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Zielsetzung: Diese Arbeit untersuchte die Beziehung zwischen intrazellulärem Eisengehalt (pgFe/Zelle) und der Fähigkeit der Histochemie und des MRT, in vitro mit Eisenoxidnanopartikel gelabelte Zellen zu detektieren. Methoden: Immortalisierte murine Peritonealmakrophagen wurden mit Very Small Iron Oxide Nanoparticles (VSOP) in aufsteigenden Konzentrationen (n=10) von 0 bis 200 µg/ml für 4 Stunden inkubiert. Die MRT-Messungen wurden an einem 7-Tesla Bruker Biospec durchgeführt. Für jedes Label-Protokoll wurden Objektträgerproben (n=6) mit den Zellen angefertigt und mit der PB-, DAB-PB- und AgAu-DAB-PB-Färbung gefärbt. Es wurde der prozentuale Anteil der sichtbar gefärbten Zellen ermittelt. Über ICP-MS bestimmten wir den intrazellulären Eisengehalt und TEM-Aufnahmen bestätigten den vesikulären Uptake von VSOP. Zusätzlich wurde der Einfluss der Zelldichte auf MR-Detektionsgrenzen an identisch gelabelten Zellen zwischen 2x10^5 und 8x10^6 Zellen/0,5ml zwischen nierigen (0,22 pgFe/Zelle) und hohen (3,81pgFe/Zelle) Eisenbeladungen untersucht. Ergebnisse: Der intrazelluläre Eisengehalt reichte von 0.12 bis 12.25 pgFe/Zelle. Die Histochemie zeigte einen höheren Prozentsatz an eisen-positiven Zellen mit steigendem Eisengehalt. Das Enhancement der Preußisch Blau Färbung(PB) mit Diaminobenzidin (DAB) und einer modifizierten AgAu-DAB Färbung führte zu einer höheren Sensitivität für intrazelluläres Eisen (>50% gefärbte Zellen bei 1,3 pgFe/Zelle versus 1,6 pgFe/Zelle) als die Preußisch Blau Färbung selbst (2,2 pgFe/Zelle). Jedoch zeigten beide Färbungen bei einem Eisengehalt unter 0,7 pgFe/Zelle weniger als 25% eisenpositive Zellen. Die T2 und T2* verkürzenden Effekte von VSOP zeigten eine positive Korrelation zur intrazellulären Eisenbeladung und zur Zelldichte. Selbst bei 0.26 pgFe/Zelle war eine sichtbare Änderung der Relaxationsraten sichtbar. Schlussfolgerung: Diese Arbeit zeigte, dass in MRT-Messungen selbst kleinste Mengen an intrazellulärem VSOP nachgewiesen werden können, welche in der Histochemie noch nicht nachgewiesen werden können. Es wurde ebenso gezeigt, dass positive Korrelationen zwischen der Zelldichte, dem intrazellulären Eisengehalt und der T2/T2*-Relaxationsraten bestehen.
Immunzellen mit hemmenden bzw. regulatorischen Eigenschaften erscheinen sehr attraktiv, um ungewollte Immunantworten, wie sie z.B. nach Transplan¬tationen auftreten, selektiv zu hemmen. In früheren Arbeiten konnten wir zeigen, dass sich mit GM-CSF und IL-4 immunregulatorische Dendritische Zellen (IL-4 DC) aus hämatopoetischen Vorläuferzellen des Knochenmarks der Lewis-Ratte generieren lassen. In der vorliegenden Arbeit wurden Makrophagen aus Knochenmarkvorläuferzellen mit M-CSF und IL-4 (IL-4 Makrophagen) generiert und mit den IL-4 DC hinsichtlich ihres Phänotyps und ihrer immunologischen Eigenschaften verglichen. M-CSF Makrophagen, die nur mit M-CSF generiert wurden, dienten hierbei als Kontrolle. Im Gegensatz zu reifen DC (mDC), die aus der Milz isoliert wurden, sind weder M-CSF Makrophagen noch IL-4 Makrophagen bzw. IL-4 DC in der Lage, naive T Lymphozyten in vitro zu aktivieren. Zudem wurde eine Zellzahl-abhängige Hemmung der mDC induzierten T Zell-Aktivierung beobachtet. So hemmten IL-4 Makrophagen die mDC-induzierte T-Zellproliferation nahezu vollständig (bis zu 96%), wenn sie in einem Zellverhältnis von 1:1 (IL-4 Makrophagen:mDC) als Kompetitorzellen eingesetzt wurden. Ähnliche Effekte waren auch für M-CSF Makrophagen und IL-4 DC zu beobachten. Zwar ist nicht geklärt, wie die Zellen diesen hemmenden Effekt vermitteln, doch lassen die Daten der vorliegenden Arbeit sowohl einen durch Oberflächenmoleküle als auch lösliche Mediatoren vermittelten Mechanismus für möglich erscheinen. Durchflusszytometrische Analysen, ergänzt durch Immunhistochemie und Real time PCR, zeigten für IL-4 Makrophagen und M-CSF Makrophagen einen Phänotyp, der gegenüber IL-4 DC, eine geringere Expression von CD80 und CD86 auf der Zelloberfläche aufwies. Die IL-4 DC wiesen ihrerseits eine geringe Expression von CD80 und CD86 in Vergleich zu mDC auf, wie in vorangegangenen Arbeiten gezeigt wurde. Alle drei Subpopulationen waren positiv für MHC I und CD40, während IL-4 Makrophagen und IL-4 DC zusätzlich positiv für MHC II waren. T Lymphozyten in Kokultur mit IL-4 Makrophagen bzw. mit M-CSF Makrophagen oder IL-4 DC wiesen nur eine geringe Proliferation auf, wenn sie anschließend mit mDC restimuliert wurden. Diese Daten deuten darauf hin, dass IL-4 Makrophagen, M-CSF Makrophagen und IL-4 DC naive T-Lymphozyten dauerhaft in ihrer Restimulierung hemmen. Dieser anergische Zustand ist möglicherweise auf die unzureichende Kostimulation zurückzuführen. Zudem wurde bei den mit IL-4 Makrophagen, M-CSF Makrophagen und IL-4 DC kokultivierten T Lymphozyten eine geringfügig erhöhte Rate an apoptotischen Zellen gemessen als bei T Lymphozyten, die zuvor alleine oder mit mDC kultiviert wurden. Auch von IL-4 Makrophagen, M-CSF Makrophagen und IL-4 DC sezernierte lösliche Faktoren können eine Rolle bei der Hemmung der T-Zellaktivierung spielen. Überstände einer 24-stündigen Kultur mit einer Million IL-4 Makrophagen, M-CSF Makrophagen und IL-4 DC, hemmten die mDC-induzierte T-Zellaktivierung mit einer Suppressionsrate von 81-85%. Mit einer nahezu vollständigen Hemmung der T-Zellaktivierung war der Effekt von Überständen aus 48-stündigen Kulturen sogar noch stärker. Wie anhand von ELISA und real time PCR gezeigt wurde, exprimierten IL-4 Makrophagen, M-CSF Makrophagen und IL-4 DC das immuninhibitorische Zytokin TGF-Beta, das für die beobachtete Hemmung der T-Zellproliferation verantwortlich sein könnte. Die Ergebnisse zeigen somit, dass die aus Knochenmarkvorläuferzellen generierten IL-4 Makrophagen und M-CSF Makrophagen die Aktivierung naiver T-Lymphozyten hemmen. Diese Eigenschaft teilen sie sich mit IL-4 DC trotz deutlicher Unterschiede bei den Phänotypen dieser Zellen. Die Ergebnisse dieser Arbeit lassen den Schluss zu, dass die aus hämatopoetischen Stammzellen des Knochenmarks hergestellten Dendritische Zellen und Makrophagen die Aktivierung naiver T-Lymphozyten effektiv hemmen. Der Mechanismus, wie dieser hemmende Effekt vermittelt wird, ist zurzeit noch unbekannt und sollte in weiteren Arbeiten analysiert werden. Von grundlegender Bedeutung wäre der erfolgreiche Nachweis, dass diese Zellen ungewollte Immunantworten antigen¬spezifisch hemmen.
Rhodococcus equi is a Gram-positive intracellular pathogen which can cause severe bronchopneumonia in foals. In recent years, the role of this bacterium as human pathogen has been noted, as R.equi infections in humans have increase in frequency. This increase is associated with the rise in immunosupressed individuals, specially AIDS patients, where infection leads to symptoms and pathology similar to those seen in foals with a high mortality rate. Due to its capability to survive and multiply in murine and equine macrophages, R.equi has been classified as a facultative intracellular bacterium. R.equi is found frequently in macrophages in alveolar infiltrate from infected animals. The pathogenicity of R.equi depends on its ability to exist and multiply inside macrophages and has been associated with the presence of virulence plasmids. It has been observed that, inside foal alveolar macrophages, R.equi-containing vacuoles (RCVs) do not mature into phagolysosomes. However, most of the intracellular events during R.equi infection have not been investigated in detail. The aim of this study was to elucidate the intracellular compartmentation of R.equi and the mechanism by which the bacteria avoid destruction in host macrophages. The importance of the virulence-associated plasmids of R.equi for the establishment of RCVs was also evaluated. Furthermore, the intracellular fate of viable and non-viable R.equi was compared in order to study whether viability of R.equi influeciantes the establishment of RCVs. In this study, the RCV was characterized by using a variety of endocytic markers to follow the path of the bacteria trhough murine macropages. Transmission electron microscopy-base analysis showed that R.equi was found equally frequently in phagosomes with loosely or thightly apposed membranes, and RCV often contains numerous membranous vesicles. Laser scanning microscopy of infected macrophages showed that the majority of phagosomes containing R.equi acquired transiently the early endosomal markers Rab5, Ptlns3P, and EEA-1, suggesting initially undisturbed phagosome maturation. Although the RCV acquired some late endosomal markers, such as Rab7, LAMP-1, and Lamp-2, they did not acquired vATPase, did not interact with pre-labeled lysosomes, and failed to acidify. These data clearly suggest that the RCV is a compartment which has left vacuoles that resemble multivesicular body compartments (MVB), which are transport intermediates between early and late endosomes and display internal vesicles very similar to the ones observed within RCVs. Analyisis of several R.equi strains containing either VapA- or VapB-expressing plasmids or neither demonstrated that the possession of the virulence-associated plasmids does not affect phagosome trafficking over a two hour period of infection. The finding that non-viable R.equi was still able to inhibit phagosome maturation (although not to the same extent as viable R.equi did) suggests that heat-insensitive factors, such as cell periphery lipids, may play a major role in inhibition of phagosome maturation, although heat-sensitive factors may also be involved.
Charcot-Marie-Tooth 1B (CMT1B) is a progressive inherited demyelinating disease of human peripheral nervous system leading to sensory and/or motor function disability and is caused by mutations in the P0 gene. Mice heterozygously deficient for P0 (P0+/-) are an adequate model of this human disorder showing myelin degeneration, formation of onion bulbs, remyelination and a reduced motor conduction velocity of around 30m/s similar to patients. Previously, it had been shown that T-lymphocytes and macrophages play a crucial role during pathogenesis in peripheral nerves of P0+/- mice. Both, T-lymphocytes and macrophages increase in number in the endoneurium and deletion of T-lymphocytes or deletion of a macrophage-directed cytokine ameliorates the disease. In this study the monocyte chemoattractant protein-1 (MCP-1) was identified as an early regulated cytokine before onset of disease is visible at the age of six months. MCP-1 mRNA and protein expression could be detected in femoral quadriceps and sciatic nerves of P0+/- mice already at the age of one month but not in cutaneous saphenous nerves which are never affected by the disease. MCP-1 was shown to be expressed by Schwann cells and to mediate the immigration of immune cells into peripheral nerves. Deletion of MCP-1 in P0+/- mice accomplished by crossbreeding P0 and MCP-1 deficient mice revealed a substantial reduction of immune cells in peripheral nerves of P0+/-/MCP-1+/- and P0+/-/MCP-1-/- mice at the age of six months. In twelve months old mice reduction of immune cells in peripheral nerves is accompanied by amelioration of demyelinating disease in P0+/-/MCP-1+/- and aggravation of demyelinating disease in lumbar ventral roots of P0+/ /MCP-1-/- mice in comparison to P0+/ /MCP 1+/+ mice. Furthermore, activation of the MEK1/2-ERK1/2 signalling cascade could be demonstrated to take place in Schwann cells of affected peripheral nerves of P0+/- mice overlapping temporarily and spatially with MCP-1 expression. An animal experiment using a MEK1/2-inhibitor in vivo, CI-1040, revealed that upon reduction of ERK1/2 phosphorylation MCP-1 mRNA expression is diminished suggesting that the activation of the MEK1/2-ERK1/2 signalling cascade is necessary for MCP-1 expression. Additionally, peripheral nerves of P0+/- mice showing reduced ERK1/2 phosphorylation and MCP-1 mRNA expression also show reduced numbers of macrophages in the endoneurium. This study shows a molecular link between a Schwann cell based mutation and immune cell function. Inhibition of the identified signalling cascade might be a putative target for therapeutic approaches.
In neoplastic diseases the tumor stroma and especially tumor-associated macrophages (TAMs) play an important role in tumor growth and progression. TAMs exhibit an intensive cross-talk with tumor cells resulting in the promotion of angiogenesis and the inhibition of local protective immune responses in certain tumor entities. Therefore, TAMs are a potential target for tumor therapy. Here it was shown that intravenously applied intracellular bacteria like Salmonella and Shigella primarily target TAMs. To exploit this feature a growth attenuated Shigella strain with the capacity to induce apoptosis in macrophages was designed. Shigella are invasive bacteria that penetrate the colonic tissue and initiate an acute inflammation. In macrophages, Shigella rapidly induces caspase-1 processing and apoptosis via the virulence factor IpaB. By genomic deletion of the aroA-locus a metabolically attenuated strain defective in intracellular growth but with retained capacity of infection, cell-to-cell spread, caspase-1 processing and apoptosis induction in macrophages was designed. It was shown that this strain primarily targets TAMs in 4T1 cell induced and transgenic MMTV-HER2/new breast cancer models. Shigella were almost exclusively found intracellularly, whereas growth attenuated Salmonella were also found extracellularly at late time points. The metabollically attenuated Shigella strain with retained virulence, but not avirulent Shigella strains, was able to activate caspase-1 and induce apoptosis in TAMs at all time points (4 h, 6 h and 7 d p.i.) in both breast cancer models. This unrestricted apoptosis induction translated into a substantial, long-lasting and highly significant reduction of TAMs number (up to 70 %) in both models. In contrast, Salmonella could only induce apoptosis in TAMs at early time points (6 h p.i.) and failed to reduce TAMs in both models. In the 4T1 model, the effect on tumor size was monitored and treatment of the mice with the attenuated Shigella strain resulted in a complete block of tumor growth. Finally, Shigella primarily infected the macrophage fraction, activated caspase-1 and induced apoptosis in cells derived from a human ovarian carcinoma ex vivo. Taken together, this data suggests that growth attenuated intracellular bacteria capable of inducing apoptosis in TAMs are a promising therapeutic option for certain cancer diseases where TAMs have a proven role for tumor growth or progression.
Connexin32- defiziente Mäuse stellen ein Mausmodell für eine Form der hereditären peripheren Neuropahtie dar. Es konnte gezeigt werden, dass Makrophagen, möglicherweise aktiviert durch MCP-1, die Demyelinisierung in Connexin32-defizienten Mäusen vermitteln. Diese Arbeit untersucht mögliche Signaltransduktionswege, die in den peripheren Nerven Connexin32- defizienter Mäuse aktiviert sein könnten und damit in Zusammenhang mit der Genexpression von MCP-1 und/oder Makrophagen-Aktivierung stehen könnten.
Unter dem Einfluss von M-CSF und GM-CSF entwickeln sich CD14-positive periphere humane Blutmonozyten zu CD68-positiven M-CSF- bzw. GM-CSF-Makrophagen. M-CSF-Makrophagen lassen sich mit INFg und LPS zu klassisch aktivierten M1-Makrophagen, oder mit IL-4 und IL-10 zu alternativ aktivierten M2-Makrophagen differenzieren. Durch GM-CSF werden aus Monozyten GM-CSF-Makrophagen induziert. Im Gegensatz zu M1-Makrophagen sind GM1-Makrophagen bisher noch wenig untersucht. Mit INFg und LPS werden GM-CSF-Makrophagen zu GM1-Makrophagen aktivert. In der vorliegenden Arbeit wurde überprüft, wie groß die Übereinstimmung zwischen M-CSF- und M2-Makrophagen sowie zwischen GM-CSF- und M1-Makrophagen / GM1-Makrophagen ist. Im Gegensatz zu M-CSF- und GM-CSF stellt Laktat aber keinen Differenzierungsfaktor für Monozyten dar. Jedoch beeinflusst Laktat den Phänotyp von M2-Makrophagen und hemmt die Ausschüttung von IL-12 und NO durch M1- und GM1-Makrophagen.
Traditionally, ischemic stroke has been regarded as the mere consequence of cessation of cerebral blood flow, e.g. due to the thromboembolic occlusion of a major brain supplying vessel. However, the simple restoration of blood flow via thrombolysis and/or mechanical recanalization alone often does not guarantee a good functional outcome. It appears that secondary detrimental processes are triggered by hypoxia and reoxygenation, which are referred to as ischemia/reperfusion (I/R) injury. During recent years it became evident that, beside thrombosis inflammation and edema formation are key players in the pathophysiology of cerebral ischemia. The contact-kinin system represents an interface between thrombotic, inflammatory and edematous circuits. It connects the intrinsic coagulation pathway with the plasma kallikrein-kinin system (KKS) via coagulation factor FXII.
The serine protease inhibitor C1-inhibitor (C1-INH) has a wide spectrum of inhibitory activities and counteracts activation of the contact-kinin system at multiple levels. The first part of the thesis aimed to multimodally interfere with infarct development by C1-INH and to analyze modes of actions of human plasma derived C1-INH Berinert® P in a murine model of focal cerebral ischemia. It was shown that C57BL/6 mice following early application of 15.0 units (U) C1-INH, but not 7.5 U developed reduced brain infarctions by ~60% and less neurological deficits in the model of transient occlusion of the middle cerebral artery (tMCAO). This protective effect was preserved at more advanced stages of infarction (day 7), without increasing the risk of intracerebral bleeding or affecting normal hemostasis. Less neurological deficits could also be observed with delayed C1-INH treatment, whereas no improvement was achieved in the model of permanent MCAO (pMCAO). Blood-brain-barrier (BBB) damage, inflammation and thrombosis were significantly improved following 15.0 U C1-INH application early after onset of ischemia. Based on its strong antiedematous, antiinflammatory and antithrombotic properties C1-INH constitutes a multifaceted therapeutic compound that protects from ischemic neurodegeneration in ‘clinically meaningful’ settings.
The second part of the thesis addresses the still elusive functional role of macrophages in the early phase of stroke, especially the role of the macrophage-specific adhesion molecule sialoadhesin (Sn). For the first time, sialoadhesin null (Sn-/-) mice, homozygous deficient for Sn on macrophages were subjected to tMCAO to assess the clinical outcome. Neurological and motor function was significantly improved in Sn-/- mice on day 1 after ischemic stroke compared with wildtype (Sn+/+) animals. These clinical improvements were clearly detectable even on day 3 following tMCAO. Infarctions on day 1 were roughly the same size as in Sn+/+ mice and did not grow until day 3. No intracerebral bleeding could be detected at any time point of data acquisition. Twenty four hours after ischemia a strong induction of Sn was detectable in Sn+/+ mice, which was previously observed only on perivascular macrophages in the normal brain. Deletion of Sn on macrophages resulted in less disturbance of the BBB and a reduced number of CD11b+ (specific marker for macrophages/microglia) cells, which, however, was not associated with altered expression levels of inflammatory cytokines. To further analyze the function of macrophages following stroke this thesis took advantage of LysM-Cre+/-/IKK2-/- mice bearing a nuclear factor (NF)-ϰB activation defect in the myeloid lineage, including macrophages. Consequently, macrophages were not able to synthesize inflammatory cytokines under the control of NF-ϰB. Surprisingly, infarct sizes and neurological deficits upon tMCAO were roughly the same in conditional knockout mice and respective wildtype littermates. These findings provide evidence that macrophages do not contribute to tissue damage and neurological deficits, at least, not by release of inflammatory cytokines in the early phase of cerebral ischemia. In contrast, Sn which is initially expressed on perivascular macrophages and upregulated on macrophages/microglia within the parenchyma following stroke, influenced functional outcome.
Charcot-Marie-Tooth disease (CMT) is a cohort of human hereditary disorders of the peripheral nervous system (PNS) which exhibit symptoms like sensory dysfunction, muscle weakness and gait disturbances. Different mutations are described as causation for this neuropathy, such as a duplication of chromosome 17 comprising the gene for the peripheral myelin protein-22 (PMP22). Based on different animal models former studies identified immune cells, i.e. macrophages and T-lymphocytes, as crucial mediators of pathology in these neuropathies. In this study, PMP22-overexpressing mice (PMP22tg, C61), serving as a model for a specific type of CMT – CMT1A – were crossbred with immune-deficient mutant mice to examine the impact of the immune system on nerve pathology. Crossbreeding of PMP22tg mice with recombination activating gene-1 (RAG-1) deficient mice, lacking mature T- and B-lymphocytes, caused no striking alterations of pathogenesis in peripheral nerves of mutant mice. In contrast, crossbreeding of PMP22tg myelin mutants with mice deficient in the chemokine monocyte chemoattractant protein-1 (MCP-1, CCL2) caused an amelioration of the demyelinating phenotype of peripheral nerves when MCP-1 was either reduced or completely absent. Furthermore, functional investigations, i.e. neurographic recordings and examinations of the grip strength of the extremities, revealed an amelioration in PMP22tg/MCP-1-/- mice in regard to a symptomatic improvement in the compound action muscle potential (CMAP) and stronger grip strength of the hindlimbs. Interestingly, peripheral nerves of PMP22tg mice showed an irregular distribution of potassium channels in presence of MCP-1, whereas the absence of MCP-1 in the myelin mutants rescued the ion channel distribution and resulted in a more wild type-like phenotype. Having shown the impact of MCP-1 as an important mediator of nerve pathology in PMP22/MCP-1 double mutants, the regulation of this chemokine became an important target for potential treatment strategies. We found that the signaling cascade MEK1/2/ERK1/2 was more strongly activated in peripheral nerves of PMP22tg mice compared to nerves of wild type mice. This activation corresponded to an increase in MCP-1 mRNA expression in peripheral nerves at the same age. Furthermore, a MEK1/2-inhibitor was used in vivo to confirm the regulation of MCP-1 by the MEK1/2/ERK1/2 pathway. After a treatment period of three weeks, a clear reduction of ERK1/2-phosphorylation as well as a reduction of MCP-1 mRNA expression was observed, accompanied by a decline in macrophage number in peripheral nerves of PMP22tg mice. These observations suggest that the expression of MCP-1 is crucial for the neuropathological progression in a mouse model for CMT1A. Therefore, this chemokine could provide a basis for a putative treatment strategy of inherited neuropathies.