial cells Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-263908 VL - 17 IS - 9 ER - TY - JOUR A1 - Sivarajan, Rinu A1 - Kessie, David Komla A1 - Oberwinkler, Heike A1 - Pallmann, Niklas A1 - Walles, Thorsten A1 - Scherzad, Agmal A1 - Hackenberg, Stephan A1 - Steinke, Maria T1 - Susceptibility of Human Airway Tissue Models Derived From Different Anatomical Sites to Bordetella pertussis and Its Virulence Factor Adenylate Cyclase Toxin JF - Frontiers in Cellular and Infection Microbiology N2 - To study the interaction of human pathogens with their host target structures, human tissue models based on primary cells are considered suitable. Complex tissue models of the human airways have been used as infection models for various viral and bacterial pathogens. The Gram-negative bacterium Bordetella pertussis is of relevant clinical interest since whooping cough has developed into a resurgent infectious disease. In the present study, we created three-dimensional tissue models of the human ciliated nasal and tracheo-bronchial mucosa. We compared the innate immune response of these models towards the B. pertussis virulence factor adenylate cyclase toxin (CyaA) and its enzymatically inactive but fully pore-forming toxoid CyaA-AC\(^-\). Applying molecular biological, histological, and microbiological assays, we found that 1 µg/ml CyaA elevated the intracellular cAMP level but did not disturb the epithelial barrier integrity of nasal and tracheo-bronchial airway mucosa tissue models. Interestingly, CyaA significantly increased interleukin 6, interleukin 8, and human beta defensin 2 secretion in nasal tissue models, whereas tracheo-bronchial tissue models were not significantly affected compared to the controls. Subsequently, we investigated the interaction of B. pertussis with both differentiated primary nasal and tracheo-bronchial tissue models and demonstrated bacterial adherence and invasion without observing host cell type-specific significant differences. Even though the nasal and the tracheo-bronchial mucosa appear similar from a histological perspective, they are differentially susceptible to B. pertussis CyaA in vitro. Our finding that nasal tissue models showed an increased innate immune response towards the B. pertussis virulence factor CyaA compared to tracheo-bronchial tissue models may reflect the key role of the nasal airway mucosa as the first line of defense against airborne pathogens. KW - human nasal epithelial cells KW - human tracheo-bronchial epithelial cells KW - human airway mucosa tissue models KW - adenylate cyclase toxin KW - Bordetella pertussis Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-253302 SN - 2235-2988 VL - 11 ER - TY - JOUR A1 - Kessie, David K. A1 - Lodes, Nina A1 - Oberwinkler, Heike A1 - Goldman, William E. A1 - Walles, Thorsten A1 - Steinke, Maria A1 - Gross, Roy T1 - Activity of Tracheal Cytotoxin of Bordetella pertussis in a Human Tracheobronchial 3D Tissue Model JF - Frontiers in Cellular and Infection Microbiology N2 - Bordetella pertussis is a highly contagious pathogen which causes whooping cough in humans. A major pathophysiology of infection is the extrusion of ciliated cells and subsequent disruption of the respiratory mucosa. Tracheal cytotoxin (TCT) is the only virulence factor produced by B. pertussis that has been able to recapitulate this pathology in animal models. This pathophysiology is well characterized in a hamster tracheal model, but human data are lacking due to scarcity of donor material. We assessed the impact of TCT and lipopolysaccharide (LPS) on the functional integrity of the human airway mucosa by using in vitro airway mucosa models developed by co-culturing human tracheobronchial epithelial cells and human tracheobronchial fibroblasts on porcine small intestinal submucosa scaffold under airlift conditions. TCT and LPS either alone and in combination induced blebbing and necrosis of the ciliated epithelia. TCT and LPS induced loss of ciliated epithelial cells and hyper-mucus production which interfered with mucociliary clearance. In addition, the toxins had a disruptive effect on the tight junction organization, significantly reduced transepithelial electrical resistance and increased FITC-Dextran permeability after toxin incubation. In summary, the results indicate that TCT collaborates with LPS to induce the disruption of the human airway mucosa as reported for the hamster tracheal model. KW - tracheal cytotoxin KW - airway epithelia KW - tissue model KW - ciliostasis KW - tight junction KW - Bordetella pertussis Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-222736 SN - 2235-2988 VL - 10 ER -