TY  - THES
A1  - Lasar, Andrea
T1  - Funktion von NF-kappa B für die Differenzierung lymphoider Zellen und die inflammatorische Aktivierung von Endothelzellen
T1  - Function of NF-kappa B for the differentiation of lymphoid cells and the inflammatory activation of endothelial cells
N2  - Die Aktivität des Transkriptionsfaktors NF-kappa B wird hauptsächlich durch inhibitorische I kappa B-Proteine kontrolliert,die durch die I kappa B-Kinasen 1 und 2 phosphoryliert und anschließend degradiert werden.Dadurch werden ver-schiedene zelluläre Prozesse wie Differenzierung und Aktivierung beeinflusst. Um die Rolle von NF-kappa B in der Differenzierung lymphoider Zellen zu untersuchen,wurden nichtdegradierbare Mutanten der I kappa B-Proteine in trans-genen Mäusen mit Hilfe des Tet-off-Systems exprimiert.Dieses erlaubt die kon-ditionale,gewebespezifische Expression der Mutanten.Im Thymus von tTA/tetI kappa B alpha-transgenen Mäusen konnte eine doxyzyklinabhängige Reduktion der CD8+-Thymozyten beobachtet werden.Eine Einschränkung der Analyse späterer Ent-wicklungsstadien war die zeitlich begrenzte Expression des Transgens,die nur in frühen Entwicklungsstadien stattfand.Die B-Zellentwicklung wurde anhand eines in vitro Differenzierungssystems nachvollzogen,das die Differenzierung von prä-B-Zellen zu unreifen bzw.reifen B-Zellen erlaubt.Dabei zeigte sich,dass ein transdominantes I kappa B alpha beide Differenzierungsschritte nahezu vollstän-dig hemmt,aber nur,wenn das endogene I kappa B alpha nicht vorhanden ist. Die Beteiligung von NF-kappa B an der inflammatorischen ktivierung von Endothel-zellen wurde mit Hilfe von retroviralen Infektionen untersucht.Dabei wurden neben mutanten I kappa B-Proteinen auch kinase-inaktive oder konstitutiv-aktive Mutanten der I kappa B-Kinasen verwendet.Die transdominanten I kappa B-Proteine sowie die kinase-inaktive IKK2 waren in der Lage,die TNF-alpha-induzierte Ex-pression aller untersuchten Chemokine und Adhäsionsmoleküle komplett zu hem-men.Dagegen wurde durch die kinase-inaktive IKK1 nur ein Teil der untersuchten Moleküle in ihrer Expression beeinflusst.Interessanterweise war eine konstitu-tiv-aktive IKK2 schon in der Abwesenheit von TNF-alpha in der Lage,die Expres-sion der untersuchten Proteine zu aktivieren.Die durch die Mutanten veränderte Expression der Adhäsionsmoleküle und Chemokine hatte auch einen Einfluss auf die in vitro Adhäsion und Transmigration von Monozyten.
N2  - The activity of the transcription factor NF-kappa B is mainly controlled by the inhibitory I kappa B proteins which are phosphorylated by the I kappa B kinases 1 and 2.This phosphorylation leads to the degradation of the I kappa B proteins thereby releasing NF-kappa B to the nucleus.The active NF-kappa B influences se-veral cellular processes like differentiation and activation. To investigate the role of NF-kappa B in the differentiation of lymphoid cells,nondegradable mutants of the I kappa B proteins were expressed in transge-nic mice based on the tet-off system.This allows the conditional tissue-speci-fic expression of the mutants.In the thymus of tTA/tetI kappa B alpha transge-nic mice,a doxycyclin-dependent reduction of the CD8+ thymocytes could be obser-ved.One restriction for the analysis of later stages of the development was the expression pattern of the transgene which was restricted to early developmental stages.The development of the transgenic B cells was investigated with an in vitro differentiation system which allows the differen-tiation to immature or mature B cells,respectively.The transdominant I kappa B alpha inhibits both steps of the differentiation almost completely,but only if the endogenous I kappa B alpha is absent. The involvement of NF-kappa B in the inflammatory activation of endothelial cells was studied by retroviral infections.In addition to the mutant I kappa B proteins,kinase-inactive or constitutively active versions of the I kappa B ki-nases were used.The transdominant I kappa B mutants as well as the kinase-inac-tive IKK2 were able to inhibit the TNF-alpha induced expression of all inve-stigated chemokines and adhesion molecules completely.In contrast,the kinase-inactive IKK1 influenced the expression of only a subset of the investigated genes.Interestingly,the constitutively active IKK2 could activate the expression of the investigated proteins already in the absence of TNF-alpha.The altered expression of adhesion molecules and chemokines also in-fluenced the in vitro adhesion and transmigration of monocytes.
KW  - NF-kappa B
KW  - I kappa B
KW  - B-Zelldifferenzierung
KW  - Tet-off-System
KW  - Entzündung
KW  - NF-kappa B
KW  - I kappa B
KW  - B cell differentiation
KW  - Tet-off system
KW  - inflammation
Y1  - 2002
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-5058
ER  - 
TY  - THES
A1  - Fellenberg, Friederike
T1  - Charakterisierung von Tumorantigenen des kutanen T-Zell Lymphoms: Serologische Immunantwort und Expressionsanalyse
T1  - characterisation of tumor antigens of the cutaneous t-cell lymphoma: serological immune response and expression analysis
N2  - Immuntherapien auf der Basis gut charakterisierter, tumorspezifischer Antigene stellen ein vielversprechendes Konzept der Tumortherapie dar. Ein potentielles Antigen für immuntherapeutische Strategien sollte möglichst tumorspezifisch exprimiert sein und es sollte einen Hinweis auf bereits erfolgte Immunantworten im Patienten geben, wie z.B. die Existenz spezifischer Antikörper oder zytotoxischer T-Zellen (CTL). Eine membranständige Lokalisation ist für die Verwendung von Tumorantigenen in Antikörpertherapien notwendig. Während für viele Neoplasien Tumorantigene bekannt sind, wurden für das kutane T-Zell Lymphom (CTCL) bislang nur sehr wenige tumorassoziierte Antigene identifiziert. Die Antigene se57-1, se70-2, cTAGE-1 und GBP-5ta wurden durch serologisches Durchsuchen einer Phagenbank aus Testis- bzw. Tumorgewebe (SEREX-Methode) identifiziert. In der vorliegenden Arbeit wurde die Immunogenität dieser vier Tumorantigene in einem neu entwickelten ELISA mit CTCL-, Parapsoriasis-, Melanom- und Kontrollseren untersucht. se70-2 und cTAGE-1 Protein erkannten nur wenige Patientenseren. Für GBP-5ta konnte dagegen eine signifikant höhere Reaktivität der CTCL-Seren im Vergleich zu den Kontrollseren ermittelt werden. Bei se57-1 waren die CTCL- und die Parapsoriasisseren hoch signifikant verschieden zu den Kontrollseren. Dieses putativ virusinduzierte Antigen sollte in zukünftigen Arbeiten auf seine mögliche Funktion als Entzündungsmarker weiter untersucht werden. Für das CTCL sollten weitere Kombinationen von Tumorantigenen auf ihren diagnostischen Wert in der Serologie getestet werden. Des Weiteren konnten in dieser Arbeit die CTCL assoziierten Antigene se2-2 und die GBP-5 Familie genauer charakterisiert werden: Die Expressionsanalyse von se2-2 Protein und mRNA in verschiedenen Normalgeweben zeigte ein differentielles Expressionsmuster. Im SEREX wurde se2-2 serologisch spezifisch nur von CTCL-Seren erkannt. Möglicherweise wäre se2-2 eine geeignete Zielstruktur für die serologische Diagnostik des CTCL. Aufgrund seiner fehlenden Tumorspezifität ist se2-2 für die Immuntherapie jedoch wenig geeignet. Die neu identifizierte GBP-5 Familie besteht aus mindestens drei Spleißvarianten (GBP-5ta, GBP-5a und GBP-5b), die zwei Proteine, GBP-5ta und GBP-5a/b, kodieren. GBP-5ta ist gegenüber GBP-5a/b C-terminal um 97 AS verkürzt. GBP-5ta mRNA wird differentiell exprimiert, während GBP-5ta Protein PBMC-spezifisch exprimiert wird. In CTCL-Tumorgewebe konnte GBP-5ta nachgewiesen werden, wogegen in Melanomzelllinien fast ausschließlich GBP-5a/b vorliegt. Gegen GBP-5ta konnte eine humorale Immunantwort bei CTCL-Patienten nachgewiesen werden: Im SEREX wurde GBP-5ta nur von CTCL-Patientenseren erkannt. Auch in der ELISA-Methode reagierten signifikant mehr Patientenseren als Kontrollseren mit GBP-5ta. Die höhere Immunogenität von GBP-5ta gegenüber GBP-5a/b im SEREX unterstreicht die Bedeutung der verkürzten Variante. Ob CTL gegen GBP-5ta präsentierende Zellen existieren, wird momentan untersucht. Die GBP-5 Spleißvarianten sind hoch homolog zur Familie der GTPasen, zu denen auch das Onkogen Ras gehört. Das verkürzte Protein von GBP-5ta könnte durch den Verlust der C-terminalen Domäne seine eventuelle anti-proliferierende Funktion verlieren. Ein Knock-out Versuch von GBP-5 könnte die Bedeutung von GBP-5 in der Tumorzelle untersuchen. Darüber hinaus wäre es vielversprechend, die GTPase Aktivität der GBP-5 Varianten in einem GTP-Bindungs-Assay zu überprüfen. GBP-5ta könnte eine mögliche Ursache des unkontrollierten Wachstums der Tumorzelle und somit eine vielversprechende potentielle Zielstruktur für therapeutische Ansätze für das CTCL sein.
N2  - Immunotherapies represent a promising concept of tumor-therapies on the basis of well-characterized, tumor-specific antigens. A potential antigen for immunotherapeutic strategies should be preferably tumor-specific expressed and should give a reference to immune responses in the patient, already taken place, as by antibodies or cytotoxic T-cells (CTL). A localization in the membrane is necessarily for antibody therapies. While for many neoplasia tumor antigens are known, the cutaneous t-cell lymphoma (CTCL) so far only very few tumor-associated antigens were identified. The tumor antigens, se57-1, se70-2, cTAGE-1 and GBP-5ta were identified by screening a testis and tumor tissue phage library (SEREX approach). In this work the immunogenicity of this four antigens was investigated in a newly developed ELISA using sera from CTCL, Parapsoriasis and melanoma patients as well as healthy controls. The ELISA results showed that only few patient sera reacted against se70-2 and cTAGE-1. CTCL sera reacted significantly more frequent against GBP-5ta than control sera. se57-1 protein was detected by sera from CTCL and Parapsoriasis patients, but hardly by any control sera. This putativ virus-induced antigen should be further examined for its possible function as inflammation marker. For the CTCL further combinations of tumor antigens should be tested to their diagnostic value. The CTCL associated antigens se2-2 and antigens of the GBP-5 family could be characterized in this work. The expression analysis of se2-2 protein and mRNA in different control tissues showed a differential expression. Secondary screening by SEREX indicated a serological specificity for se2-2. se2-2 could be a suitable target for serological diagnostic of the CTCL but due to its missing expression specificity se2-2 is little suitable for immunotherapy. The newly identified GBP-5 family consists of at least three splicing variants (GBP-5ta, GBP-5a and GBP-5b), coding for two proteins, GBP-5ta and GBP-5a/b. GBP-5ta is C-terminally truncated by 97 aa in comparison to GBP-5a/b. GBP-5ta mRNA is differentially expressed, while GBP-5ta protein is PBMC-specific. GBP-5ta is expressed in CTCL tumor tissue, while in melanoma cell lines almost exclusively GBP-5a/b was found. A humoral immune response in CTCL patients against GBP-5ta could be: SEREX indicated a serological specificity. Accordingly to the ELISA method significantly more patients` sera than control sera reacted against GBP-5ta. The higher immunogenicity of GBP-5ta in comparison to GBP-5a/b underlines the importance of the shortened variant. Whether CTL exist against GBP-5ta epitopes presently examined. The GBP-5 splicing variants are highly homologous to the GTPase superfamily including the ras oncogen. The loss of the C-terminal domain might be one reason why the truncated protein GBP-5ta loses its possible anti-proliferating function. GBP-5 knockout experiments could examine the meaning of GBP-5 in the tumor cell. Beyond that, it would be promising to examine the GTPase activity of the GBP-5 variants in a GTP-binding-assay. GBP-5ta could be a possible cause of the uncontrolled growth of the tumor cell and thus a promising potential target for therapy for the CTCL.
KW  - Hautlymphom
KW  - Tumorantigen
KW  - CTCL
KW  - Tumorimmunologie
KW  - Guanylat bindende Proteine
KW  - Entzündung
KW  - ELISA
KW  - CTCL
KW  - tumor immunology
KW  - guanylate binding proteins
KW  - inflammation
KW  - ELISA
Y1  - 2003
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-7561
ER  - 
TY  - THES
A1  - Guderian, Frank
T1  - Zellulärer und gewebsspezifischer Nachweis von C-reaktivem Protein
T1  - Cellular and tissue-specific detection of c-reactive protein
N2  - Der Serum-CRP-Wert ist bei verschiedenen atherosklerotisch bedingten Erkrankungen und bei Nierenerkrankungen erhöht. Ob das CRP dabei eine pathophysiologische Rolle spielt oder eher nur als Marker fungiert, ist bisher nicht bekannt. Im Rahmen dieser Arbeit wurde die Bildung von CRP auf zellulärer Ebene und der Nachweis von CRP bei diabetischen Patienten mit chronischer Nierenerkrankung untersucht.
N2  - Serum levels of C-reactive protein (CRP) increase during various atherosclerotic as well as kidney diseases. Whether CRP plays a pathophysiological role or rather serves as a marker is unknown. Here, we investigated the production of CRP and its role in diabetic patients with chronic kidney disease.
KW  - Clone 8
KW  - C-raktives Protein
KW  - diabetische Nephropathie
KW  - Entzündung
KW  - mCRP
KW  - clone 8
KW  - C-reactive protein
KW  - diabetic nephropathy
KW  - inflammation
KW  - modified CRP
Y1  - 2004
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-13448
ER  - 
TY  - THES
A1  - Timmermann, Meike
T1  - Zelluläre Regulation und klinische Aspekte des monocyten-/macrophagenspezifischen Proteins CD163
T1  - Cellular regulation and clinical aspects of the monocyte/macrophage-specific protein CD163
N2  - In der vorliegenden Arbeit wurde die zelluläre Regulation des monocyten-/ macrophagenspezifischen Oberflächenproteins CD163 untersucht und klinische Aspekte der löslichen Form des CD163 (sCD163) diskutiert. sCD163 wird in vivo durch einen inflammatorischen Reiz von der Zelloberfläche abgespalten. Bislang waren jedoch noch keine Mediatoren charakterisiert worden, die immer unter Entzündungsbedingungen vorhanden sind. In den eigenen Untersuchungen des Shedding von CD163 konnten für die Generierung des sCD163 neue endogene Aktivatoren identifiziert werden. Sowohl reaktive Sauerstoffspezies, wie Wasserstoffperoxid oder Stickstoffmonoxid, als auch das Produkt von endogenen Oxidationsreaktionen mit reaktiven Sauerstoffspezies 8-iso Prostaglandin F2a erwiesen sich als potente Aktivatoren des Shedding von CD163. Neben den bekannten physiologischen Funktionen des 8-iso Prostaglandin F2a konnte erstmals eine neue Funktion bei Entzündungen definiert werden. Dieser Effekt wurde spezifisch durch 8-iso Prostaglandin F2a hervorgerufen, da das isomere Prostaglandin F2a unter gleichen Bedingungen keinen Einfluss auf das Shedding von CD163 ausübte. Das Immunsuppressivum Cyclosporin A konnte ebenfalls als Induktor des Shedding von CD163 ermittelt werden. Damit konnte zusätzlich zur bekannten immunmodulatorischen Wirkung des Cyclosporin A eine weitere antiinflammatorische Wirkung über Monocyten/Macrophagen aufgezeigt werden. Durch Untersuchungen der Inhibierung des Shedding von CD163 konnten Gemeinsamkeiten bezüglich der in die sCD163-Generierung involvierten Mediatoren dargestellt werden. Obwohl die untersuchten Verbindungen wahrscheinlich über unterschiedliche Signalwege das Shedding von CD163 induzieren, waren die Anwesenheit von reaktiven Sauerstoffspezies und intrazellulärem Calcium und die Beteiligung einer TIMP-3-sensitiven Metalloproteinase an diesem Prozess essentiell. Bei einem Vergleich zwischen dem Shedding von CD163 und Tumor necrosis factor-a (TNF-a) ergaben sich Gemeinsamkeiten durch die Induktion des Shedding beider Verbindungen durch 8-iso Prostaglandin F2a und in sehr viel geringerem Maße durch Wasserstoffperoxid. Im Gegensatz dazu waren deutliche Unterschiede in dem Ausmaß der induzierten Stimulation des Shedding durch Stickstoffmonoxid, Prostaglandin F2a und Cyclosporin A zu erkennen. Im Hinblick auf die entgegengesetzten Wirkungen von sCD163 als antiinflammatorisch wirkende Verbindung und TNF-a als proinflammatorisches Cytokin, konnte dargestellt werden, dass die Freisetzung durch unterschiedliche Aktivatoren erfolgt. Nach Bestimmung der Konzentrationen von sCD163 und 8-iso PGF2a in bronchoalveolärer Lavage-Flüssigkeit von Patienten mit Cystischer Fibrose konnten keine abschließende Aussagen über die Eignung beider Parameter als biologische Marker für chronische Entzündungen der Lunge bei diesen Patienten getroffen werden. Weiterführend zu der Kenntnis, dass sCD163 die antiinflammatorische Wirkung über eine Interaktion des Proteins mit humanen T-Lymphocyten und nachfolgender Hemmung der Proliferation dieser Zellen ausübt, wurde diese Wechselwirkung genauer untersucht. In quantitativen Bestimmungen des sCD163 in isolierten T-Lymphocyten verschiedener Spender konnte erstmals gezeigt werden, dass sCD163 zu einem Teil konstitutiv in die T-Lymphocyten aufgenommen wird und dass diese Aufnahme durch proinflammatorische Aktivierung der T-Lymphocyten stark gesteigert werden kann. Durch fluoreszenzmikroskopische Aufnahmen unstimulierter T-Lymphocyten konnte die intrazelluläre Lokalisation des sCD163 visualisiert werden. Nach Aktivierung der Zellen mit einem proinflammatorischen Reiz fand innerhalb der Zellen eine Translokalisation des sCD163 aus dem cytoplasmatischen Bereich zur Zellmembran statt. Damit konnte erstmals gezeigt werden, dass abhängig vom Aktivierungsstatus der T-Lymphocyten eine Umverteilung des sCD163 innerhalb der Zellen erfolgt. Eine quantitative Bestimmung des sCD163 und seines Bindungspartners in T-Lymphocyten nichtmuskuläres Myosin Typ IIA gelang mittels eines neu entwickeltem ELISA, der spezifisch sCD163 und Myosin ausschließlich im Komplex erfasst. Damit konnte durch die in dieser Arbeit beschriebenen Untersuchungen ein grundlegender Beitrag zur Charakterisierung der Regulation der Proteinexpression und des Shedding von CD163 in humanen Monocyten sowie der Interaktion des sCD163 mit T-Lymphocyten geleistet werden.
N2  - In the present thesis, cellular regulation of the monocyte/macrophage specific membrane protein CD163 was investigated and clinical aspects of the soluble form of CD163 (sCD163) were discussed. sCD163 is shed from the cell surface in vivo upon an inflammatory stimulus. So far no mediators had been characterized that are persistently present under inflammatory conditions. In the present investigation of the shedding of CD163, new endogenous activators for the generation of sCD163 were successfully identified. Both reactive oxygen species, as hydrogen peroxide or nitric monoxide, and the product of endogenous oxidative reactions 8-iso prostaglandin F2a turned out to be potent activators of the shedding of CD163. In addition to the known physiological functions of 8-iso prostaglandin F2a a novel function of this compound in inflammation was defined. This effect was specifically generated by 8-iso prostaglandin F2a as prostaglandin F2a did not influence the shedding of CD163 under the same conditions. The immunosuppressive drug cyclosporine A was also established as an inductor of the shedding of CD163. Accordingly, another anti-inflammatory effect via monocytes/macrophages was pointed out in addition to the well known immunomodulatory effects of cyclosporine A. Investigations of the inhibition of shedding of CD163 led to the identification of key mediators involved in the generation of sCD163. Even though the tested compounds may induce shedding via different signal transduction pathways, the presence of reactive oxygen species and intracellular calcium and the involvement of a TIMP-3 sensitive metalloproteinase were essential in this process. The tested activators revealed different abilities for inducing the formation of reactive oxygen species. Comparing shedding of CD163 and tumor necrosis factor-a (TNF-a), similarities in induced shedding by 8-iso prostaglandin F2a and to a lower extend by hydrogen peroxide were seen. In contrast, significant differences were recognized in the extent of shedding induced via stimulation by nitric oxide, prostaglandin F2a, and cyclosporine A. With regard to the opposite effects of sCD163 as an anti-inflammatory compound and TNF-a as a pro-inflammatory cytokine it was demonstrated that shedding occurred via induction by different activators. The determination of concentrations of sCD163 and 8-iso prostaglandin F2a in bronchoalveolar lavage fluid of patients with cystic fibrosis allowed no conclusive statement about the suitability of both parameters as marker for chronic inflammation. In extension to earlier insights in the anti-inflammatory effects of sCD163 via interaction of the protein with human T-lymphocytes and subsequent inhibition of the proliferation of these cells these interactions were analyzed in detail. Quantifications of sCD163 in isolated T-lymphocytes from different donors revealed for the first time that sCD163 is constitutively taken up into T-lymphocytes and that this process can significantly be enhanced by pro-inflammatory activation of T-lymphocytes. The intracellular localization of sCD163 was visualized by fluorescence microscopy of T-lymphocytes. Upon activation of the cells by a pro-inflammatory stimulus a translocalization of sCD163 was observed within the cells from the cytoplasmatic region to the cell membrane. Thus, it was shown for the first time that an activation dependent translocalization of sCD163 occurs within the T-lymphocytes. The quantitative determination of sCD163 and non-muscular myosin type IIA as its intracellular binding partner in T-lymphocytes was successful using a newly developed ELISA that detects specifically sCD163 and myosin as a complex. To conclude, the investigations described in this thesis contributed substantially to the understanding of the regulation of the protein expression and shedding of CD163 in human monocytes and of the interaction of sCD163 with T-lymphocytes.
KW  - Antigen CD163
KW  - Monozyt
KW  - Entzündung
KW  - Prostaglandine
KW  - CD163
KW  - Monocyten
KW  - Regulation
KW  - Entzündung
KW  - Isoprostaglandin
KW  - CD163
KW  - monocytes
KW  - regulation
KW  - inflammation
KW  - isoprostaglandin
Y1  - 2005
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-16028
ER  - 
TY  - THES
A1  - Wienrich, Bernd Gregor
T1  - Expression von LEEP-CAM (Lymphocyte Endothelial EPithelial-Cell Adhesion Molecule) in Haut und Hoden - funktionelle Implikationen für die Immunevasion epithelialer Hauttumoren und Entzündungen immunprivilegierter Gewebe
T1  - Expression of LEEP-CAM (Lymphocyte Endpthelial EPithelial-Cell Adhesion Molecule) in Skin and testis –functional implication of immunevasion in epithelial skincancer and inflammation in immunologically privileged tissue
N2  - Der Schutz vor der Einwanderung von Immunzellen ist einerseits unter physiologischen Bedingungen wichtig für die Integrität immunprivilegierter Organe, andererseits aber auch (mit)entscheidend für die Pathogenese maligner Tumoren. Vor diesem Hintergrund wurde LEEP-CAM (Lymphocyte Endothelial EPithelial-Cell Adhesion Molecule) untersucht, ein Adhäsionsmolekül, welches in der Epidermis und den dermalen Blutgefäßen in normaler Haut konstitutiv exprimiert wird. Durch immunhistochemische Untersuchungen wurde im ersten Teil der Arbeit gezeigt, dass LEEP-CAM in Basalzellkarzinomen, Plattenepithelkarzinomen und Keratoakanthomen der Haut deutlich vermindert oder gar nicht exprimiert wird. Die verminderte Expression war mit fehlender Infiltration von T-Lymphozyten in das Tumorgewebe assoziiert, was insbesondere durch zwei hinsichtlich ihrer LEEP-CAM-Expression unterschiedenen Populationen von Keratoakanthomen nahe gelegt wurde. Die Hypothese, dass LEEP-CAM in die epidermale Rekrutierung aktivierter T-Zellen involviert ist, wurde durch funktionelle Stamper-Woodruff-Experimente (Adhäsion aktivierter T-Lymphozyten an Gewebe-Gefrierschnitte) mit Basalzellkarzinomen und psoriatischer Haut gestützt. Durch metabolische Markierung mit 35(S)-Methionin und anschließende Radioimmunpräzipitation sowie durch durchflusszytometrische Untersuchungen an kultivierten Zellen wurde gezeigt, dass LEEPCAM in transformierten Keratinozyten im Vergleich zu normalen Keratinozyten deutlich vermindert synthetisiert und exprimiert wird. In zwei komplementären murinen Karzinogenese-Modellen wurde die Assoziation der verminderten LEEP-CAM-Expression mit Entdifferenzierung und invasivem Wachstum der Tumorzellen untermauert. Insgesamt kann experimentelle Evidenz für die Hypothese, dass die Herabregulation der LEEP-CAM-Expression ein (Teil)-Mechanismus ist, durch welchen sich invasiv wachsende Tumoren den Angriffen des Immunsystems entziehen können, präsentiert werden. Im Weiteren wurde die Expression und Funktion von LEEPCAM im Keimepithel des Hodens (als ein Beispiel für ein immunprivilegiertes Gewebe) untersucht. Durch immunhistochemische Untersuchungen wurde die konstitutive Expression von LEEP-CAM in den Sertoli-Zellen des Keimepithels nachgewiesen. Mittels Immun-Elektronenmikroskopie wurde dann die Lokalisation an desmosomalen Strukturen sowie entlang der Zellmembran gezeigt. Im Hinblick auf die Funktion von LEEP-CAM wurde in modifizierten Stamper-Woodruff-Experimenten erstmals gezeigt, dass aktivierte T-Lymphozyten an das Keimepithel des Hodens binden können und dass diese Adhäsion durch LEEP-CAM-gerichtete Antikörper inhibiert werden kann. Damit ist LEEP-CAM das erste Molekül, für welches direkte experimentelle Evidenz eine mögliche Rolle bei der testikulären Lymphozyten-Rekrutierung belegt. Dies könnte Relevanz für die Pathogenese von Orchitiden, den häufigsten Ursachen männlicher Infertilität, haben.
N2  - Under physiologic conditions protection of invading immune cells is on one hand important for integrity of immune-privileged organs and on the other hand crucial for the pathogenesis of malignant tumors. In the current thesis LEEP-CAM (Lymphocyte Endothelial Epithelial-Cell Adhesion Molecule), an adhesion molecule which is expressed in the epidermis and dermal blood vessels was investigated. In immunohistochemical stains LEEP-CAM expression was dramatically reduced or absent in basal cell carcinoma, squamous cell carcinoma or keratoacanthoma. Reduced expression was associated with lack of infiltrating T-lymphocytes in the tumor tissue, which was especially obvious in keratoacanthoma. The hypothesis that LEEP-CAM is involved in epidermal recruiting of activated T cells was verified by functional Stamper-Woodruff experiments (adhesion of activated T lymphocytes to frozen tissue sections) for basal cell carcinoma and psoriasis. By metabolic labeling with 35-S-methionin and subsequent radioimmuno-precipitation and additional FACS analysis we could demonstrate, that LEEP-CAM synthesis and expression was reduced in transformed keratinocytes in comparison to primary keratinocytes. The association of reduced LEEP-CAM expression with differentiation and invasive tumor growth was confirmed in two complementary murine carcinogenesis models. In summary, reduced expression of LEEP-CAM may be a mechanism by which invasive tumors are capable of escaping the immune surveillance. In the second part of the thesis, expression and function of LEEP-CAM in the testis was investigated. Constitutive expression of LEEP-CAM was identified immunhistochemically in Sertoli cells. By immunoelectron microscopy LEEP-CAM was localized to desmosomal structures and along the cell membrane. Functional analysis by modified Stamper-Woodruff experiments demonstrated the capability of activated T-lymphocytes to bind to germinal tissue of human testis. This adhesion could be blocked by anti-LEEP-CAM-antibodies. Our studies suggest that LEEP-CAM may the first molecule which is involved in lymphocyte testicular recruitment. This may be relevant for the pathogenesis of orchtitis.
KW  - Zell-Adhesionsmolekül
KW  - Hoden
KW  - Haut
KW  - Hauttumor
KW  - Hautkrebs
KW  - Basaliom
KW  - Epitheliom
KW  - Spinaliom
KW  - Endothel
KW  - Epithel
KW  - Keimepithel
KW  - Plattenepithel
KW  - Keratoakant
KW  - LEEP-CAM
KW  - adhesion molecule
KW  - inflammation
KW  - human testis
KW  - LEEP-CAM
KW  - adhesion molecule
KW  - inflammation
KW  - human testis
Y1  - 2006
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-27872
ER  - 
TY  - THES
A1  - Müller, Verena
T1  - Candida albicans-induzierte Genexpression in primären humanen Endothelzellen - Mechanismen der Signaltransduktion und Möglichkeiten der Intervention
T1  - Candida albicans-induced gene expression in primary human endothelial cells - mechanisms of signal transduction and possibilities of intervention
N2  - Endothelzellen sind ein aktiver Bestandteil der angeborenen Immunabwehr des Menschen gegen mikrobielle Pathogene. Unter ungünstigen Bedingungen kann die Abwehrreaktion sogar zu einer lebensbedrohlichen Sepsis führen. Hier wurde die bislang wenig bekannte Endothelantwort auf den fakultativ humanpathogenen Hefepilz Candida albicans, einem der häufigsten Verursacher von letaler Sepsis beim Menschen, näher untersucht. Mittels Oligonukleotid-Mikroarray-Analyse von HUVEC nach Exposition mit C. albicans konnten 56 hochregulierte Gene identifiziert werden, während 69 Gene herunterreguliert wurden. Ein bedeutender Anteil der regulierten Gene ist an Prozessen der angeborenen Immunantwort beteiligt und dient hauptsächlich der Rekrutierung von Neutrophilen. Weitere Untersuchungen ergaben eine zentrale Rolle des proinflammatorischen NF-kappaB-Weges bei der Regulation des Candida-induzierten Transkriptoms von Endothelzellen. Es konnte gezeigt werden, dass C. albicans diesen Signalweg sequenziell aktiviert. Zusätzlich konnte durch die Expression einer dominant-negativen Mutante einer Signalkomponente des NF-kappaB-Signalwegs die Candida-vermittelte Induktion von kappaB-abhängigen Genen gehemmt werden. Mit einem pharmakologischen Ansatz wurde der p38 MAP Kinase-Signalweg als weiterer bedeutsamer Signalweg identifiziert, der die Expression einzelner Candida-Zielgene wie CXCL8/IL-8 moduliert. Schließlich wurde gezeigt, dass die Candida-induzierte NF-kappaB-Aktivierung im untersuchten endothelialen Zellsystem unabhängig von den Toll-like Rezeptoren TLR2 und TLR4 geschieht, die üblicherweise an der Erkennung mikrobieller Pathogene beteiligt sind. Durch RNA-Interferenz-Experimente konnte jedoch dargelegt werden, dass das Adaptermolekül MyD88 und die Kinase IRAK1, die beide entscheidend an der TLR-vermittelten Signaltransduktion beteiligt sind, essentiell für die Weiterleitung des Signals in Endothelzellen sind. Nachfolgend konnte mit TLR3 zumindest einer der signaltransduzierenden Rezeptoren identifiziert werden. Als erste umfassende Untersuchung der endothelialen Antwort auf Candida albicans erlaubt die vorliegende Arbeit neue Einblicke in die komplexen Signalmuster von Endothelzellen, die dieser klinisch bedeutende Krankheitserreger auslöst.
N2  - Endothelial cells (ECs) actively participate in the innate defence against microbial pathogens. Under unfavourable conditions defence reactions can even turn into life-threatening responses resulting in sepsis. Here the so far largely unknown EC reaction patterns to Candida albicans were studied. C. albicans is a facultative human pathogenic fungus and a major cause of lethality in septic patients. Oligonucleotide microarray analysis revealed 56 genes that were transcriptionally up-regulated and 69 that were suppressed upon exposure of ECs to C. albicans. A major portion of these genes is involved in defence mechanisms of the innate immune system with a high representation of genes serving the recruitment of neutrophils to sites of infection. Further examination of candidate signalling cascades established a central role of the proinflammatory NF-kappaB pathway in the regulation of the Candida-modulated transcriptome of ECs. It was shown that the NF-kappaB signalling pathway becomes activated at various levels. In addition, expression of a dominant negative mutant of a NF-kappaB signalling pathway compound blocked the Candida-induced kappaB-dependent gene expression. Using a pharmacological approach the stress-activated p38 mitogen-activated protein (MAP) kinase pathway was identified as a second major regulatory pathway which critically contributes to the regulation of selected Candida target genes such as CXCL8/IL-8. Candida-induced NF-kappaB activation is mediated independently of Toll-like receptors (TLR) 2 and 4 that commonly have been implicated with microbial pattern recognition. Nevertheless, knock-down of the adapter molecule MyD88 and the essential downstream kinase of TLR-, IL-1R- and IL-18R-signalling, IRAK1, suggested that recognition and signalling via a TLR apart from TLR2/TLR4 is crucial for Candida-induced gene expression in primary ECs. Finally, RNAi experiments indicate that most likely TLR3 represents this receptor. These data provide the first comprehensive analysis of endothelial gene responses to Candida albicans and present novel insights into the complex signalling patterns triggered by this important pathogen.
KW  - Angeborene Immunität
KW  - Endothelzelle
KW  - Toll-like-Rezeptoren
KW  - Candida albicans
KW  - Entzündung
KW  - innate immunity
KW  - endothelial cell
KW  - toll-like receptors
KW  - Candida albicans
KW  - inflammation
Y1  - 2007
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-26224
ER  - 
TY  - THES
A1  - Schopf, Thilo
T1  - Wertigkeit von Entzündungsparametern in der postoperativen Phase nach Implantation von Hüft- und Kniegelenk-Totalendoprothesen
T1  - relevance of inflammatory parameters after hip and knee arthroplasty
N2  - Ziel dieser Arbeit ist, die Wertigkeit von Entzündungsparametern (CRP, BSG, Leukozyten und Temperatur) in der postoperativen Phase anhand einer retrospektiven Studie mit 531 Patienten nach Implantation von Knie- und Hüft-Totalendoprothesen zu beurteilen. Hierbei sollten zum einen die Auswirkungen von Vorerkrankungen (Asthma bronchiale, Rheumatoider Arthritis, Nikotinabusus, Gicht/Hyperurikämie, Z. n. Thrombosen) auf den postoperativen Verlauf der Entzündungsparameter und zum anderen postoperative Komplikationen (Thrombosen, bronchopulmonale Infekte, Harnwegsinfekte, Wundinfekte, Protheseninfekte) anhand der Entzündungsparameter erfasst werden. Die Auswertung erfolgte mittels SPSS für Windows durch den Mann-Whitney Test als nicht parametrischen Test für unabhängige Variablen. Im Durchschnitt stieg der CRP-Wert von 0,6 mg/dl präoperativ auf etwa 8,5 mg/dl um den 3. postoperativen Tag an und fiel dann durchschnittlich auf 1,4 mg/dl um den 14. postoperativen Tag ab. Die BSG-Werte stiegen von etwa 18 mm/h präoperativ auf 52 mm/h um den 3. postoperativen Tag an. Der höchste BSG-Wert (56 mm/h) wurde erst um den 7. postoperativen Tag erreicht. Danach fiel der BSG-Wert leicht ab auf durchschnittlich etwa 43 mm/h um den 14. postoperativen Tag. Die Temperaturkurve verlief ähnlich: Auch hier stieg die Temperatur rasch auf einen Höchstwert von 37,1°C um den 2. postoperativen Tag. Es folgte ein langsamer Abfall der Temperatur, bis hin zu Normwerten ab dem 10. postoperativen Tag. Die Leukozyten zeigten im Durchschnitt einen geradlinigen Verlauf mit durchschnittlichen Werten zwischen 7 und 8 G/l, allerdings bei einer großen Standartabweichung. Patienten mit Asthma bronchiale zeigten präoperativ signifikant erhöhte BSG und Leukozytenwerte. Patienten mit Gicht/Hyperurikämie fielen durch signifikant niedrigere Temperaturwerte am 6. und 12. postoperativen Tag sowie durch Trends zu niedrigeren Werten am 10. und 16. postoperativen Tag auf. Signifikant höhere Werte fanden sich bei der CRP-AUC-Kurve vom 7.-14. postoperativen Tag. Des Weiteren fanden sich Trends zu höheren Werten am 14. postoperativen Tag bei der BSG und am 3. postoperativen Tag bei den Leukozyten. Bei Patienten mit Z.n. Thrombose zeigte sich der postoperative BSG-Verlauf vom 3.-14. Tag signifikant erniedrigt, ebenso waren die postoperativen Temperaturwerte vom 15. und 16. Tag signifikant niedriger. Der einzig signifikante Unterschied zwischen Rauchern und Nichtrauchern fand sich in der präoperativen BSG, wo Raucher signifikant niedrigere Werte hatten. Des Weiteren zeigten sich Trends zu höheren Leukozytenwerten am 3. und 7. postoperativen Tag sowie Trends zu niedrigeren Temperaturen am 1., 2., 7., 8. und 14. postoperativen Tag. Patienten mit Rheumatoider Arthritis fielen durch signifikant erhöhte präoperative CRP- und BSG-Werte auf. Zusätzlich traten Trends zu höheren Werten am 14. postoperativen Tag für CRP, BSG und Leukozyten auf. Dem Trend zur Temperaturerhöhung am 2. postoperativen Tag folgten erneute Trends am 9. und 11. postoperativen Tag sowie signifikant höhere Temperaturen am 10. und 12. postoperativen Tag. Patienten, die einen Harnwegsinfekt erlitten, hatten signifikant erhöhte Werte am 14. postoperativen Tag für CRP und BSG. Auch die CRP-AUC-Kurve zeigte diesen Verlauf signifikant. Bei Patienten, die an einem bronchopulmonalem Infekt erkrankten, war der CRP-Wert des 3. postoperativen Tages signifikant erhöht. Dies ließ sich auch in der CRP-AUC-Kurve vom 0.-3. postoperativen Tag signifikant nachweisen. Darüber hinaus lag ein Trend am 3.-7. postoperativen Tag zu höheren Werten vor. Bei Patienten mit tiefer Beinvenenthrombose fiel eine signifikante Temperaturerhöhung am 7., 8. und 11. postoperativen Tag auf, sowie ein Trend am 9., 10. und 12. postoperativen Tag. Die CRP-Werte stiegen um den 14. postoperativen Tag signifikant an. Gleiches Verhalten zeigte die CRP-AUC-Kurve vom 7.-14. postoperativen Tag. Patienten mit Wundinfektionen fielen durch Trends zu niedrigeren Temperaturwerten am 4. und 5. postoperativen Tag auf. Außerdem stieg um den 7. postoperativen Tag die BSG trendwertig an. Die Leukozyten waren präoperativ signifikant erhöht. Dagegen war bei Patienten mit TEP-Infektion der CRP-Wert um den 14. postoperativen Tag signifikant erhöht. Die Temperaturwerte des 8. postoperativen Tages zeigten einen Trend zu niedrigeren Zahlen. Die Ergebnisse entsprechen in etwa denen anderer Studien. Insgesamt lässt sich eine Tendenz ablesen: BSG und Temperatur sind vor allem bei den erwähnten Vorerkrankungen erhöht, Leukozyten spielen kaum eine Rolle und die CRP-Bestimmung findet ihren Platz hauptsächlich in der Diagnostik von Komplikationen. Außerdem wird klar, dass kein Entzündungsparameter spezifisch für eine bestimmte Vorerkrankung oder Komplikation ist. Darüber hinaus sind nicht Einzelwerte, sondern viel mehr der Verlauf der Entzündungsparameter entscheidend.
N2  - Blood parameter like CRP (C-reactive protein), ESR (erythrocyte sedimentation rate), white blood cells (leukocytes) and body temperature were messured after total hip and knee arthroplasty in 531 patients. The effects of bronchial asthma, rheumatiod arthritis, smoking, gout and a deep vein thrombosis in the past on inflammatory parameters were investigated, on the oher side we tried to check out, whether deep vene thrombosis, bronchial or pulmonary infections, urinary tract infections, wound infections or infections of the endoprothesis influence the developing of inflammatory parameters.
KW  - Totalendoprothese
KW  - Entzündung
KW  - Hüftgelenkentzündung
KW  - TEP
KW  - Komplikation
KW  - Laborparameter
KW  - Entzündungsparameter
KW  - postoperative Komplikationen
KW  - Endoprothese
KW  - inflammation
KW  - hip
KW  - knee
KW  - arthroplasty
KW  - complications
Y1  - 2007
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-25028
ER  - 
TY  - THES
A1  - Adamek, Anna Katharina
T1  - Einfluss des Immunsystems und der endothelialen NO-Synthase auf den myokardialen ischämischen Schaden
T1  - Influence of immune system and endothelial NO synthase on myocardial ischemic injury
N2  - Die Entwicklung von therapeutischen Strategien, die den infarktbedingten Untergang des Myokardgewebes minimieren und die Gewebsheilung nach abgelaufenem Myokardinfarkt unterstützen, gehört zu dem Hauptziel in der modernen Kardiologie. Bis jedoch eine spezifische Intervention als Therapieform anerkannt wird, ist ein detailliertes Entschlüsseln der zellulären und molekularen Mechanismen während und nach der Myokardschädigung notwendig. Die vorliegende Arbeit beschäftigt sich intensiv mit den Vorgängen der Stickstoffmonoxid- (NO) Produktion und der Inflammation nach Okklusion von Kranzarterien. Im ersten Teil der Dissertation steht die endotheliale NO-Synthase-Expression (eNOS) im Mittelpunkt der Untersuchung. eNOS ist als wichtiger Katalysator an der Biosynthese von Stickstoffmonoxid, das als protektiver Faktor für die Gefäßhomöostase seit Jahren bekannt ist, beteiligt. Ferner besteht experimentell sehr gute Evidenz dafür, dass der endothelialen NO-Synthase am Ausmaß des kardialen Ischämie-/ Reperfusionsschadens eine entscheidende Rolle zukommt. Folglich wurde mittels der Substanz AVE 9488 versucht, die eNOS-Expression in Mäusen zu steigern und den Effekt auf das Infarktgeschehen näher zu betrachten. Die Behandlung mit AVE 9488 erzielte einen signifikant reduzierten Ischämie-/Reperfusionsschaden. Bei anschließenden Ischämie-/Reperfusionsveruchen mit eNOS defizienten Mäusen war der protektive Effekt wieder aufgehoben. Der Erfolg dieser Substanz wird in der signifikanten Reduktion des oxidativen Stresses vermutet. Ein zusätzlicher wichtiger Parameter, der während der Ischämie/Reperfusion aktiviert wird, ist der Schlüssel-Transkriptionsfaktor Nuclear Factor kappa B (NF-kB). Durch seine Bindung an bestimmte Enhancer und Promotoren reguliert der Faktor die Entzündungsprozesse, indem er die Genexpression proinflammatorischer Marker verstärkt. Folglich wurden eine Reduktion der Inflammation sowie ein protektiver Effekt nach erfolgter ischämischer Schädigung durch Hemmung von NF-kB angenommen. Zur Prüfung dieser Hypothese wurden NF-kB-Untereinheit p50 defiziente Mäuse (p50 KO) einer Okklusion einer Herzkranzarterie unterzogen. Durch die Hemmung der NF-kB-Aktivierung kam es zu einer signifikanten Reduzierung des Infarktareals im Vergleich zu den entsprechenden Wildtyp-Mäusen. Der große Benefit konnte auf die geringere Einwanderung der neutrophilen Granulozyten in das infarzierte Gebiet zurückgeführt werden. Knochenmarktransplantationsversuche mit p50 KO- und Wildtyp-Knochenmark untermauerten die Beobachtung, dass die beeinträchtigte Aktivierung von NF-kB in p50 defizienten Leukozyten protektive Effekte in der Ischämie/Reperfusion vermittelt. Die Aktivierung der proinflammatorischen Proteine während des linksventrikulären Remodelings nach Myokardinfarkt gehört zum Fokus des dritten Teils dieser Arbeit. Dieser Teil beschäftigt sich mit der Frage, inwieweit eine hochdosierte Aspirin-Therapie die linksventrikulären Umbauprozesse günstig beeinflussen kann. Dafür wurden Mäuse für 4 Wochen mit Placebo oder Aspirin (120 mg/kg pro Tag) mittels osmotischer Mini-Pumpen, die 2 Stunden nach Ligatur der Kranzarterie implantiert wurden, behandelt. In beiden Gruppen kam es zur erwarteten linksventrikulären Dilatation nach Myokardinfarkt, jedoch ohne signifikanten Unterschied zwischen Placebo- und Aspirin-behandelten Tieren. Es kam allerdings zu einer erwarteten Reduktion proinflammatorischer Proteine durch die Aspirin-Therapie. So war die Expression von Tumor-Nekrose-Faktor-alpha; (TNF-alpha) und Interleukin-1ß (IL-ß) in der Aspirin-Gruppe signifikant reduziert. Zusammenfassend lässt sich sagen, dass durch die gezielte Beeinflussung bestimmter Faktoren in der Ischämie/Reperfusion wie z. B. die Verstärkung der eNOS-Expression oder die Hemmung der NF-kB-Aktivierung die Ischämieschädigung signifikant reduziert werden kann.
N2  - One of the major therapeutic goals of modern cardiology is to design strategies aimed at minimizing myocardial necrosis and optimizing cardiac repair following myocardial infarction. However, a sound understanding of the cellular and molecular mechanism is necessary before a specific intervention is pursued on a therapeutic basis. The present work includes important aspects of inflammation and nitric oxide (NO) production after occlusion of the coronary artery. The first part of the thesis focused on endothelial NO synthase (eNOS). eNOS is a promotor of NO biosynthesis, which regulates vascular and myocardial function. Moreover, endothelial NOS is cardioprotective in ischemia/reperfusion injury. Therefore, the effects of AVE 9488, a novel pharmacon designed to selectively increase eNOS protein expression and NO formation, was tested on cardiac ischemia/reperfusion injury in vivo. Ischemia/reperfusion damage was significantly reduced in mice treated with AVE 9488 when compared to placebo treated mice. The protective effect was blunted in eNOS knockout mice treated with the eNOS enhancer. The expression of inflammatory markers was not influenced by the therapy. Reactive oxygen species were significantly reduced in mice treated with the eNOS enhancer. In addition, the transcription factor nuclear factor kappa B (NF-kB) is important in cardiac damage. NF-kB is activated by various stimuli implicated in ischemia/reperfusion injury and increases the expression of proinflammatory markers by binding on special enhancer and promoters. Inhibition of NF-kB might therefore reduce the inflammatory response and achieve protective effects after myocardial infarction. To prove this hypothesis mice with targeted deletion of the NF-kB subunit p50 (p50 KO) underwent 30 minutes of coronary artery ligation and 24 hours of reperfusion in vivo. Ischemia/reperfusion damage was significantly reduced in the p50 KO animals when compared with matching wild-type (WT) mice. Although adhesion molecules such as intercellular adhesion molecule were up-regulated in left ventricles of p50 KO mice, fewer neutrophils infiltrated the infarct area, suggesting leukocytes as a potential mediator of the protection observed in the p50 KO. This was confirmed in adoptive transfer experiments: whereas transplantation of KO bone marrow in KO animals sustained the protective effect on ischemia/reperfusion injury, transplantation of WT bone marrow in KO animals abolished it. The last part tested the hypothesis that inhibition of the proinflammatory response to myocardial infarction could improve left ventricular remodeling. Therefore, mice were treated for 4 weeks with placebo or aspirin (120 mg/kg per day) by Alzet mini-osmotic pumps implanted 2 hours after ligation of the left anterior descending artery. On echocardiography, animals 4 weeks after myocardial infarction exhibited left ventricular dilatation as expected. However, there was no difference between the placebo and the Aspirin group. The expression of the proinflammatory cytokines tumor necrosis factor alpha; (TNF-alpha) and interleukin 1ß (IL-1ß) which were markedly upregulated in mice with myocardial infarction on placebo were significantly reduced by Aspirin treatment. However, left ventricular remodeling after myocardial infarction was not altered. In conclusion, the use of specific strategies to inhibit the NF-kB activation or to increase eNOS expression in ischemia/reperfusion constitutes a promising novel therapeutic approach to reduce ischemic damage. However, successful application of anti-inflammatory interventions in the treatment of ischemic remodeling will require a better understanding of the specific molecular steps in the regulation of cardiac injury and repair.
KW  - Ischämie
KW  - Reperfusion
KW  - Entzündung
KW  - Oxidativer Stress
KW  - ischemia
KW  - reperfusion
KW  - inflammation
Y1  - 2008
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-35795
ER  - 
TY  - THES
A1  - Schwab, Nicholas
T1  - The importance of CD8\(^+\) T cells and antigen-presenting cells in the immune reaction of primary inflammatory versus degenerative diseases
T1  - Die Bedeutung CD8\(^+\) T-Zellen und Antigen-präsentierender Zellen in der Immunreaktion primär inflammatorischer gegenüber degenerativen Erkrankungen
N2  - The bidirectional influence of parenchymal cells and cells of the immune system, especially of antigen-presenting and CD8\(^+\) T cells, in situations of putative auto- immune pathogenicity and degeneration was the main topic of this thesis. In the first part, the influence of human muscle cells on antigen-presenting cells was investigated. In inflammatory myopathies prominent infiltrates of immune cells containing T cells and antigen-presenting cells like macrophages and dendritic cells are present. The hypothesis was that human myoblasts have an inhibiting influence on these antigen-presenting cells under homeostatic conditions. A dysfunction or impairment under inflammatory circumstances might contribute to the development of myopathic conditions. The surface analysis of dendritic cells cocultured with myoblasts showed that immature dendritic cells could be driven into a reversible semi- mature state with significantly elevated levels of CD80. These dendritic cells were additionally characterized by their inhibiting function on T-cell proliferation. It was also shown that the lysates of healthy myoblasts could strongly enhance the phagocytic ability of macrophages, which could help with muscle regeneration and which might be disturbed in myositis patients. The second part of this thesis was about the clonal specificity of CD8\(^+\) T cells in a mouse model with genetically induced over-expression of PLP in oligodendrocytes. Here, we could show that the cytotoxic T lymphocytes, which had previously been shown to be pathogenic, were clonally expanded in the CNS of the transgenic mice. The amino acid sequences of the corresponding receptor chains were not identical, yet showed some similarities, which could mean that these clones recognize similar antigens (or epitopes of the same antigen). The knockout of PD-1 in this setting allowed for an analysis of the importance of tissue immune regulation. It became evident that the absence of PD-1 induced a larger number of clonal expansions in the CNS, hinting towards a reduced threshold for clonal disturbance and activation in these T cells. The expansions were, however, not pathogenic by themselves. Only in the presence of tissue damage and an antigenic stimulus (in our case the overexpression of PLP), the PD-1 limitation exacerbated the immune pathogenicity. Therefore, only in the presence of a “tissue damage signal”, the dyshomeostasis of T cells lacking PD-1 achieved high pathogenetic relevance. Finally, we investigated the pathogenetic role of CD8 T cells in Rasmussen encephalitis, a rare and chronic neurological disease mainly affecting children. The analysis of the T-cell receptor repertoire in Rasmussen encephalitis patients in the peripheral CD4\(^+\) and CD8\(^+\) T-cell compartments as well as the brain revealed the involvement of T cells in the pathogenicity of this disease. Many clonal expansions in the brain matched CD8\(^+\) T-cell expansions in the periphery on the sequence level. These putatively pathogenic clones could be visualized by immunohistochemistry in the brain and were found in close proximity to astrocytes and neurons. Additionally, the expanded clones could be found in the periphery of patients for at least one year.
N2  - Der Einfluss von Parenchymzellen auf Immunzellen und umgekehrt, im Besonderen von Antigen-präsentierenden Zellen und CD8\(^+\) T-Zellen, im Zusammenhang von auto- immuner Pathogenese und Degeneration war das Hauptthema dieser Dissertation. Im ersten Teil wurde der Einfluss menschlicher Muskelzellen auf Antigen- präsentierende Zellen untersucht. In entzündlichen Myopathien kommt es zu massiven Infiltraten von Immunzellen, die T-Zellen und auch Antigen-präsentierende Zellen wie Makrophagen und dendritische Zellen enthalten. Die Hypothese war, dass menschliche Myoblasten einen hemmenden Einfluss auf die Antigen-präsentierenden Zellen unter homöostatischen Bedingungen haben. Eine Störung dieses Einflusses oder eine Beeinträchtigung unter entzündlichen Rahmenbedingungen könnte eventuell zur Entwicklung eines myopathischen Zustands beitragen. In der Oberflächenanalyse der dendritischen Zellen, die mit Myoblasten kultiviert wurden, zeigte sich, dass unreife dendritische Zellen in einen halb-reifen Zustand versetzt werden konnten, der sich beispielsweise durch stark erhöhte CD80 Expression kennzeichnet. Diese dendritischen Zellen wurden weiterhin charakterisiert über ihre hemmende Funktion auf die T-Zell Proliferation. Außerdem wurde gezeigt, dass Zelllysate gesunder Myoblasten die Phagozytoserate von Makrophagen enorm verstärken, was die Regeneration des Muskelgewebes erhöhen und möglicherweise in Myositispatienten gestört sein könnte. Im zweiten Teil der Dissertation ging es um die klonale Spezifität von CD8\(^+\) T-Zellen in einem Mausmodell mit genetisch induzierter Überexpression von PLP in Oligodendrozyten. Hier konnte gezeigt werden, dass die zytotoxischen T-Zellen, deren Pathogenität Gegenstand früherer Arbeiten war, im ZNS der transgenen Mäuse klonal expandiert waren. Die Aminosäuresequenzen der TCRβ Kette der expandierten Klone waren nicht identisch, zeigten jedoch einige Ähnlichkeiten, die darauf hinweisen könnten, dass diese Klone ähnliche Antigene (oder Epitope des gleichen Antigens) erkennen. Die genetisch induzierte Abwesenheit von PD-1 ermöglichte es, in diesem Zusammenhang den Einfluss von spezifischer Immunregulation im Gewebe zu untersuchen. Es zeigte sich, dass die Deletion von PD-1 eine erhöhte Anzahl von klonalen Expansionen im ZNS der Mäuse erzeugte, was auf eine herabgesetzte Schwelle für klonale Störungen und Aktivierung schließen lässt. Diese Expansionen 
 waren jedoch für sich genommen nicht pathogen. Nur in der Anwesenheit eines Gewebeschadens und eines zusätzlicher Antigenstimulus (in unserem Fall in Form der PLP Überexpression) konnte man die erhöhte Pathogenität durch die PD-1 Deletion erkennen. Deswegen erreichten die PD-1 deletierten T-Zellen nur in der Gegenwart eines „Gewebeschaden-Signals“ hohe pathogenetische Relevanz. Schließlich untersuchten wir die pathogenetische Rolle von CD8\(^+\) T-Zellen in der Rasmussen Enzephalitis, einer seltenen, chronischen Erkrankung des Gehirns, die hauptsächlich in Kindern vorkommt. Die Analyse des T-Zell-Rezeptor Repertoires in Rasmussen Enzephalitis Patienten in peripheren CD4\(^+\) und CD8\(^+\) T-Zell Populationen und im Gehirn zeigte die Beteiligung von T-Zellen in der Pathogenese dieser Krankheit auf. Viele klonale Expansionen waren zwischen Gehirn und der peripheren CD8\(^+\) Population bis hin zur Aminosäuresequenz identisch. Diese vermutlich pathogenen Klone konnten in Gehirnbiopsien von Rasmussenpatienten histochemisch nachgewiesen werden und wurden in enger Nachbarschaft zu Astrozyten und Neuronen gefunden. Zusätzlich konnten diese expandierten Kone in der Peripherie von Patienten für die beobachteten Zeiträume (mindestens ein Jahr) nachgewiesen werden.
KW  - T-Lymphozyt
KW  - Entzündung
KW  - Degeneration
KW  - Immunsystem
KW  - Rasmussen-Syndrom
KW  - T lymphocyte
KW  - inflammation
KW  - degeneration
KW  - immune system
KW  - rasmussen encephalitis
Y1  - 2009
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-37330
ER  - 
TY  - THES
A1  - Raab, Viktoria Maria
T1  - Histologische Charakterisierung Vaccinia-Virus infizierter humaner Tumore im Mausmodell
T1  - Histological charaterization of Vaccinia-Virus infected human tumors in mice
N2  - Onkolytische Viren spielen eine immer bedeutendere Rolle für die Tumorforschung, weil in zahlreichen präklinischen Studien gezeigt werden konnte, dass viral bedingte Onkolyse zu einer Tumorregression führt. Ein äußerst vielversprechender Kandidat der onkolytischen Viren ist das Vaccinia-Virus. In der vorliegenden Arbeit wurde mit dem attenuierten Vaccinia-Virus GLV-1h68 gearbeitet, welches nach systemischer Applikation eine Regression von Tumoren verursacht. Obwohl bereits zahlreiche onkolytische Viren in klinischen Studien Anwendung finden, sind zugrunde liegende Abläufe bei einer Virusinfektion solider Tumore sowie Mechanismen, welche für die Tumorregression verantwortlich sind, immer noch nicht erschlossen. Um Aufschluss über notwendige Parameter für eine effiziente Infektion eines soliden Tumors mit GLV-1h68 zu erlangen, wurden im ersten Teil dieser Arbeit die uninfizierte Tumormikroumgebung sowie stromale Veränderungen in der frühe Phase der Infektion untersucht. Als Tumormodell diente hierbei ein humanes autologes Melanomzellpaar (888-MEL und 1936-MEL). Diese beiden Zelllinien sind Teil einer Reihe von fünf verschiedenen Melanomzelllinien, welche alle aus den widerkehrenden Metastasen eines einzelnen Patienten (Patient 888) isoliert wurden. 888-MEL zeigt nach Virusinfektion mit GLV-1h68 ein regredierendes Verhalten (therapeutischer Index: 88,0) und ist somit respondierend nach GLV-1h68-Infektion. 1936-MEL hingegen zeigte mit einem therapeutischen Index von 13,7 ein nur schwach verlangsamtes Wachstum solider Tumore, und ist somit schwach-respondierend nach GLV-1h68-Infektion. Als ein Grund, weshalb diese beiden autologen Melanomzelllinien unterschiedlich auf GLV-1h68-Infektion reagieren, wurde die Anzahl der Viruspartikel vermutet, welche 1 dpi im soliden Tumor vorliegt. Eine mögliche Korrelation zwischen initialem viralen Titer 1 dpi und späterer Tumorregression konnte experimentell aber nicht nachgewiesen werden. Zwei voneinander unabhängige Experimentreihen zeigten, dass bei identischer systemischer Applikation in den beiden soliden Tumoren kein Unterschied des viralen Titers vorlag. Weiterhin wurden die Komponenten der Tumormikroumgebung und ihr möglicher Einfluss auf die Effizienz der Virusinfektion untersucht. Immunhistologische Studien zeigten, dass es im uninfizierten Zustand bei soliden 888-MEL Tumoren zu einer massiven Infiltration CD45-positiver Zellen kam, die bei 1936-MEL-Tumoren jedoch nicht zu finden war. Die Beobachtung steht in Übereinstimmung mit Ergebnissen einer vergleichenden Microarray-Analyse, die das Infiltrat CD45-positiver Zellen in 888-MEL Tumoren genauer charakterisierte. Es wurde mit Microarray-Analyse eine erhöhte Expression chemotaktischer Moleküle in soliden 888-MEL Tumoren nachgewiesen. Unter anderem wird CCL8 (MCP-2) erhöht exprimiert. Als chemotaktisches Molekül hat CCL8 eine erhöhte Monozyteninfiltration zur Folge. Weiterhin wurde eine erhöhte Expression von MIF (macrophage migration inhibitory factor) und dem entsprechendem Rezeptor CD74 in uninfizierten 888-MEL-Tumoren gemessen. MIF induziert als proinflammatorisches Zytokin die Synthese inflammatorischer Mediatoren. Dies erklärt die Anhäufung CD45-positiver Zellen in der Tumormikroumgebung. Durch eine erhöhte Expression MHC II-verwandter Gene in soliden 888-MEL- Tumoren wurden die CD45-positiven Zellen als Monozyten identifiziert. Um die Funktion der Immunzellen zu analysieren, wurde durch eine intraperitoneale Applikation des Zytostatikums Cyclophosphamid eine Monozytendepletion induziert. Diese Immundepletion resultierte in soliden 888-MEL- Tumoren in einer signifikant verringerten Virusreplikation und -Ausbreitung nach Infektion mit GLV-1h68. Diese Ergebnisse implizieren, dass durch eine erhöhte Infiltration CD45-positiver Zellen in die Tumormikroumgebung die GLV-1h68-Infektion und -Replikation erleichtert wird. Nach Ausbreitung der Infektion kommt es in respondierenden Tumoren nach einem ersten Wachtumsarrest zu einer Tumorregression. Um Aufschluss über den beteiligten Mechanismus bei der Tumorregression zu erlangen, wurden GLV-1h68-infizierte-Tumore in der späten Phase der Infektion untersucht. Drei mögliche Mechanismen viral verursachter Onkolyse wurden beschrieben: Tumorzell-spezifische Onkolyse, Zerstörung der Tumorvaskulatur oder anti-tumorale Immunantwort. Für diese Experimente wurden humane Brustkarzinomzellen als Tumormodell verwendet. Mit diesem Tumormodell sollte analysiert werden, welcher der drei bislang diskutierten Mechanismen bei einer GLV-1h68-Infektion vorlag. Als erstes zeigten histologische Studien, dass Virusinfektion und -Replikation zu ausgedehnten Tumornekrosen führen. Dabei blieben die Blutgefäße in uninfizierten und auch in infizierten Bereichen des Tumors intakt und funktionell aktiv. Systemische Perfusion der Vaskulatur mit Lektin zeigte, dass die Tumorvaskulatur an das periphere Blutgefäßsystem angeschlossen war. Nachfolgende Experimente zeigten, dass Endothelzellen nicht durch die Viren infiziert wurden, wohingegen aber Endothelzell-ummantelnde, Gefäß-stabilisierende Perizyten nur in uninfizierten, nicht aber in infizierten Bereichen des Tumors vorkamen. Perizyten wurden möglicherweise durch Virusinfektion lysiert. Morphologische und funktionelle Analyse der Blutgefäße im Tumor zeigte, dass GLV-1h68-Infektion Hyperpermeabilität, Vasodilatation und eine erhöhte Expression des Adhäsionsmoleküls CD31 verursachte. Eine erhöhte CD31-Expression erleichtert eine Infiltration rekrutierter Immunzellen. Das konnte durch immunhistochemische Färbung von CD45 und MHC II besonders in intratumoralen Bereichen gezeigt werden. Durch Cyclophosphamid-vermittelte Immunsuppression wurde nachgewiesen, dass diese rekrutierten Immunzellen keinen ausschlaggebenden Einfluss auf die Tumorregression haben. Nach Immundepletion in soliden GI-101A-Tumoren konnte eine verstärkte Virusinfektion, effektivere Onkolyse und frühzeitigere Tumorregression nachgewiesen werden. Zusammenfassend zeigten diese Ergebnisse, dass der dominierende Mechanismus, welcher zur Tumorregression führt, die Onkolyse ist.
N2  - Preclinical application of oncolytic viruses to induce virus-mediated tumor rejection revealed promising results in the past few years. Vaccinia virus GLV-1h68, used in this study, was shown to induce complete tumor disappearance upon infection. However the exact underlying mechanisms of viral infection and virus-mediated tumor regression are still not well understood. This study describes the characterization of the early phase of a GLV-1h68 infection and the role of stromal components as well as the mechanisms involved in tumor regression. To address the question, which components are necessary for an effective GLV-1h68 infection, followed by successive rounds of viral replication, the first part of this study focused on the characterization of the early phase of Vaccinia virus infection in a human autologous melanoma system. Five different cell lines were previously generated from a melanoma patient experiencing several reoccurrences in a 12 year span. The melanoma cell line expanded from a metastasis at an early time point (888-MEL) retained responsiveness to GLV-1h68 treatment, while the subsequent cell line 1936-MEL (studied here), became non-responsive to the same treatment. To address the influence of the amount of viral particles homing to the tumor within initial 24 hpi, 888-MEL and 1936-MEL tumors were compared. It could clearly be demonstrated, that the initial homing of viral particles is not the reason for further effective viral replication and spreading. The comparative viral titers were measured in 888-MEL and 1936-MEL tumors 1 dpi and found similar. Immuno-histological comparison of xenografts generated with 888-MEL or 1936-MEL revealed a massive infiltration of CD45-positive cells in 888-MEL tumors, but not in 1936-MEL tumors. Comparative microarray analysis of uninfected 888-MEL and 1936-MEL solid tumors supported these findings. Beside a significant up-regulation of CCL8 in 888-MEL tumors, an increased expression of CD74/MIF suggests an increased monocyte infiltration in 888-MEL uninfected tumors, which is not apparent in 1936-MEL tumors. To gain better understanding of an immune cell infiltration into solid 888-MEL tumors, a monocyte depletion study using the immunosuppressive agent cyclophosphamide (CPA) was carried out. This treatment resulted in a highly significant reduction of viral replication and spreading in 888-MEL tumors following infection with GLV-1h68. These results demonstrated that the replication efficiency of GLV-1h68 is higher in 888-MEL xenografts compared to 1936-MEL. The enhanced replication is in direct correlation with a higher number of CD45-positive cells, which infiltrated the tumor site prior to virus injection. Through successive rounds of viral replication the virus can spread throughout the tumor and induces tumor regression. To gain insights into mechanisms involved in tumor regression, late stages of a GLV-1h68 infection were characterized in human breast tumor xenografts (GI-101A). Theoretically oncolytic virus therapy could be based on three different mechanisms: by tumor cell specific oncolysis, by destruction of the tumor vasculature or by an anti-tumoral immunological response. Here the contribution of the three factors was analyzed. Histological examination showed that viral infection of GI-101A tumors led to broad tumor necrosis. However, the tumor vasculature in infected tumor areas remained functional and endothelial cells were not infected neither in tumors nor in cultured cells. It was further demonstrated, that viral tumor colonization activated the tumor endothelium leading to vascular hyperpermeability, vessel dilatation and an increased expression of the adhesion molecule CD31, which in a next step facilitated infiltration of inflammatory cell. This could be visualized by immunohistochemical staining of MHCII- and CD45-positive cells. The stainings revealed increased intratumoral infiltration of immune cells within infected tumor xenografts. The recruited immune cells however, do not seem to be causative for the tumorregression, since immunosuppression of GLV-1h68-infected animals led to increased viral replication and broader distribution in the tumor tissue, resulting in more efficient oncolysis and earlier start of the tumor regression phase. In summary, these results indicate that GLV-1h68 mediated oncolysis is the primary mechanism of tumor regression. Therefore, enhancing the viral replication and distribution within the tumor microenvironment should lead to improved therapeutic results in preclinical studies and clinical applications.
KW  - Vaccinia-Virus
KW  - Leukozyt
KW  - Allgemeine Entzündungsreaktion
KW  - Immunstimulation
KW  - Immunsuppression
KW  - Vaccinia-Virus
KW  - inflammation
KW  - leukocyte
KW  - innate immunity
Y1  - 2010
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-49024
ER  - 
TY  - THES
A1  - Grimm, Martin
T1  - Die Bedeutung der Expression des Tumornekrosefaktor-alpha bei Patienten mit kolorektalem Karzinom
T1  - Tumor Necrosis Factor-α expression in patients with colorectal cancer
N2  - Für Tumorprogression müssen entartete Zellen Wege finden, die immunologische Abwehr und die Apoptose zu umgehen. Tumorzellen haben dafür verschiedene, sogenannte Tumor-Escape-Mechanismen entwickelt. Gegenstand dieser Arbeit war in diesem Zusammenhang die Untersuchung des TNF-α-TNF-R1-Systems. Eine signifikante erhöhte TNF-α Protein- und Genexpression konnte in Gewebeproben kolorektaler Karzinome nachgewiesen werden, wobei eine mäßig starke Korrelation beider Analysemethoden ersichtlich war (т = 0.794). Sowohl die immunhistochemische Analyse als auch die Genexpression durch RT-PCR konnten mit Tumorprogression assoziiert werden. Mit erhöhter Expression des Apoptose-induzierenden Zytokins TNF-α durch Tumorzellen konnte darüber hinaus ein signifikant schlechteres Gesamtüberleben der Patienten mit KRK beobachtet werden. In unmittelbarer Umgebung TNF-α exprimierender Tumorzellen wurden zahlreiche TNF-R1+/CD8+ Zellen analysiert, die als Hinweis auf Apoptose in TILs angesehen werden können. Dieser Weg könnte als Tumor-Escape-Mechanismus verstanden werden. Die Verwendung potentieller TNF-α Biologicals (z.B. Etanercept, Infliximab) bleibt jedoch unter dem Aspekt einer geringfügig erhöhten Lymphominzidenz gegenüber der Normalbevölkerung auch als kritisch zu bewerten. Der Einsatz von Anti-TNF-α-Therapien stellt jedoch eine vielversprechende Option bei Patienten mit metastasiertem KRK und Tumorrezidiv dar. Zusammenfassend liefern die Ergebnisse dieser Arbeit zusätzlichen Einblick in die Regulationsmechanismen, die verantwortlich für die Immunsuppression durch kolorektale Karzinome sein können. Diese basiswissenschaftlichen Erkenntnisse stellen eine mögliche Grundlage neuer Behandlungsmöglichkeiten kolorektaler Karzinomen dar, die weiter erforscht werden sollten.
N2  - The progressive growth of malignancies is accompanied by a decline in the immune response through mechanisms which are poorly understood. Apoptosis and induction of inflammation by tumor released cytokines as tumor escape mechanisms have been proposed to play an important role in colorectal carcinogenesis. Expression of Tumor necrosis factor-alpha (TNF-α) was analyzed in colorectal cancer specimen by immunohistochemistry and RT-PCR. TNF-α expression on protein and mRNA level were correlated with clinical characteristics and impact on survival. TNFR-1 was co-labelled with TNF-α and CD8+ cytotoxic T cells in immunofluorescence double staining experiments. 94% of the patients with CRC expressed TNF-α. High TNF-α expression was significantly associated with positive lymph node stage and recurrence of the tumor. Multivariate analysis revealed high TNF-α expression as an independent prognostic factor. Immunohistochemistry was correlated with RT-PCR results (т = 0.794). Immunofluorescence double staining experiments revealed increased TNFR-1 expression by CD8+ cells. TNF-α expression by tumor cells may be an efficient immunological escape mechanism by inflammation-enhanced metastases and probably by induction of apoptosis in tumor-infiltrating CD8+ immune cells resulting in a down regulation of the tumoral immune response. Our data support the role of tumor-derived TNF-α expression as an important promoter of tumoral immune escape mechanisms and malignant progression. Targeting TNF-α (e.g. Etanercept, Infliximab) may be a promising option, especially in cases with high TNF-α expression and positive lymph node metastases.
KW  - Cancer
KW  - Tumor escape mechanism
KW  - death receptor signalling
KW  - apoptosis
KW  - inflammation
KW  - colorectal carcinoma
Y1  - 2010
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-52757
ER  - 
TY  - THES
A1  - Rodenberg, Hella Katharina
T1  - Inflammation und Mangelernährung bei Dialysepatienten mit Diabetes Mellitus Typ 2
T1  - Inflammation and malnutrition in patients with type 2 diabtes mellitus on hemodialysis
N2  - In der vorliegenden Arbeit wird der Einfluss von hs-CRP und Albumin auf die kardiovaskuläre Ereignisrate und das Überleben von Patienten mit Diabetes Mellitus Typ 2 an der Hämodialyse untersucht. Grundlagen für die hier dargestellte Auswertung sind die in der 4D Studie erhobenen Daten. Die 4D Studie hat prospektiv, randomisiert, doppelblind und placebo-kontrolliert untersucht, ob die Behandlung mit Atorvastatin bei Patienten mit Diabetes Mellitus Typ 2 an der Hämodialyse den primären Endpunkt bestehend aus Herzinfarkt, kardialem Tod und Schlaganfall zu senken vermag. Die Daten zum hs-CRP und Albumin wurden bei Studienbeginn und nach sechs Monaten erhoben. In einer post-hoc Analyse mit Hilfe eines multivariaten Cox Regressionsmodels konnte bestätigt werden, dass ein erhöhter Spiegel an hs-CRP und ein verminderter Spiegel an Albumin im Zusammenhang mit einer vermehrten kardiovaskulären Ereignisrate und Mortalität stehen. Eine Behandlung mit Atorvastatin führte zwar nicht zu einer Risikosenkung für den primären Endpunkt oder die Mortalität, hatte aber einen stabilisierenden Effekt auf des hs-CRP Spiegel.
N2  - In this dissertation the influence of high sensitive (hs)-CRP and Albumin on cardiovascular (cv) events and mortality in patients with type 2 diabetes mellitus on hemodialysis is determined. Based on the data of the „4D“ (Die Deutsche Dialyse Diabetes) Study a prospective, double-blind, placebo controlled study a post-hoc analysis was accomplished. The data of hs-CRP and Albumin were aroused at baseline and six month later. Via multivariate cox-regressions analysis it could be considered that elevated hs-CRP and reduced Albumin are associated with an increased risk for cv events and mortality. A treatment with Atorvastatin indeed didn’t neither reduce the risk for cv events nor the risk for mortality but had a stabilizing effect on hs-CRP level.
KW  - Hämodialyse
KW  - Mangelernährung
KW  - Proteinmangel
KW  - Inflammation
KW  - hs-CRP
KW  - Albumin
KW  - inflammation
KW  - malnutrition
KW  - hemodialysis
KW  - hs-CRP
KW  - albumin
Y1  - 2011
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-71145
ER  - 
TY  - THES
A1  - Rauh, Katharina
T1  - Erythropoietin und Inflammation bei diabetischer Nephropathie
T1  - Erythropoietin and Inflammation in Diabetic Chronic Kidney Disease
N2  - Bei Patienten mit Diabetes mellitus Typ 2 und chronischer Niereninsuffizienz ist Anämie häufig. Zum Teil ist sie durch ungenügende EPO-Produktion bedingt. Zusätzlich wird die Hämoglobinsynthese, wie bei der Anämie chronischer Krankheiten (anemia of chronic disease, ACD) beschrieben, durch entzündliche Vorgänge unterdrückt. Der Stellenwert endogenen Erythropoietins bei Patienten mit diabetischer Nephropathie und ACD bleibt noch unsicher sowie auch der Zusammenhang zwischen EPO und der Nierenfunktion. Diese Querschnittsanalyse schloss 224 Patienten mit Typ 2-Diabetes in allen Stadien chronischer Niereninsuffizienz (CNI-Stadium 1-5) ein. Das mediane Alter betrug 67 Jahre, 54 % waren männlich und die mediane GFR lag bei 49 ml/min. Gemäß den Definitionen der K/DOQI-Richtlinien waren 41 % der Patienten anämisch. Von der Studie ausgeschlossen wurden wegen der Anämie behandelte Patienten und solche mit Eisenmangel. Prädiktoren der log-transformierten EPO-Spiegel wurden unter Benutzung multivariater linearer Regressionsmodelle ausgewertet. Die univariate und inverse Beziehung zwischen GFR und EPO-Spiegeln (p = 0,009) wurde in der multivariaten Analyse nicht-signifikant. Erhöhtes CRP (p < 0,001), niedriges Ferritin (p = 0,002), kardiovaskuläre Ereignisse in der Vorgeschichte (p = 0,02) und Hypertension (p = 0,04) waren nach Adjustierung für Alter, Geschlecht, Hb, GFR und andere klinische Faktoren unabhängig mit erhöhten EPO-Spiegeln assoziiert. In der untersuchten Population fand sich kein Zusammenhang zwischen EPO-Spiegeln und Hämoglobin. Bei diabetischen Patienten mit chronischer Niereninsuffizienz werden die EPO-Spiegel trotz gleichzeitig niedriger Hämoglobinspiegel vor allem durch Entzündungsparameter und den Eisenstatus vorhergesagt und sind dabei unabhängig von der Nierenfunktion. Deshalb könnte die Anämie bei Patienten mit diabetischer Nephropathie hauptsächlich durch Inflammation entstehen, die zu einem relativen Eisenmangel und einer Resistenz des Knochenmarks gegenüber endogenem EPO führt.
N2  - BACKGROUND: Anemia is prevalent in patients with type 2 diabetes mellitus (DM) and chronic kidney disease (CKD) and is caused in part by insufficient erythropoietin (EPO) production. In addition, inflammatory processes also suppress hemoglobin synthesis as described in anemia of chronic diseases (ACD). The role of endogenous EPO in diabetic CKD and in ACD and its relationship to kidney function remain uncertain. METHODS: This cross-sectional analysis included 224 diabetic patients with CKD stages 1 to 5 (median age 67 yrs, 54% male, median GFR 49 ml/min). Anemia was defined as per K/DOQI guidelines and was prevalent in 41% of the patients. Patients treated for anemia and iron deficient patients were excluded. Predictors of log-transformed EPO-levels were evaluated using multivariate linear regression modeling. RESULTS: The univariate and inverse relationship between GFR and EPO-level (p = 0.009) became non-significant in multivariate analyses. Elevated C-reactive protein (p < 0.001), low ferritin (p = 0.002) , history of CVD (p = 0.02) and hypertension (p = 0.04) were independently associated with elevated EPO-level, after adjusting for age, gender, hemoglobin, GFR, and other clinical factors. Hemoglobin was not associated with EPO-level in this population. CONCLUSIONS: In diabetic patients with CKD, elevated EPO-levels were predicted mainly by inflammatory markers and iron status, despite low hemoglobin levels and independent of kidney function. Therefore, anemia in diabetic CKD could be explained in part by inflammation-mediated iron dysregulation and resistance to endogenous EPO.
KW  - Diabetes mellitus
KW  - Anämie
KW  - Erythropoietin
KW  - Chronische Niereninsuffizienz
KW  - Entzündung
KW  - Inflammation
KW  - anemia
KW  - diabetes mellitus
KW  - chronic kidney disease
KW  - erythropoietin
KW  - inflammation
Y1  - 2011
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-66637
ER  - 
TY  - JOUR
A1  - Zanucco, Emanuele
A1  - Götz, Rudolf
A1  - Potapenko, Tamara
A1  - Carraretto, Irene
A1  - Ceteci, Semra
A1  - Ceteci, Fatih
A1  - Seeger, Werner
A1  - Savai, Rajkumar
A1  - Rapp, Ulf R.
T1  - Expression of B-RAF V600E in Type II Pneumocytes Causes Abnormalities in Alveolar Formation, Airspace Enlargement and Tumor Formation in Mice
JF  - PLOS ONE
N2  - Growth factor induced signaling cascades are key regulatory elements in tissue development, maintenance and regeneration. Perturbations of these cascades have severe consequences, leading to developmental disorders and neoplastic diseases. As a major function in signal transduction, activating mutations in RAF family kinases are the cause of human tumorigenesis, where B-RAF V600E has been identified as the prevalent mutant. In order to address the oncogenic function of B-RAF V600E, we have generated transgenic mice expressing the activated oncogene specifically in lung alveolar epithelial type II cells. Constitutive expression of B-RAF V600E caused abnormalities in alveolar epithelium formation that led to airspace enlargements. These lung lesions showed signs of tissue remodeling and were often associated with chronic inflammation and low incidence of lung tumors. The inflammatory cell infiltration did not precede the formation of the lung lesions but was rather accompanied with late tumor development. These data support a model where the continuous regenerative process initiated by oncogenic B-RAF-driven alveolar disruption provides a tumor-promoting environment associated with chronic inflammation.
KW  - obstructive pulmonary-disease
KW  - lung-cancer
KW  - somatic mutations
KW  - epithelial-cells
KW  - mouse models
KW  - protein
KW  - kinase
KW  - inflammation
KW  - activation
KW  - pathway
Y1  - 2011
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-137061
VL  - 6
IS  - 12
ER  - 
TY  - JOUR
A1  - Baune, Bernhard T.
A1  - Konrad, Carsten
A1  - Grotegerd, Dominik
A1  - Suslow, Thomas
A1  - Birosova, Eva
A1  - Ohrmann, Patricia
A1  - Bauer, Jochen
A1  - Arolt, Volker
A1  - Heindel, Walter
A1  - Domschke, Katharina
A1  - Schöning, Sonja
A1  - Rauch, Astrid V.
A1  - Uhlmann, Christina
A1  - Kugel, Harald
A1  - Dannlowski, Udo
T1  - Interleukin-6 gene (IL-6): a possible role in brain morphology in the healthy adult brain
JF  - Journal of Neuroinflammation
N2  - Background: Cytokines such as interleukin 6 (IL-6) have been implicated in dual functions in neuropsychiatric disorders. Little is known about the genetic predisposition to neurodegenerative and neuroproliferative properties of cytokine genes. In this study the potential dual role of several IL-6 polymorphisms in brain morphology is investigated. 
Methodology: In a large sample of healthy individuals (N = 303), associations between genetic variants of IL-6 (rs1800795; rs1800796, rs2069833, rs2069840) and brain volume (gray matter volume) were analyzed using voxel-based morphometry (VBM). Selection of single nucleotide polymorphisms (SNPs) followed a tagging SNP approach (e. g., Stampa algorigthm), yielding a capture 97.08% of the variation in the IL-6 gene using four tagging SNPs. Principal findings/results In a whole-brain analysis, the polymorphism rs1800795 (-174 C/G) showed a strong main effect of genotype (43 CC vs. 150 CG vs. 100 GG; x = 24, y = -10, z = -15; F(2,286) = 8.54, p(uncorrected) = 0.0002; p(AlphaSim-corrected) = 0.002; cluster size k = 577) within the right hippocampus head. Homozygous carriers of the G-allele had significantly larger hippocampus gray matter volumes compared to heterozygous subjects. None of the other investigated SNPs showed a significant association with grey matter volume in whole-brain analyses. 
Conclusions/significance: These findings suggest a possible neuroprotective role of the G-allele of the SNP rs1800795 on hippocampal volumes. Studies on the role of this SNP in psychiatric populations and especially in those with an affected hippocampus (e.g., by maltreatment, stress) are warranted.
KW  - aging brain
KW  - hippocampal neurogenesis
KW  - cholinergic neurons
KW  - neurothrophic factor
KW  - Alzheimers disease
KW  - neurite outgrowth
KW  - inflammatory cytokines
KW  - major depression
KW  - nervour system
KW  - dentate gyrus
KW  - genetics
KW  - inflammation
KW  - interleukin 6
KW  - neuroprotection
KW  - voxel-based morphometry
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130804
VL  - 9
IS  - 125
ER  - 
TY  - JOUR
A1  - Willems, Coen H. M. P.
A1  - Urlichs, Florian
A1  - Seidenspinner, Silvia
A1  - Kunzmann, Steffen
A1  - Speer, Christian P.
A1  - Kramer, Boris W.
T1  - Poractant alfa (Curosurf (R)) increases phagocytosis of apoptotic neutrophils by alveolar macrophages in vivo
JF  - Respiratory Research
N2  - Background: Clearance of apoptotic neutrophils in the lung is an essential process to limit inflammation, since they could become a pro-inflammatory stimulus themselves. The clearance is partially mediated by alveolar macrophages, which phagocytose these apoptotic cells. The phagocytosis of apoptotic immune cells by monocytes in vitro has been shown to be augmented by several constituents of pulmonary surfactant, e. g. phospholipids and hydrophobic surfactant proteins. In this study, we assessed the influence of exogenous poractant alfa (Curosurf (R)) instillation on the in vivo phagocytosis of apoptotic neutrophils by alveolar macrophages. 
Methods: Poractant alfa (200 mg/kg) was instilled intratracheally in the lungs of three months old adult male C57/Black 6 mice, followed by apoptotic neutrophil instillation. Bronchoalveloar lavage was performed and alveolar macrophages and neutrophils were counted. Phagocytosis of apoptotic neutrophils was quantified by determining the number of apoptotic neutrophils per alveolar macrophages. 
Results: Exogenous surfactant increased the number of alveolar macrophages engulfing apoptotic neutrophils 2.6 fold. The phagocytosis of apoptotic neutrophils was increased in the presence of exogenous surfactant by a 4.7 fold increase in phagocytosed apoptotic neutrophils per alveolar macrophage. 
Conclusions: We conclude that the anti-inflammatory properties of surfactant therapy may be mediated in part by increased numbers of alveolar macrophages and increased phagocytosis of apoptotic neutrophils by alveolar macrophages.
KW  - preterm
KW  - surfactant protein-A
KW  - respiratory-distress-syndrome
KW  - synthetic surfactant
KW  - human monocytes
KW  - SIRP-alpha
KW  - lung
KW  - cells
KW  - inflammation
KW  - resolution
KW  - anti inflammation
KW  - drug therapy
KW  - surfactant
Y1  - 2012
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130721
VL  - 13
IS  - 17
ER  - 
TY  - JOUR
A1  - Hedrich, Christian M.
A1  - Hofmann, Sigrun R.
A1  - Pablik, Jessica
A1  - Morbach, Henner
A1  - Girschick, Hermann J.
T1  - Autoinflammatory bone disorders with special focus on chronic recurrent multifocal osteomyelitis (CRMO)
JF  - Pediatric Rheumatology
N2  - Sterile bone inflammation is the hallmark of autoinflammatory bone disorders, including chronic nonbacterial osteomyelitis (CNO) with its most severe form chronic recurrent multifocal osteomyelitis (CRMO). Autoinflammatory osteopathies are the result of a dysregulated innate immune system, resulting in immune cell infiltration of the bone and subsequent osteoclast differentiation and activation. Interestingly, autoinflammatory bone disorders are associated with inflammation of the skin and/or the intestine. In several monogenic autoinflammatory bone disorders mutations in disease-causing genes have been reported. However, regardless of recent developments, the molecular pathogenesis of CNO/CRMO remains unclear. Here, we discuss the clinical presentation and molecular pathophysiology of human autoinflammatory osteopathies and animal models with special focus on CNO/CRMO. Treatment options in monogenic autoinflammatory bone disorders and CRMO will be illustrated.
KW  - bisphosphonate treatment
KW  - IL-10 expression
KW  - TNF-α
KW  - IL-10
KW  - inflammation
KW  - bone
KW  - CRMO
KW  - CNO
KW  - DIRA
KW  - PAPA
KW  - Majeed-Syndrome
KW  - disease
KW  - deficiency
KW  - pediatric patients
KW  - treatment
KW  - TLR4
KW  - PAPA syndrome
KW  - hypertrophic osteodystrophy
KW  - chronic nonbacterial osteomyelitis
KW  - congenital dyserythropoietic anemia
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125694
SN  - 1546-0096
VL  - 11
IS  - 47
ER  - 
TY  - JOUR
A1  - Blömer, Nadja
A1  - Pachel, Christina
A1  - Hofmann, Urlich
A1  - Nordbeck, Peter
A1  - Bauer, Wolfgang
A1  - Mathes, Denise
A1  - Frey, Anna
A1  - Bayer, Barbara
A1  - Vogel, Benjamin
A1  - Ertl, Georg
T1  - 5-Lipoxygenase facilitates healing after myocardial infarction
JF  - Basic Research in Cardiology
N2  - Early healing after myocardial infarction (MI) is characterized by a strong inflammatory reaction. Most leukotrienes are pro-inflammatory and are therefore potential mediators of healing and remodeling after myocardial ischemia. The enzyme 5-lipoxygenase (5-LOX) has a key role in the transformation of arachidonic acid in leukotrienes. Thus, we tested the effect of 5-LOX on healing after MI. After chronic coronary artery ligation, early mortality was significantly increased in 5-LOX\(^{−/−}\) when compared to matching wildtype (WT) mice due to left ventricular rupture. This effect could be reproduced in mice treated with the 5-LOX inhibitor Zileuton. A perfusion mismatch due to the vasoactive potential of leukotrienes is not responsible for left ventricular rupture since local blood flow assessed by magnetic resonance perfusion measurements was not different. However, after MI, there was an accentuation of the inflammatory reaction with an increase of pro-inflammatory macrophages. Yet, mortality was not changed in chimeric mice (WT vs. 5-LOX\(^{−/−}\) bone marrow in 5-LOX\(^{−/−}\) animals), indicating that an altered function of 5-LOX\(^{−/−}\) inflammatory cells is not responsible for the phenotype. Collagen production and accumulation of fibroblasts were significantly reduced in 5-LOX\(^{−/−}\) mice in vivo after MI. This might be due to an impaired migration of 5-LOX\(^{−/−}\) fibroblasts, as shown in vitro to serum. In conclusion, a lack or inhibition of 5-LOX increases mortality after MI because of healing defects. This is not mediated by a change in local blood flow, but through an altered inflammation and/or fibroblast function.
KW  - lipoxygenase
KW  - myocardial infarction
KW  - extracellular matrix remodeling
KW  - inflammation
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132602
VL  - 108
IS  - 4
ER  - 
TY  - JOUR
A1  - Hedrich, Christian M.
A1  - Hofmann, Sigrun R.
A1  - Pablik, Jessica
A1  - Morbach, Henner
A1  - Girschick, Hermann J.
T1  - Autoinflammatory bone disorders with special focus on chronic recurrent multifocal osteomyelitis (CRMO)
JF  - Pediatric Rheumatology
N2  - Sterile bone inflammation is the hallmark of autoinflammatory bone disorders, including chronic nonbacterial osteomyelitis (CNO) with its most severe form chronic recurrent multifocal osteomyelitis (CRMO). Autoinflammatory osteopathies are the result of a dysregulated innate immune system, resulting in immune cell infiltration of the bone and subsequent osteoclast differentiation and activation. Interestingly, autoinflammatory bone disorders are associated with inflammation of the skin and/or the intestine. In several monogenic autoinflammatory bone disorders mutations in disease-causing genes have been reported. However, regardless of recent developments, the molecular pathogenesis of CNO/CRMO remains unclear.

Here, we discuss the clinical presentation and molecular pathophysiology of human autoinflammatory osteopathies and animal models with special focus on CNO/CRMO. Treatment options in monogenic autoinflammatory bone disorders and CRMO will be illustrated.
KW  - TNF-α
KW  - PAPA
KW  - DIRA
KW  - Majeed
KW  - CNO
KW  - CRMO
KW  - bone
KW  - inflammation
KW  - IL-10
KW  - treatment
KW  - TLR4
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-132456
VL  - 11
IS  - 47
ER  - 
TY  - JOUR
A1  - Weibel, Stephanie
A1  - Basse-Luesebrink, Thomas Christian
A1  - Hess, Michael
A1  - Hofmann, Elisabeth
A1  - Seubert, Carolin
A1  - Langbein-Laugwitz, Johanna
A1  - Gentschev, Ivaylo
A1  - Sturm, Volker Jörg Friedrich
A1  - Ye, Yuxiang
A1  - Kampf, Thomas
A1  - Jakob, Peter Michael
A1  - Szalay, Aladar A.
T1  - Imaging of Intratumoral Inflammation during Oncolytic Virotherapy of Tumors by \(^{19}\)F-Magnetic Resonance Imaging (MRI)
JF  - PLoS ONE
N2  - Background
Oncolytic virotherapy of tumors is an up-coming, promising therapeutic modality of cancer therapy. Unfortunately, non-invasive techniques to evaluate the inflammatory host response to treatment are rare. Here, we evaluate \(^{19}\)F magnetic resonance imaging (MRI) which enables the non-invasive visualization of inflammatory processes in pathological conditions by the use of perfluorocarbon nanoemulsions (PFC) for monitoring of oncolytic virotherapy.

Methodology/Principal Findings
The Vaccinia virus strain GLV-1h68 was used as an oncolytic agent for the treatment of different tumor models. Systemic application of PFC emulsions followed by \(^1H\)/\(^{19}\)F MRI of mock-infected and GLV-1h68-infected tumor-bearing mice revealed a significant accumulation of the \(^{19}\)F signal in the tumor rim of virus-treated mice. Histological examination of tumors confirmed a similar spatial distribution of the \(^{19}\)F signal hot spots and \(CD68^+\)-macrophages. Thereby, the \(CD68^+\)-macrophages encapsulate the GFP-positive viral infection foci. In multiple tumor models, we specifically visualized early inflammatory cell recruitment in Vaccinia virus colonized tumors. Furthermore, we documented that the \(^{19}\)F signal correlated with the extent of viral spreading within tumors.

Conclusions/Significance
These results suggest \(^{19}\)F MRI as a non-invasive methodology to document the tumor-associated host immune response as well as the extent of intratumoral viral replication. Thus, \(^{19}\)F MRI represents a new platform to non-invasively investigate the role of the host immune response for therapeutic outcome of oncolytic virotherapy and individual patient response.
KW  - inflammation
KW  - fluorescence microscopy
KW  - oncolytic viruses
KW  - fluorescence imaging
KW  - macrophages
KW  - magnetic resonance imaging
KW  - histology
KW  - in vivo imaging
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-130311
VL  - 8
IS  - 3
ER  - 
TY  - JOUR
A1  - Wolf, Annette
A1  - Akrap, Nina
A1  - Marg, Berenice
A1  - Galliardt, Helena
A1  - Heiligentag, Martyna
A1  - Humpert, Fabian
A1  - Sauer, Markus
A1  - Kaltschmidt, Barbara
A1  - Kaltschmidt, Christian
A1  - Seidel, Thorsten
T1  - Elements of Transcriptional Machinery Are Compatible among Plants and Mammals
JF  - PLoS ONE
N2  - In the present work, the objective has been to analyse the compatibility of plant and human transcriptional machinery. The experiments revealed that nuclear import and export are conserved among plants and mammals. Further it has been shown that transactivation of a human promoter occurs by human transcription factor NF-\(\kappa\) B in plant cells, demonstrating that the transcriptional machinery is highly conserved in both kingdoms. Functionality was also seen for regulatory elements of NF-\(\kappa\) B such as its inhibitor I\(\kappa\)B isoform \(\alpha\) that negatively regulated the transactivation activity of the p50/RelA heterodimer by interaction with NF-\(\kappa\)B in plant cells. Nuclear export of RelA could be demonstrated by FRAP-measurements so that RelA shows nucleo-cytoplasmic shuttling as reported for RelA in mammalian cells. The data reveals the high level of compatibility of human transcriptional elements with the plant transcriptional machinery. Thus, Arabidopsis thaliana mesophyll protoplasts might provide a new heterologous expression system for the investigation of the human NF-\(\kappa\)B signaling pathways. The system successfully enabled the controlled manipulation of NF-\(\kappa\)B activity. We suggest the plant protoplast system as a tool for reconstitution and analyses of mammalian pathways and for direct observation of responses to e. g. pharmaceuticals. The major advantage of the system is the absence of interference with endogenous factors that affect and crosstalk with the pathway.
KW  - complexes
KW  - in vivo
KW  - DNA-binding
KW  - nuclear proe
KW  - gene expression
KW  - NF-KAPPA-B
KW  - RNA-binding protein
KW  - alpha
KW  - inflammation
KW  - homodimers
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-131203
VL  - 8
IS  - 1
ER  - 
TY  - JOUR
A1  - Pachel, Christina
A1  - Mathes, Denise
A1  - Bayer, Barbara
A1  - Dienesch, Charlotte
A1  - Wangorsch, Gaby
A1  - Heitzmann, Wolfram
A1  - Lang, Isabell
A1  - Ardehali, Hossein
A1  - Ertl, Georg
A1  - Dandekar, Thomas
A1  - Wajant, Harald
A1  - Frantz, Stefan
T1  - Exogenous Administration of a Recombinant Variant of TWEAK Impairs Healing after Myocardial Infarction by Aggravation of Inflammation
JF  - PLoS ONE
N2  - Background: Tumor necrosis factor-like weak inducer of apoptosis (TWEAK) and its receptor fibroblast growth factorinducible 14 (Fn14) are upregulated after myocardial infarction (MI) in both humans and mice. They modulate inflammation and the extracellular matrix, and could therefore be important for healing and remodeling after MI. However, the function of TWEAK after MI remains poorly defined.
Methods and results: Following ligation of the left coronary artery, mice were injected twice per week with a recombinant human serum albumin conjugated variant of TWEAK (HSA-Flag-TWEAK), mimicking the activity of soluble TWEAK. Treatment with HSA-Flag-TWEAK resulted in significantly increased mortality in comparison to the placebo group due to myocardial rupture. Infarct size, extracellular matrix remodeling, and apoptosis rates were not different after MI. However, HSA-Flag-TWEAK treatment increased infiltration of proinflammatory cells into the myocardium. Accordingly, depletion of neutrophils prevented cardiac ruptures without modulating all-cause mortality.
Conclusion: Treatment of mice with HSA-Flag-TWEAK induces myocardial healing defects after experimental MI. This is mediated by an exaggerated neutrophil infiltration into the myocardium.
KW  - apoptosis
KW  - myocardial infarction
KW  - neutrophils
KW  - cytokines
KW  - inflammation
KW  - myocardium
KW  - heart
KW  - extracellular matrix
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-129889
VL  - 8
IS  - 11
ER  - 
TY  - JOUR
A1  - Rittner, Heike Lydia
A1  - Hackel, Dagmar
A1  - Pflücke, Diana
A1  - Neumann, Annick
A1  - Viebahn, Johannes
A1  - Mousa, Shaaban
A1  - Wischmeyer, Erhard
A1  - Roewer, Norbert
A1  - Brack, Alexander
T1  - The Connection of Monocytes and Reactive Oxygen Species in Pain
JF  - PLoS ONE
N2  - The interplay of specific leukocyte subpopulations, resident cells and proalgesic mediators results in pain in inflammation. Proalgesic mediators like reactive oxygen species (ROS) and downstream products elicit pain by stimulation of transient receptor potential (TRP) channels. The contribution of leukocyte subpopulations however is less clear. Local injection of neutrophilic chemokines elicits neutrophil recruitment but no hyperalgesia in rats. In meta-analyses the monocytic chemoattractant, CCL2 (monocyte chemoattractant protein-1; MCP-1), was identified as an important factor in the pathophysiology of human and animal pain. In this study, intraplantar injection of CCL2 elicited thermal and mechanical pain in Wistar but not in Dark Agouti (DA) rats, which lack p47phox, a part of the NADPH oxidase complex. Inflammatory hyperalgesia after complete Freund's adjuvant (CFA) as well as capsaicin-induced hyperalgesia and capsaicin-induced current flow in dorsal root ganglion neurons in DA were comparable to Wistar rats. Macrophages from DA expressed lower levels of CCR2 and thereby migrated less towards CCL2 and formed limited amounts of ROS in vitro and 4-hydroxynonenal (4-HNE) in the tissue in response to CCL2 compared to Wistar rats. Local adoptive transfer of peritoneal macrophages from Wistar but not from DA rats reconstituted CCL2-triggered hyperalgesia in leukocyte-depleted DA and Wistar rats. A pharmacological stimulator of ROS production (phytol) restored CCL2-induced hyperalgesia in vivo in DA rats. In Wistar rats, CCL2-induced hyperalgesia was completely blocked by superoxide dismutase (SOD), catalase or tempol. Likewise, inhibition of NADPH oxidase by apocynin reduced CCL2-elicited hyperalgesia but not CFA-induced inflammatory hyperalgesia. In summary, we provide a link between CCL2, CCR2 expression on macrophages, NADPH oxidase, ROS and the development CCL2-triggered hyperalgesia, which is different from CFA-induced hyperalgesia. The study further supports the impact of CCL2 and ROS as potential targets in pain therapy.
KW  - analysis of variance
KW  - chemokines
KW  - hyperalgesia
KW  - inflammation
KW  - macrophages
KW  - monocytes
KW  - white blood cells
KW  - wistar rats
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-96669
ER  - 
TY  - THES
A1  - Partheil, Anna
T1  - Monozyten und Prostaglandine in der Schmerzentstehung
T1  - Monocytes and prostaglandins in the development of inflammatory pain
N2  - Schmerz ist eine klassische Komponente von Entzündungsreaktionen. Im Rahmen des Entzündungsgeschehens werden Zytokine und Chemokine freigesetzt, die Leukozyten zum Entzündungsort rekrutieren.  Über die Freisetzung weiterer proalgetischer Mediatoren tragen diese zur Aktivierung und Sensitivierung von Nozizeptoren und damit zur Schmerzentstehung bei. Das Monozyten-rekrutierende Chemokin CCL2 verursachte in Verhaltensexperimenten eine Hyperalgesie bei Ratten. Die Hyperalgesie war durch den Cox-2 Inhibitor Parecoxib vollständig reversibel. Daher wurde in dieser Arbeit  die Rolle von Monozyten und Prostaglandinen in der Entstehung dieser Hyperalgesie untersucht. Dazu wurde in vitro die Cox-2 Expression und die Prostaglandin-Bildung in humanen Monozyten und Peritonealmakrophagen der Ratte nach CCL2 Stimulation bestimmt. Zudem wurde in vivo die Cox-2 Expression im Rückenmark und in der Rattenpfote nach CCL2 Injektion in die Pfote untersucht.
N2  - One of the main components of inflammation is pain. In inflammation cytokines and chemokines are secreted and recruit leukocytes to the site of inflammation. Leukocytes release proalgesic mediators that activate and sensitize nociceptors and cause pain. Behavioral tests showed that the chemokine CCL2 (monocyte recruiting protein 2) causes hyperalgesia in rats. This hyperalgesia was blocked by parecoxib, a Cox-2 inhibitor. To further investigate the role of monocytes and prostaglandins in the development of hyperalgesia, Cox-2 expression and prostaglandin production were determined in vitro after stimulation of human monocytes and rat peritoneal macrophages with CCL2. In vivo, Cox-2 expression in spinal cord and paw tissue of rats was examined after injection of CCL2 into the paw.
KW  - Schmerz
KW  - CCL2
KW  - pain
KW  - Entzündung
KW  - Monozyten
KW  - Prostaglandine
KW  - inflammation
KW  - monocytes
KW  - prostaglandins
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-85091
ER  - 
TY  - JOUR
A1  - Schupp, Nicole
A1  - Ali, Badreldin H.
A1  - Beegam, Sumyia
A1  - Al-Husseni, Isehaq
A1  - Al-Shukaili, Ahmed
A1  - Nemmar, Abderrahim
A1  - Schierling, Simone
A1  - Queisser, Nina
T1  - Effect of gum arabic on oxidative stress and inflammation in adenine-induced chronic renal failure in rats
JF  - PLoS One
N2  - Inflammation and oxidative stress are known to be involved in the pathogenesis of chronic kidney disease in humans, and in chronic renal failure (CRF) in rats. The aim of this work was to study the role of inflammation and oxidative stress in adenine-induced CRF and the effect thereon of the purported nephroprotective agent gum arabic (GA). Rats were divided into four groups and treated for 4 weeks as follows: control, adenine in feed (0.75%, w/w), GA in drinking water (15%, w/v) and adenine+GA, as before. Urine, blood and kidneys were collected from the rats at the end of the treatment for analysis of conventional renal function tests (plasma creatinine and urea concentration). In addition, the concentrations of the pro-inflammatory cytokine TNF-a and the oxidative stress markers glutathione and superoxide dismutase, renal apoptosis, superoxide formation and DNA double strand break frequency, detected by immunohistochemistry for
c-H2AX, were measured. Adenine significantly increased the concentrations of urea and creatinine in plasma, significantly decreased the creatinine clearance and induced significant increases in the concentration of the measured inflammatory mediators.
Further, it caused oxidative stress and DNA damage. Treatment with GA significantly ameliorated these actions. The mechanism of the reported salutary effect of GA in adenine-induced CRF is associated with mitigation of the adenine-induced inflammation and generation of free radicals.
KW  - adenine
KW  - blood plasma
KW  - creatinine
KW  - inflammation
KW  - inflammatory diseases
KW  - Kidneys
KW  - Oxidative stress
KW  - Water resources
Y1  - 2013
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-95787
ER  - 
TY  - JOUR
A1  - Albert-Weissenberger, Christiane
A1  - Mencl, Stine
A1  - Schuhmann, Michael K.
A1  - Salur, Irmak
A1  - Göb, Eva
A1  - Langhauser, Friederike
A1  - Hopp, Sarah
A1  - Hennig, Nelli
A1  - Meuth, Sven G.
A1  - Nolte, Marc W.
A1  - Sirén, Anna-Leena
A1  - Kleinschnitz, Christoph
T1  - C1-Inhibitor protects from focal brain trauma in a cortical cryolesion mice model by reducing thrombo-inflammation
JF  - Frontiers in Cellular Neuroscience
N2  - Traumatic brain injury (TBI) induces a strong inflammatory response which includes blood-brain barrier damage, edema formation and infiltration of different immune cell subsets. More recently, microvascular thrombosis has been identified as another pathophysiological feature of TBI. The contact-kinin system represents an interface between inflammatory and thrombotic circuits and is activated in different neurological diseases. C1-Inhibitor counteracts activation of the contact-kinin system at multiple levels. We investigated the therapeutic potential of C1-Inhibitor in a model of TBI. Male and female C57BL/6 mice were subjected to cortical cryolesion and treated with C1-Inhibitor after 1 h. Lesion volumes were assessed between day 1 and day 5 and blood-brain barrier damage, thrombus formation as well as the local inflammatory response were determined post TBI. Treatment of male mice with 15.0 IU C1-Inhibitor, but not 7.5 IU, 1 h after cryolesion reduced lesion volumes by ~75% on day 1. This protective effect was preserved in female mice and at later stages of trauma. Mechanistically, C1-Inhibitor stabilized the blood-brain barrier and decreased the invasion of immune cells into the brain parenchyma. Moreover, C1-Inhibitor had strong antithrombotic effects. C1-Inhibitor represents a multifaceted anti-inflammatory and antithrombotic compound that prevents traumatic neurodegeneration in clinically meaningful settings.
KW  - thrombosis
KW  - traumatic brain injury
KW  - C1-inhibitor
KW  - blood-brain barrier
KW  - contact-kinin system
KW  - edema
KW  - inflammation
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119263
SN  - 1662-5102
VL  - 8
ER  - 
TY  - JOUR
A1  - Hütten, Mareike
A1  - Dhanasingh, Anandhan
A1  - Hessler, Roland
A1  - Stöver, Timo
A1  - Esser, Karl-Heinz
A1  - Möller, Martin
A1  - Lenarz, Thomas
A1  - Jolly, Claude
A1  - Groll, Jürgen
A1  - Scheper, Verena
T1  - In Vitro and In Vivo Evaluation of a Hydrogel Reservoir as a Continuous Drug Delivery System for Inner Ear Treatment
JF  - PLoS ONE
N2  - Fibrous tissue growth and loss of residual hearing after cochlear implantation can be reduced by application of the glucocorticoid dexamethasone-21-phosphate-disodium-salt (DEX). To date, sustained delivery of this agent to the cochlea using a number of pharmaceutical technologies has not been entirely successful. In this study we examine a novel way of continuous local drug application into the inner ear using a refillable hydrogel functionalized silicone reservoir. A PEG-based hydrogel made of reactive NCO-sP(EO-stat-PO) prepolymers was evaluated as a drug conveying and delivery system in vitro and in vivo. Encapsulating the free form hydrogel into a silicone tube with a small opening for the drug diffusion resulted in delayed drug release but unaffected diffusion of DEX through the gel compared to the free form hydrogel. Additionally, controlled DEX release over several weeks could be demonstrated using the hydrogel filled reservoir. Using a guinea-pig cochlear trauma model the reservoir delivery of DEX significantly protected residual hearing and reduced fibrosis. As well as being used as a device in its own right or in combination with cochlear implants, the hydrogel-filled reservoir represents a new drug delivery system that feasibly could be replenished with therapeutic agents to provide sustained treatment of the inner ear.
KW  - gels
KW  - cochlea
KW  - silicones
KW  - deafness
KW  - inner ear
KW  - drug delivery
KW  - inflammation
KW  - connective tissue
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-119375
VL  - 9
IS  - 8
ER  - 
TY  - JOUR
A1  - Cardani, Diego
A1  - Sardi, Claudia
A1  - La Ferla, Barbara
A1  - D'Orazio, Guiseppe
A1  - Sommariva, Michele
A1  - Marcucci, Fabrizio
A1  - Olivero, Daniela
A1  - Tagliabue, Elda
A1  - Koepsell, Hermann
A1  - Nicotra, Francesco
A1  - Balsari, Andrea
A1  - Rumio, Christiano
T1  - Sodium glucose cotransporter 1 ligand BLF501 as a novel tool for management of gastrointestinal mucositis
JF  - Molecular Cancer
N2  - Background: Recent studies demonstrated that engagement of sodium glucose transporter 1 (SGLT-1) by orally administered D-glucose protects the intestinal mucosa from lipopolysaccharide (LPS)-induced injury. We tested whether SGLT-1 engagement might protect the intestinal mucosa from doxorubicin (DXR)- and 5-fluorouracil (5-FU)-induced injury in animal models mimicking acute or chronic mucositis. 
Methods: Mice were treated intraperitoneally with DXR, alone or in combination with 5-FU, and orally with BLF501, a glucose-derived synthetic compound with high affinity for SGLT-1. Intestinal mucosal epithelium integrity was assessed by histological analysis, cellular proliferation assays, real-time PCR gene expression assays and Western blot assays. Student's t-test (paired two-tailed) and X-2 analyses were used for comparisons between groups. Differences were considered significant at p < 0.05. 
Results: BLF501 administration in mice treated with DXR and/or 5-FU decreased the injuries to the mucosa in terms of epithelial integrity and cellular proliferative ability. Co-treatment with BLF501 led to a normal expression and distribution of both zonula occludens-1 (ZO-1) and beta-catenin, which were underexpressed after treatment with either chemotherapeutic agent alone. BLF501 administration also restored normal expression of caspase-3 and ezrin/radixin/moesin (ERM), which were overexpressed after treatment with DXR and 5-FU. In SGLT1-/- mice, BLF501 had no detectable effects. BLF501 administration in wild-type mice with growing A431 tumors did not modify antitumor activity of DXR. 
Conclusions: BLF501-induced protection of the intestinal mucosa is a promising novel therapeutic approach to reducing the severity of chemotherapy-induced mucositis.
KW  - apoptosis
KW  - prevention
KW  - doxorubicin
KW  - cancer
KW  - gastrointestinal mucositis
KW  - SGLT-1
KW  - synthetic D-glucose analogy
KW  - chemotherapy
KW  - inflammation
KW  - clinical practice guidelines
KW  - intestinal mucositis
KW  - epithelial cells
KW  - oral mucositis
KW  - gene-expression
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-117352
SN  - 1476-4598
VL  - 13
IS  - 23
ER  - 
TY  - JOUR
A1  - Rittner, Heike L.
A1  - Wang, Ying
A1  - Gehringer, Rebekka
A1  - Mousa, Shaaban A.
A1  - Hackel, Dagmar
A1  - Brack, Alexander
T1  - CXCL10 Controls Inflammatory Pain via Opioid Peptide- Containing Macrophages in Electroacupuncture
N2  - Acupuncture is widely used for pain treatment in patients with osteoarthritis or low back pain, but molecular mechanisms remain largely enigmatic. In the early phase of inflammation neutrophilic chemokines direct opioid-containing neutrophils in the inflamed tissue and stimulate opioid peptide release and antinociception. In this study the molecular pathway and neuroimmune connections in complete Freund's adjuvant (CFA)-induced hind paw inflammation and electroacupuncture for peripheral pain control were analyzed. Free moving Wistar rats with hind paw inflammation were treated twice with electroacupuncture at GB30 (Huan Tiao - gall bladder meridian) (day 0 and 1) and analyzed for mechanical and thermal nociceptive thresholds. The cytokine profiles as well as the expression of opioid peptides were quantified in the inflamed paw. Electroacupuncture elicited long-term antinociception blocked by local injection of anti-opioid peptide antibodies (beta-endorphin, met-enkephalin, dynorphin A). The treatment altered the cytokine profile towards an anti-inflammatory pattern but augmented interferon (IFN)-gamma and the chemokine CXCL10 (IP-10: interferon gamma-inducible protein) protein and mRNA expression with concomitant increased numbers of opioid peptide-containing CXCR3+ macrophages. In rats with CFA hind paw inflammation without acupuncture repeated injection of CXCL10 triggered opioid-mediated antinociception and increase opioid-containing macrophages. Conversely, neutralization of CXCL10 time-dependently decreased electroacupuncture-induced antinociception and the number of infiltrating opioid peptide-expressing CXCR3+ macrophages. In summary, we describe a novel function of the chemokine CXCL10 - as a regulator for an increase of opioid-containing macrophages and antinociceptive mediator in inflammatory pain and as a key chemokine regulated by electroacupuncture.
KW  - opioids
KW  - inflammation
KW  - macrophages
KW  - cytokines
KW  - chemokines
KW  - enzyme-linkes immunoassays
KW  - acupuncture
KW  - analysis of variance
Y1  - 2014
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-112979
ER  - 
TY  - THES
A1  - Panjwani, Priyadarshini
T1  - Induction, Imaging, Histo-morphological and Molecular Characterization of Myocarditis in the Rat to Explore Novel Diagnostic Strategies for the Detection of Myocardial Inflammation
T1  - Induktion, Bildgebung und, Histo-morphologische sowie Molekulare Charakterisierung der Myokarditis im Rattenmodell zur Entwicklung neuer diagnostischer Strategien zum Nachweis von Herzmuskelentzündungen
N2  - Fulminant myocarditis is rare but a potentially life-threatening disease. Acute or mild myocarditis following acute ischemia is generally associated with a profound activation of the host’s immune system. On one hand this is mandatory to protect the host’s heart by fighting the invading agents (i.e., bacteria, viruses or other microbial agents) and/or to induce healing and repair processes in the damaged myocardium. On other hand, uncontrolled activation of the immune system may result in the generation of auto-reactive (not always beneficial) immune cells. 
Myocarditis or inflammatory cardiomyopathy is characterized by focal or diffuse infiltrates, myocyte necrosis and/or apoptosis and subsequent fibrotic replacement of the heart muscle. In humans, about 30% of the myocarditis-patients develop dilated cardiomyopathy. As the clinical picture of myocarditis is multifaceted, it is difficult to diagnose the disease. Therefore, the main goal of the present work was to test and further develop novel non-invasive methods for the detection of myocardial inflammation by employing both contrast enhanced MRI techniques as well as novel nuclear tracers that are suitable for  in vivo PET/ SPECT imaging.
As a part of this thesis, a pre-clinical animal model was successfully established by immunizing female Lewis rats with whole-porcine cardiac myosin (CM). Induction of Experimental Autoimmune Myocarditis (EAM) is considered successful when anti-myosin antibody titers are increased more than 100-fold over control animals and pericardial effusion develops. In addition, cardiac tissues from EAM-rats versus controls were analyzed for the expression of various pro-inflammatory and fibrosis markers. To further exploit non-invasive MRI techniques for the detection of myocarditis, our EAM-rats were injected either with (1) ultra-small Paramagnetic iron oxide particles (USPIO’s; Feraheme®), allowing for in vivo imaging , (2) micron sized paramagnetic iron oxide particles (MPIO) for ex vivo inflammatory cell-tracking by cMRI, or (3) with different radioactive nuclear tracers (67gallium citrate, 68gallium-labeled somatostatin analogue, and 68gallium-labeled cyclic RGD-peptide) which in the present work have been employed for autoradiographic imaging, but in principle are also suitable for in vivo nuclear imaging (PET/SPECT). In order to compare imaging results with histology, consecutive heart sections were stained with hematoxylin & eosin (HE, for cell infiltrates) and Masson Goldner trichrome (MGT, for fibrosis); in addition, immuno-stainings were performed with anti-CD68 (macrophages), anti-SSRT2A (somatostatin receptor type 2A), anti-CD61 (β3-integrins) and anti-CD31 (platelet endothelial cell adhesion molecule 1).
Sera from immunized rats strongly reacted with cardiac myosin. In immunized rats, echocardiography and subsequent MRI revealed huge amounts of pericardial effusion (days 18-21). Analysis of the kinetics of myocardial infiltrates revealed maximal macrophage invasion between days 14 and 28. Disappearance of macrophages resulted in replacement-fibrosis in formerly cell-infiltrated myocardial areas. This finding was confirmed by the time-dependent differential expression of corresponding cytokines in the myocardium. Immunized animals reacted either with an early or a late pattern of post-inflammation fibrosis. Areas with massive cellular infiltrates were easily detectible in autoradiograms showing a high focal uptake of 67gallium-citrate and 68gallium labeled somatostatin analogues (68Ga DOTA-TATE). Myocardium with a loss of cardiomyocytes presented a high uptake of 68gallium labeled cyclic RGD-peptide (68Ga NOTA-RGD). MRI cell tracking experiments with Feraheme® as the contrast-agent were inconclusive; however, strikingly better results were obtained when MPIOs were used as a contrast-agent: histological findings correlated well with in vivo and ex vivo MPIO-enhanced MRI images. 
Imaging of myocardial inflammatory processes including the kinetics of macrophage invasion after microbial or ischemic damage is still a major challenge in, both animal models and in human patients. By applying a broad panel of biochemical, histological, molecular and imaging methods, we show here that different patterns of reactivity may occur upon induction of myocarditis using one and the same rat strain. In particular, immunized Lewis rats may react either with an early or a late pattern of macrophage invasion and subsequent post-inflammation fibrosis. Imaging results achieved in the acute inflammatory phase of the myocarditis with MPIOs, 67gallium citrate and 68gallium linked to somatostatin will stimulate further development of contrast agents and radioactive-nuclear tracers for the non-invasive detection of acute myocarditis and in the near future perhaps even in human patients.
N2  - Eine fulminant verlaufende Myokarditis ist eine seltene aber potentiell lebensbedrohliche Erkrankung. Akute oder chronische Myokarditis gehen generell mit einer starken Aktivierung des Immunsystems der Betroffenen einher. Zum einen ist dies notwendig, um das Herz durch Bekämpfung der Eindringlinge (z.B. Bakterien, Viren oder andere mikrobielle Erreger) zu schützen und/oder Heilungs- und Reparaturprozesse im geschädigten Myokard einzuleiten. Zum anderen kann eine unkontrollierte Aktivierung des Immunsystems aber auch zur Entstehung von (nicht immer vorteilhaften) auto-reaktiven Immunzellen führen.
Eine Myokarditis oder entzündliche Kardiomyopathie ist charakterisiert durch fokale oder diffuse Infiltrate, Nekrose und/oder Apoptose der Myozyten und einen fortschreitenden fibrotischen Ersatz des Herzmuskelgewebes. Beim Menschen entwickeln etwa 30% der Myokarditis-Patienten eine dilatative Kardiomyopathie. Da das klinische Bild der Myokarditis sehr vielfältig sein kann, ist die Diagnosestellung dieser Erkrankung schwierig. Deshalb war es das Kernziel dieser Arbeit, nicht-invasive Methoden zum Nachweis myokardialer Entzündungen zu testen, und dabei neue Bildgebungsverfahren unter Einsatz von neuen MRT-Kontrastmitteln sowie neuen nuklearen Tracern, die auch für PET/SPECT geeignet wären, zu entwickeln. Diese Verfahren wurden von uns zunächst an einem human-analogen Ratten-Modell evaluiert, mit dem Ziel später evtl. auch einmal beim Menschen eingesetzt werden zu können.
Für unser präklinisches Tiermodell wurden weibliche Lewis-Ratten mit kardialem Myosin aus Schweinen immunisiert. Die erfolgreiche Induktion einer „Experimentellen Autoimmunen Myokarditis (EAM)“ wurde durch einen signifikanten Anstieg der Anti-Myosin Antikörpertiter in immunisierten Tieren und die Ausbildung eines Perikardergusses (Echokardiographie) bestätigt. Zusätzlich wurde aus apikalem kardialem Gewebe RNA isoliert und die Expression verschiedener pro-inflammatorischer und pro-fibrotischer molekularer Marker untersucht. Um die Bildgebung mittels kontrast-verstärktem cMRT zu optimieren, wurden den Tieren entweder kleine Eisenoxid-Nanopartikel (Ultra small paramagnetic iron oxide particles, USPIO; Feraheme®), oder sog. ,,Micronsized paramagnetic iron oxide particles (MPIO)‘‘ für das Tracking inflammatorischer Zellen injiziert. Im daraufolgenden Schritt wurden radioaktive nukleare Tracer (67Gallium-Citrat, 68Gallium-markierte Somatostatin-Analoga und 68Gallium-markierte zyklische RGD-Peptide) injiziert, um dann Autoradiogramme von Herzschnitten zu gewinnen.
KW  - Ratte
KW  - inflammation
KW  - Myokarditis
KW  - Kernspintomografie
KW  - myocarditis
KW  - MRI
KW  - cardiovascular
KW  - Entzündung
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-122469
ER  - 
TY  - JOUR
A1  - Schick, Martin Alexander
A1  - Baar, Wolfgang
A1  - Bruno, Raphael Romano
A1  - Wollborn, Jakob
A1  - Held, Christopher
A1  - Schneider, Reinhard
A1  - Flemming, Sven
A1  - Schlegel, Nicolas
A1  - Roewer, Norbert
A1  - Neuhaus, Winfried
A1  - Wunder, Christian
T1  - Balanced hydroxyethylstarch (HES 130/0.4) impairs kidney function in-vivo without inflammation
JF  - PLoS One
N2  - Volume therapy is a standard procedure in daily perioperative care, and there is an ongoing discussion about the benefits of colloid resuscitation with hydroxyethylstarch (HES). In sepsis HES should be avoided due to a higher risk for acute kidney injury (AKI). Results of the usage of HES in patients without sepsis are controversial. Therefore we conducted an animal study to evaluate the impact of 6% HES 130/0.4 on kidney integrity with sepsis or under healthy conditions Sepsis was induced by standardized Colon Ascendens Stent Peritonitis (sCASP). sCASP-group as well as control group (C) remained untreated for 24 h. After 18 h sCASP+HES group (sCASP+VOL) and control+HES (C+VOL) received 50 ml/KG balanced 6% HES (VOL) 130/0.4 over 6h. After 24h kidney function was measured via Inulin- and PAH-Clearance in re-anesthetized rats, and serum urea, creatinine (crea), cystatin C and Neutrophil gelatinase-associated lipocalin (NGAL) as well as histopathology were analysed. In vitro human proximal tubule cells (PTC) were cultured +/- lipopolysaccharid (LPS) and with 0.1–4.0% VOL. Cell viability was measured with XTT-, cell toxicity with LDH-test. sCASP induced severe septic AKI demonstrated divergent results regarding renal function by clearance or creatinine measure focusing on VOL. Soleley HES (C+VOL) deteriorated renal function without sCASP. Histopathology revealed significantly derangements in all HES groups compared to control. In vitro LPS did not worsen the HES induced reduction of cell viability in PTC cells. For the first time, we demonstrated, that application of 50 ml/KG 6% HES 130/0.4 over 6 hours induced AKI without inflammation in vivo. Severity of sCASP induced septic AKI might be no longer susceptible to the way of volume expansion
KW  - colloids
KW  - kidneys
KW  - histopathology
KW  - blood
KW  - creatinine
KW  - sepsis
KW  - urine
KW  - inflammation
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-126068
VL  - 10
IS  - 9
ER  - 
TY  - JOUR
A1  - Loeffler, Claudia
A1  - Loeffler, Jürgen
A1  - Kobsar, Anna
A1  - Speer, Christian P.
A1  - Eigenthaler, Martin
T1  - Septic Vs Colonizing Group B Streptococci Differentially Regulate Inflammation and Apoptosis in Human Coronary Artery Endothelial Cells - a Pilot Study
JF  - Journal of Pediatrics and Neonatal Care
N2  - In this pilot study, we exemplify differences between a septic and a colonizing GBS strain during their interaction with Endothelial Cells by evaluating cytokine levels, surface and apoptosis-related molecules. These preliminary results indicate that in vitro infection using an exemplary septic GBS strain results in diminished activation of the innate immune response.
KW  - streptococci
KW  - apoptosis
KW  - inflammation
KW  - endothelial cells
KW  - innate immunity
KW  - early onset sepsis
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125596
VL  - 2
IS  - 2
ER  - 
TY  - JOUR
A1  - Wagner, Martin
A1  - Ashby, Damien R.
A1  - Kurtz, Caroline
A1  - Alam, Ahsan
A1  - Busbridge, Mark
A1  - Raff, Ulrike
A1  - Zimmermann, Josef
A1  - Heuschmann, Peter U.
A1  - Wanner, Christoph
A1  - Schramm, Lothar
T1  - Hepcidin-25 in diabetic chronic kidney disease is predictive for mortality and progression to end stage renal disease
JF  - PLoS One
N2  - Background
Anemia is common and is associated with impaired clinical outcomes in diabetic chronic kidney disease (CKD). It may be explained by reduced erythropoietin (EPO) synthesis, but recent data suggest that EPO-resistance and diminished iron availability due to inflammation contribute significantly. In this cohort study, we evaluated the impact of hepcidin-25—the key hormone of iron-metabolism—on clinical outcomes in diabetic patients with CKD along with endogenous EPO levels.

Methods
249 diabetic patients with CKD of any stage, excluding end-stage renal disease (ESRD), were enrolled (2003–2005), if they were not on EPO-stimulating agent and iron therapy. Hepcidin-25 levels were measured by radioimmunoassay. The association of hepcidin-25 at baseline with clinical variables was investigated using linear regression models. All-cause mortality and a composite endpoint of CKD progression (ESRD or doubling of serum creatinine) were analyzed by Cox proportional hazards models.

Results
Patients (age 67 yrs, 53% male, GFR 51 ml/min, hemoglobin 131 g/L, EPO 13.5 U/L, hepcidin-25 62.0 ng/ml) were followed for a median time of 4.2 yrs. Forty-nine patients died (19.7%) and forty (16.1%) patients reached the composite endpoint. Elevated hepcidin levels were independently associated with higher ferritin-levels, lower EPO-levels and impaired kidney function (all p<0.05). Hepcidin was related to mortality, along with its interaction with EPO, older age, greater proteinuria and elevated CRP (all p<0.05). Hepcidin was also predictive for progression of CKD, aside from baseline GFR, proteinuria, low albumin- and hemoglobin-levels and a history of CVD (all p<0.05).

Conclusions
We found hepcidin-25 to be associated with EPO and impaired kidney function in diabetic CKD. Elevated hepcidin-25 and EPO-levels were independent predictors of mortality, while hepcidin-25 was also predictive for progression of CKD. Both hepcidin-25 and EPO may represent important prognostic factors of clinical outcome and have the potential to further define “high risk” populations in CKD.
KW  - diabetes mellitus
KW  - inflammation
KW  - type 2 diabetes
KW  - hemoglobin
KW  - chronic kidney disease
KW  - anemia
KW  - ferritin
KW  - proteinuria
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-125514
VL  - 10
IS  - 4
ER  - 
TY  - JOUR
A1  - Schrewe, L.
A1  - Lill, C. M.
A1  - Liu, T.
A1  - Salmen, A.
A1  - Gerdes, L. A.
A1  - Guillot-Noel, L.
A1  - Akkad, D. A.
A1  - Blaschke, P.
A1  - Graetz, C.
A1  - Hoffjan, S.
A1  - Kroner, A.
A1  - Demir, S.
A1  - Böhme, A.
A1  - Rieckmann, P.
A1  - El Ali, A.
A1  - Hagemann, N.
A1  - Hermann, D. M.
A1  - Cournu-Rebeix, I.
A1  - Zipp, F.
A1  - Kümpfel, T.
A1  - Buttmann, M.
A1  - Zettl, U. K.
A1  - Fontaine, B.
A1  - Bertram, L.
A1  - Gold, R.
A1  - Chan, A.
T1  - Investigation of sex-specific effects of apolipoprotein E on severity of EAE and MS
JF  - Journal of Neuroinflammation
N2  - Background: Despite pleiotropic immunomodulatory effects of apolipoprotein E (apoE) in vitro, its effects on the clinical course of experimental autoimmune encephalomyelitis (EAE) and multiple sclerosis (MS) are still controversial. As sex hormones modify immunomodulatory apoE functions, they may explain contentious findings. This study aimed to investigate sex-specific effects of apoE on disease course of EAE and MS. 
Methods: MOG\(_{35-55}\) induced EAE in female and male apoE-deficient mice was assessed clinically and histopathologically. apoE expression was investigated by qPCR. The association of the MS severity score (MSSS) and APOE rs429358 and rs7412 was assessed across 3237 MS patients using linear regression analyses. 
Results: EAE disease course was slightly attenuated in male apoE-deficient (apoE\(^{-/-}\)) mice compared to wildtype mice (cumulative median score: apoE\(^{-/-}\) = 2 [IQR 0.0-4.5]; wildtype = 4 [IQR 1.0-5.0]; n = 10 each group, p = 0.0002). In contrast, EAE was more severe in female apoE\(^{-/-}\) mice compared to wildtype mice (cumulative median score: apoE\(^{-/-}\) = 3 [IQR 2.0-4.5]; wildtype = 3 [IQR 0.0-4.0]; n = 10, p = 0.003). In wildtype animals, apoE expression during the chronic EAE phase was increased in both females and males (in comparison to naive animals; p < 0.001). However, in MS, we did not observe a significant association between MSSS and rs429358 or rs7412, neither in the overall analyses nor upon stratification for sex. 
Conclusions: apoE exerts moderate sex-specific effects on EAE severity. However, the results in the apoE knock-out model are not comparable to effects of polymorphic variants in the human APOE gene, thus pinpointing the challenge of translating findings from the EAE model to the human disease.
KW  - immune
KW  - apoE
KW  - gender
KW  - inflammation
KW  - association studies in genetics
KW  - apoe
KW  - CNS disease
KW  - system
KW  - multiple sclerosis
KW  - MSSS
KW  - experimental autoimmune encephalomyelitis
KW  - disease severity
KW  - cognitive function
KW  - Alzheimer disease
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-136252
VL  - 12
IS  - 234
ER  - 
TY  - JOUR
A1  - Schuhmann, Michael K.
A1  - Bittner, Stefan
A1  - Meuth, Sven G.
A1  - Kleinschnitz, Christoph
A1  - Fluri, Felix
T1  - Fingolimod (FTY720-P) does not stabilize the blood-brain barrier under inflammatory conditions in an in vitro model
JF  - International Journal of Molecular Sciences
N2  - Breakdown of the blood-brain barrier (BBB) is an early hallmark of multiple sclerosis (MS), a progressive inflammatory disease of the central nervous system. Cell adhesion in the BBB is modulated by sphingosine-1-phosphate (S1P), a signaling protein, via S1P receptors (S1P\(_1\)). Fingolimod phosphate (FTY720-P) a functional S1P\(_1\) antagonist has been shown to improve the relapse rate in relapsing-remitting MS by preventing the egress of lymphocytes from lymph nodes. However, its role in modulating BBB permeabilityin particular, on the tight junction proteins occludin, claudin 5 and ZO-1has not been well elucidated to date. In the present study, FTY720-P did not change the transendothelial electrical resistance in a rat brain microvascular endothelial cell (RBMEC) culture exposed to inflammatory conditions and thus did not decrease endothelial barrier permeability. In contrast, occludin was reduced in RBMEC culture after adding FTY720-P. Additionally, FTY720-P did not alter the amount of endothelial matrix metalloproteinase (MMP)-9 and MMP-2 in RBMEC cultures. Taken together, our observations support the assumption that S1P\(_1\) plays a dual role in vascular permeability, depending on its ligand. Thus, S1P\(_1\) provides a mechanistic basis for FTY720-P-associated disruption of endothelial barrierssuch as the blood-retinal barrierwhich might result in macular edema.
KW  - randomized controlled trial
KW  - Sphingosine 1-Phosphate
KW  - vascular permeability
KW  - rat brain microvascular endothelial cell culture
KW  - tight junctions
KW  - FTY720-P
KW  - blood-brain barrier
KW  - inflammation
KW  - novo renal transplantation
KW  - endothelial cells
KW  - experimental autoimmune encephalomyelitis
KW  - relapsing multiple sclerosis
KW  - Zonula Occludens-1
KW  - matrix metalloproteinases
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-145047
VL  - 16
ER  - 
TY  - JOUR
A1  - Ebert, Regina
A1  - Benisch, Peggy
A1  - Krug, Melanie
A1  - Zeck, Sabine
A1  - Meißner-Weigl, Jutta
A1  - Steinert, Andre
A1  - Rauner, Martina
A1  - Hofbauer, Lorenz
A1  - Jakob, Franz
T1  - Acute phase serum amyloid A induces proinflammatory cytokines and mineralization via toll-like receptor 4 in mesenchymal stem cells
JF  - Stem Cell Research
N2  - The role of serum amyloid A (SAA) proteins, which are ligands for toll-like receptors, was analyzed in human bone marrow-derived mesenchymal stem cells (hMSCs) and their osteogenic offspring with a focus on senescence, differentiation andmineralization. In vitro aged hMSC developed a senescence-associated secretory phenotype (SASP), resulting in enhanced SAA1/2, TLR2/4 and proinflammatory cytokine (IL6, IL8, IL1\(\beta\), CXCL1, CXCL2) expression before entering replicative senescence. Recombinant human SAA1 (rhSAA1) induced SASP-related genes and proteins in MSC, which could be abolished by cotreatment with the TLR4-inhibitor CLI-095. The same pattern of SASP-resembling genes was stimulated upon induction of osteogenic differentiation, which is accompanied by autocrine SAA1/2 expression. In this context additional rhSAA1 enhanced the SASP-like phenotype, accelerated the proinflammatory phase of osteogenic differentiation and enhanced mineralization. Autocrine/paracrine and rhSAA1 via TLR4 stimulate a proinflammatory phenotype that is both part of the early phase of osteogenic differentiation and the development of senescence. This signaling cascade is tightly involved in bone formation and mineralization, but may also propagate pathological extraosseous calcification conditions such as calcifying inflammation and atherosclerosis.
KW  - human atherosclerotic lesions
KW  - senescence
KW  - expression
KW  - toll-like receptor
KW  - mineralization
KW  - osteogenic differentiation
KW  - serum amyloid A
KW  - inflammation
KW  - mesenchymal stem cells
KW  - WNT5A
KW  - model
KW  - lines
KW  - stromal cells
KW  - RT-PCR
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-148491
VL  - 15
ER  - 
TY  - JOUR
A1  - Macedo, Robson
A1  - Javadi, Som Mehrbod
A1  - Higuchi, Takahiro
A1  - Ferreira de Carvalho, Marilia Daniela
A1  - Lima Paiva Medeiros, Vanessa de Fátima
A1  - Azevedo, Ítalo Medeiros
A1  - Lima, Francisco Pignataro
A1  - Medeiros, Aldo Cunha
T1  - Heart and systemic effects of statin pretreatment in a rat model of abdominal sepsis. Assessment by Tc\(^{99m}\)-sestamibi biodistribition
JF  - Acta Cirúrgica Brasileira
N2  - PURPOSE: 
To evaluate the heart and the Tc-99m-sestamibi biodistribution after statin pretreatment in a rat model of abdominal sepsis. 

METHODS: 
Twenty-four Wistar rats were randomly distributed into four groups (n=6 per group): 1) sepsis with simvastatin treatment, 2) sepsis with vehicle, 3) sham control with simvastatin and 4) sham control with vehicle. 24 hours after cecal ligation and puncture rats received 1.0MBq of Tc-99m-sestamibi i.v. 30min after, animals were euthanized for ex-vivo tissue counting and myocardium histological analysis. 

RESULTS: 
Myocardial histologic alterations were not detected 24 hours post-sepsis. There was significantly increased cardiac Tc-99m-sestamibi activity in the sepsis group with simvastatin treatment (1.9\(\pm\)0.3%ID/g, p<0.001) in comparison to the sepsis group+vehicle (1.0\(\pm\)0.2% ID/g), control sham group+ simvastatin (1.2\(\pm\)0.3% ID/g) and control sham group (1.3\(\pm\)0.2% ID/g). Significant Tc-99m-sestamibi activity in liver, kidney and lungs was also detected in the sepsis group treated with simvastatinin comparison to the other groups. 

CONCLUSIONS: 
Statin treatment altered the biodistribution of Tc-99m-sestamibi with increased cardiac and solid organ activity in rats with abdominal sepsis, while no impact on controls. Increased myocardial tracer activity may be a result of a possible protection effect due to increased tissue perfusion mediated by statins.
KW  - P-glycoprotein expression
KW  - mechanisms retention
KW  - Simvastatin
KW  - Technetium Tc 99m Sestamibi Rats
KW  - heart
KW  - inflammation
KW  - sepsis
Y1  - 2015
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-151887
VL  - 30
IS  - 6
SP  - 388
EP  - 393
ER  - 
TY  - JOUR
A1  - Fehrholz, Markus
A1  - Glaser, Kirsten
A1  - Seidenspinner, Silvia
A1  - Ottensmeier, Barbara
A1  - Curstedt, Tore
A1  - Speer, Christian P.
A1  - Kunzmann, Steffen
T1  - Impact of the New Generation Reconstituted Surfactant CHF5633 on Human CD4\(^+\) Lymphocytes
JF  - PLoS One
N2  - Background
Natural surfactant preparations, commonly isolated from porcine or bovine lungs, are used to treat respiratory distress syndrome in preterm infants. Besides biophysical effectiveness, several studies have documented additional immunomodulatory properties. Within the near future, synthetic surfactant preparations may be a promising alternative. CHF5633 is a new generation reconstituted synthetic surfactant preparation with defined composition, containing dipalmitoyl-phosphatidylcholine, palmitoyl-oleoyl-phosphatidylglycerol and synthetic analogs of surfactant protein (SP-) B and SP-C. While its biophysical effectiveness has been demonstrated in vitro and in vivo, possible immunomodulatory abilities are currently unknown.

Aim
The aim of the current study was to define a potential impact of CHF5633 and its single components on pro- and anti-inflammatory cytokine responses in human CD4\(^+\) lymphocytes.

Methods
Purified human CD4\(^+\) T cells were activated using anti CD3/CD28 antibodies and exposed to CHF5633, its components, or to the well-known animal-derived surfactant Poractant alfa (Curosurf®). Proliferative response and cell viability were assessed using flow cytometry and a methylthiazolyldiphenyltetrazolium bromide colorimetric assay. The mRNA expression of IFNγ, IL-2, IL-17A, IL-22, IL-4, and IL-10 was measured by quantitative PCR, while intracellular protein expression was assessed by means of flow cytometry.

Results
Neither CHF5633 nor any of its phospholipid components with or without SP-B or SP-C analogs had any influence on proliferative ability and viability of CD4\(^+\) lymphocytes under the given conditions. IFNγ, IL-2, IL-17A, IL-22, IL-4, and IL-10 mRNA as well as IFNγ, IL-2, IL-4 and IL-10 protein levels were unaffected in both non-activated and activated CD4+ lymphocytes after exposure to CHF5633 or its constituents compared to non-exposed controls. However, in comparison to Curosurf®, expression levels of anti-inflammatory IL-4 and IL-10 mRNA were significantly increased in CHF5633 exposed CD4\(^+\) lymphocytes.

Conclusion
For the first time, the immunomodulatory capacity of CHF5633 on CD4\(^+\) lymphocytes was evaluated. CHF5633 did not show any cytotoxicity on CD4\(^+\) cells. Moreover, our in vitro data indicate that CHF5633 does not exert unintended pro-inflammatory effects on non-activated and activated CD4+ T cells. As far as anti-inflammatory cytokines are concerned, it might lack an overall reductive ability in comparison to animal-derived surfactants, potentially leaving pro- and anti-inflammatory cytokine response in balance.
KW  - lymphocytes
KW  - surfactants
KW  - flow cytometry
KW  - monocytes
KW  - RNA isolation
KW  - T cells
KW  - cytokines
KW  - inflammation
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146419
VL  - 11
IS  - 4
ER  - 
TY  - JOUR
A1  - Suliman, Salwa
A1  - Sun, Yang
A1  - Pedersen, Torbjorn O.
A1  - Xue, Ying
A1  - Nickel, Joachim
A1  - Waag, Thilo
A1  - Finne-Wistrand, Anna
A1  - Steinmüller-Nethl, Doris
A1  - Krueger, Anke
A1  - Costea, Daniela E.
A1  - Mustafa, Kamal
T1  - In vivo host response and degradation of copolymer scaffolds functionalized with nanodiamonds and bone morphogenetic protein 2
JF  - Advanced Healthcare Materials
N2  - The aim is to evaluate the effect of modifying poly[(L-lactide)-co-(epsilon-caprolactone)] scaffolds (PLCL) with nanodiamonds (nDP) or with nDP+physisorbed BMP-2 (nDP+BMP-2) on in vivo host tissue response and degradation. The scaffolds are implanted subcutaneously in Balb/c mice and retrieved after 1, 8, and 27 weeks. Molecular weight analysis shows that modified scaffolds degrade faster than the unmodified. Gene analysis at week 1 shows highest expression of proinflammatory markers around nDP scaffolds; although the presence of inflammatory cells and foreign body giant cells is more prominent around the PLCL. Tissue regeneration markers are highly expressed in the nDP+BMP-2 scaffolds at week 8. A fibrous capsule is detectable by week 8, thinnest around nDP scaffolds and at week 27 thickest around PLCL scaffolds. mRNA levels of ALP, COL1 alpha 2, and ANGPT1 are signifi cantly upregulating in the nDP+BMP-2 scaffolds at week 1 with ectopic bone seen at week 8. Even when almost 90% of the scaffold is degraded at week 27, nDP are observable at implantation areas without adverse effects. In conclusion, modifying PLCL scaffolds with nDP does not aggravate the host response and physisorbed BMP-2 delivery attenuates infl ammation while lowering the dose of BMP-2 to a relatively safe and economical level.
KW  - inflammatory response
KW  - biocompatibility
KW  - BMP-2 delivery
KW  - inflammation
KW  - tissue engineering
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-189764
VL  - 5
IS  - 6
ER  - 
TY  - JOUR
A1  - Rosenbaum, Corinna
A1  - Schick, Martin Alexander
A1  - Wollborn, Jakob
A1  - Heider, Andreas
A1  - Scholz, Claus-Jürgen
A1  - Cecil, Alexander
A1  - Niesler, Beate
A1  - Hirrlinger, Johannes
A1  - Walles, Heike
A1  - Metzger, Marco
T1  - Activation of Myenteric Glia during Acute Inflammation In Vitro and In Vivo
JF  - PLoS One
N2  - Background
Enteric glial cells (EGCs) are the main constituent of the enteric nervous system and share similarities with astrocytes from the central nervous system including their reactivity to an inflammatory microenvironment. Previous studies on EGC pathophysiology have specifically focused on mucosal glia activation and its contribution to mucosal inflammatory processes observed in the gut of inflammatory bowel disease (IBD) patients. In contrast knowledge is scarce on intestinal inflammation not locally restricted to the mucosa but systemically affecting the intestine and its effect on the overall EGC network.

Methods and Results
In this study, we analyzed the biological effects of a systemic LPS-induced hyperinflammatory insult on overall EGCs in a rat model in vivo, mimicking the clinical situation of systemic inflammation response syndrome (SIRS). Tissues from small and large intestine were removed 4 hours after systemic LPS-injection and analyzed on transcript and protein level. Laser capture microdissection was performed to study plexus-specific gene expression alterations. Upon systemic LPS-injection in vivo we observed a rapid and dramatic activation of Glial Fibrillary Acidic Protein (GFAP)-expressing glia on mRNA level, locally restricted to the myenteric plexus. To study the specific role of the GFAP subpopulation, we established flow cytometry-purified primary glial cell cultures from GFAP promotor-driven EGFP reporter mice. After LPS stimulation, we analyzed cytokine secretion and global gene expression profiles, which were finally implemented in a bioinformatic comparative transcriptome analysis. Enriched GFAP+ glial cells cultured as gliospheres secreted increased levels of prominent inflammatory cytokines upon LPS stimulation. Additionally, a shift in myenteric glial gene expression profile was induced that predominantly affected genes associated with immune response.

Conclusion and Significance
Our findings identify the myenteric GFAP-expressing glial subpopulation as particularly susceptible and responsive to acute systemic inflammation of the gut wall and complement knowledge on glial involvement in mucosal inflammation of the intestine.
KW  - gene expression
KW  - gastrointestinal tract
KW  - inflammatory bowel disease
KW  - central nervous system
KW  - systemic inflammatory response syndrome
KW  - inflammation
KW  - astrocytes
KW  - cytokines
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146544
VL  - 11
IS  - 3
ER  - 
TY  - JOUR
A1  - Alrefai, Hani
A1  - Muhammad, Khalid
A1  - Rudolf, Ronald
A1  - Pham, Duong Anh Thuy
A1  - Klein-Hessling, Stefan
A1  - Patra, Amiya K.
A1  - Avots, Andris
A1  - Bukur, Valesca
A1  - Sahin,, Ugur
A1  - Tenzer, Stefan
A1  - Goebeler, Matthias
A1  - Kerstan, Andreas
A1  - Serfling, Edgar
T1  - NFATc1 supports imiquimod-induced skin inflammation by suppressing IL-10 synthesis in B cells
JF  - Nature Communications
N2  - Epicutaneous application of Aldara cream containing the TLR7 agonist imiquimod (IMQ) to mice induces skin inflammation that exhibits many aspects of psoriasis, an inflammatory human skin disease. Here we show that mice depleted of B cells or bearing interleukin (IL)-10-deficient B cells show a fulminant inflammation upon IMQ exposure, whereas ablation of NFATc1 in B cells results in a suppression of Aldara-induced inflammation. In vitro, IMQ induces the proliferation and IL-10 expression by B cells that is blocked by BCR signals inducing NFATc1. By binding to HDAC1, a transcriptional repressor, and to an intronic site of the Il10 gene, NFATc1 suppresses IL-10 expression that dampens the production of tumour necrosis factor-α and IL-17 by T cells. These data indicate a close link between NFATc1 and IL-10 expression in B cells and suggest NFATc1 and, in particular, its inducible short isoform, NFATc1/αA, as a potential target to treat human psoriasis.
KW  - B cells
KW  - psoriasis
KW  - interleukins
KW  - inflammation
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-173053
VL  - 7
ER  - 
TY  - JOUR
A1  - Howangyin, Kiave-Yune
A1  - Zlatanova, Ivana
A1  - Pinto, Cristina
A1  - Ngkelo, Anta
A1  - Cochain, Clément
A1  - Rouanet, Marie
A1  - Vilar, José
A1  - Lemitre, Mathilde
A1  - Stockmann, Christian
A1  - Fleischmann, Bernd K.
A1  - Mallat, Ziad
A1  - Silvestre, Jean-Sébastien
T1  - Myeloid-epithelial-reproductive receptor tyrosine kinase and milk fat globule epidermal growth factor 8 coordinately improve remodeling after myocardial infarction via local delivery of vascular endothelial growth factor
JF  - Circulation
N2  - Background: In infarcted heart, improper clearance of dying cells by activated neighboring phagocytes may precipitate the transition to heart failure. We analyzed the coordinated role of 2 major mediators of efferocytosis, the myeloid-epithelial-reproductive protein tyrosine kinase (Mertk) and the milk fat globule epidermal growth factor (Mfge8), in directing cardiac remodeling by skewing the inflammatory response after myocardial infarction. 
Methods and Results: We generated double-deficient mice for Mertk and Mfge8 (Mertk\(^{-/-}\)/Mfge8\(^{-/-}\)) and challenged them with acute coronary ligature. Compared with wild-type, Mertk-deficient (Mertk\(^{-/-}\)), or Mfge8-deficient (Mfge8\(^{-/-}\)) animals, Mertk\(^{-/-}\)/Mfge8\(^{-/-}\) mice displayed greater alteration in cardiac function and remodeling. Mertk and Mfge8 were expressed mainly by cardiac Ly6C\(^{High and Low}\) monocytes and macrophages. In parallel, Mertk\(^{-/-}\)/Mfge8\(^{-/-}\) bone marrow chimeras manifested increased accumulation of apoptotic cells, enhanced fibrotic area, and larger infarct size, as well as reduced angiogenesis. We found that the abrogation of efferocytosis affected neither the ability of circulating monocytes to infiltrate cardiac tissue nor the number of resident Ly6C\(^{High}\) and Ly6C\(^{Low}\) monocytes/macrophages populating the infarcted milieu. In contrast, combined Mertk and Mfge8 deficiency in Ly6C\(^{High}\)/Ly6C\(^{Low}\) monocytes/macrophages either obtained from in vitro differentiation of bone marrow cells or isolated from infarcted hearts altered their capacity of efferocytosis and subsequently blunted vascular endothelial growth factor A (VEGFA) release. Using LysMCre\(^+\)/VEGFA\(^{fl/fl}\) mice, we further identified an important role for myeloid-derived VEGFA in improving cardiac function and angiogenesis. 
Conclusions: After myocardial infarction, Mertk- and Mfge8-expressing monocyte/macrophages synergistically engage the clearance of injured cardiomyocytes, favoring the secretion of VEGFA to locally repair the dysfunctional heart.
KW  - inflammation
KW  - macrophages
KW  - myocardial infarction
KW  - myocarditis
KW  - neovascularization, physiologic
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-190755
VL  - 133
IS  - 9
ER  - 
TY  - JOUR
A1  - Schuhmann, Michael K.
A1  - Gunreben, Ignaz
A1  - Kleinschnitz, Christoph
A1  - Kraft, Peter
T1  - Immunohistochemical Analysis of Cerebral Thrombi Retrieved by Mechanical Thrombectomy from Patients with Acute Ischemic Stroke
JF  - International Journal of Molecular Sciences
N2  - Mechanical thrombectomy is a novel treatment option for patients with acute ischemic stroke (AIS). Only a few studies have previously suggested strategies to categorize retrieved clots according to their histologic composition. However, these reports did not analyze potential biomarkers that are of importance in stroke-related inflammation. We therefore histopathologically investigated 37 intracerebral thrombi mechanically retrieved from patients with AIS, and focused on the composition of immune cells and platelets. We also conducted correlation analyses of distinctive morphologic patterns (erythrocytic, serpentine, layered, red, white, mixed appearance) with clinical parameters. Most T cells and monocytes were detected in erythrocytic and red clots, in which the distribution of these cells was random. In contrast, von Willebrand factor (vWF)-positive areas co-localized with regions of fibrin and collagen. While clots with huge amounts of vWF seem to be associated with a high National Institute of Health Stroke Scale score at admission, histologic findings could not predict the clinical outcome at discharge. In summary, we provide the first histologic description of mechanically retrieved intracerebral thrombi regarding biomarkers relevant for inflammation in ischemic stroke.
KW  - thrombus formation
KW  - immune cells
KW  - lymphocytes
KW  - mechanical thrombectomy
KW  - ischemic stroke
KW  - inflammation
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-166206
VL  - 17
IS  - 3
ER  - 
TY  - JOUR
A1  - Grimmig, Tanja
A1  - Moench, Romana
A1  - Kreckel, Jennifer
A1  - Haack, Stephanie
A1  - Rueckert, Felix
A1  - Rehder, Roberta
A1  - Tripathi, Sudipta
A1  - Ribas, Carmen
A1  - Chandraker, Anil
A1  - Germer, Christoph T.
A1  - Gasser, Martin
A1  - Waaga-Gasser, Ana Maria
T1  - Toll Like Receptor 2, 4, and 9 Signaling Promotes Autoregulative Tumor Cell Growth and VEGF/PDGF Expression in Human Pancreatic Cancer
JF  - International Journal of Molecular Sciences
N2  - Toll like receptor (TLR) signaling has been suggested to play an important role in the inflammatory microenvironment of solid tumors and through this inflammation-mediated tumor growth. Here, we studied the role of tumor cells in their process of self-maintaining TLR expression independent of inflammatory cells and cytokine milieu for autoregulative tumor growth signaling in pancreatic cancer. We analyzed the expression of TLR2, -4, and -9 in primary human cancers and their impact on tumor growth via induced activation in several established pancreatic cancers. TLR-stimulated pancreatic cancer cells were specifically investigated for activated signaling pathways of VEGF/PDGF and anti-apoptotic Bcl-xL expression as well as tumor cell growth. The primary pancreatic cancers and cell lines expressed TLR2, -4, and -9. TLR-specific stimulation resulted in activated MAP-kinase signaling, most likely via autoregulative stimulation of demonstrated TLR-induced VEGF and PDGF expression. Moreover, TLR activation prompted the expression of Bcl-xL and has been demonstrated for the first time to induce tumor cell proliferation in pancreatic cancer. These findings strongly suggest that pancreatic cancer cells use specific Toll like receptor signaling to promote tumor cell proliferation and emphasize the particular role of TLR2, -4, and -9 in this autoregulative process of tumor cell activation and proliferation in pancreatic cancer.
KW  - tumor growth
KW  - TLR2
KW  - TLR4
KW  - TLR9
KW  - pancreatic cancer
KW  - inflammation
Y1  - 2016
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-165743
VL  - 17
IS  - 12
ER  - 
TY  - THES
A1  - Karl, Franziska
T1  - The role of miR-21 in the pathophysiology of neuropathic pain using the model of B7-H1 knockout mice
T1  - Die Rolle von miR-21 in der Pathophysiologie von neuropathischem Schmerz am Model der B7-H1 defizienten Maus
N2  - The impact of microRNA (miRNA) as key players in the regulation of immune and neuronal gene expression and their role as master switches in the pathophysiology of neuropathic pain is increasingly recognized. miR-21 is a promising candidate that could be linked to the immune and the nociceptive system. To further investigate the pathophysiological role of miR-21 in neuropathic pain, we assesed mice deficient of B7 homolog 1 (B7-H1 ko), a protein with suppressive effect on inflammatory responses.
B7-H1 ko mice and wildtype littermates (WT) of three different age-groups, young (8 weeks), middle-aged (6 months), and old (12 months) received a spared nerve injury (SNI). Thermal withdrawal latencies and mechanical withdrawal thresholds were determined. Further, we investigated anxiety-, depression-like and cognitive behavior. Quantitative real time PCR was used to determine miR-21 relative expression in peripheral nerves, dorsal root ganglia and white blood cells (WBC) at distinct time points after SNI. 
Naïve B7-H1 ko mice showed mechanical hyposensitivity with increasing age. Young and middle-aged B7-H1 ko mice displayed lower mechanical withdrawal thresholds compared to WT mice. From day three after SNI both genotypes developed mechanical and heat hypersensitivity, without intergroup differences. As supported by the results of three behavioral tests, no relevant differences were found for anxiety-like behavior after SNI in B7-H1 ko and WT mice. Also, there was no indication of depression-like behavior after SNI or any effect of SNI on cognition in both genotypes. The injured nerves of B7-H1 ko and WT mice showed higher miR-21 expression and invasion of macrophages and T cells 7 days after SNI without intergroup differences. Perineurial miR-21 inhibitor injection reversed SNI-induced mechanical and heat hypersensitivity in old B7-H1 ko and WT mice.
This study reveals that reduced mechanical thresholds and heat withdrawal latencies are associated with miR-21 induction in the tibial and common peroneal nerve after SNI, which can be reversed by perineurial injection of a miR-21 inhibitor. Contrary to expectations, miR-21 expression levels were not higher in B7-H1 ko compared to WT mice. Thus, the B7-H1 ko mouse may be of minor importance for the study of miR-21 related pain. However, these results spot the contribution of miR-21 in the pathophysiology of neuropathic pain and emphasize the crucial role of miRNA in the regulation of neuronal and immune circuits that contribute to neuropathic pain.
N2  - Die Beteiligung von microRNA (miRNA) an der Genregulation immunologischer und neuronaler Prozesse und deren Rolle als Schlüsselelement in der Pathophysiologie von neuropathischem Schmerz gewinnt zunehmend an Bedeutung. miR-21 ist ein vielversprechender Kandidat, der sowohl das Immunsystem, als auch das nozizeptive System beeinflusst. Um die pathophysiologische Rolle von miR-21 bei neuropathischem Schmerz besser zu verstehen wurden Mäuse mit B7 homolog 1 Defizienz (B7-H1 ko), einem immunsupprimierendem Protein, untersucht. Eine frühere Studie zeigte eine Hochregulierung von miR-21 in murinen Lymphozyten.
Junge (8 Wochen), mittelalte (6 Monate) und alte (12 Monate) B7-H1 ko Mäuse und Wildtypwurfgeschwister (WT) erhielten eine spared nerve injury (SNI) als neuropathischem Schmerzmodell. Es wurden thermische Rückzugslatenzen und mechanische Rückzugsschwellen bestimmt. Des weiteren wurde sowohl das Angstverhalten, das depressive Verhalten, als auch das kognitive Verhalten untersucht. Um die relative Expression von miR-21 in den peripheren Nerven, den Spinalganglien und in den weißen Blutzellen zu verschiedenen Zeitpunkten zu bestimmen, wurde die quantitative real time PCR angewandt. 
Naive B7-H1 ko Mäuse zeigten mit zunehmendem Alter eine mechanische Hyposensitivität. Bereits 3 Tage nach SNI entwickelten beide Genotypen eine Überempfindlichkeit gegenüber Hitze und mechanischer Stimulation. In drei durchgeführten Verhaltenstests konnten keine relevanten Unterschiede im Angstverhalten nach SNI von B7-H1 ko und WT Mäusen festgestellt werden. Bei beiden Genotypen gab es weder Hinweise auf depressives Verhalten nach SNI, noch wurde das kognitive Verhalten durch SNI beeinträchtigt. Die verletzen Nerven der B7-H1 ko und WT Mäuse zeigten 7 Tage nach SNI eine höhere miR-21 Expression und eine Invasion durch Makrophagen und T-Zellen ohne Gruppenunterschiede. Die perineurale Injektion eines miR-21 Inhibitors konnte die durch SNI induzierte mechanische und thermische Hypersensitivität lindern. 
Diese Studie zeigt, dass der Anstieg von miR-21 im N. tibialis und N. peroneus communis mit reduzierten Rückzugsschwellen gegen mechanische Reize und verkürzten Wegzugslatenzen bei Hitzestimulation einhergeht, welche durch perineurale Injektion eines miR-21 Inhibitors verringert werden können. Entgegen der Erwartungen zeigten B7-H1 ko Mäuse im Vergleich zu WT Mäusen keine erhöhte miR-21 Expression und sind daher möglicherweise von geringer Bedeutung für die Untersuchung von miR-21 assoziiertem Schmerz. Jedoch bekräftigen diese Ergebnisse eine Beteiligung von miR-21 an der Pathophysiologie von neuropathischem Schmerz und bestätigen die wichtige Rolle von miRNA bei der Regulation von neuronalen und immunologischen Prozessen, die zu neuropathischem Schmerz beitragen.
KW  - neuropathic pain
KW  - inflammation
KW  - B7-H1
KW  - immune system
KW  - neuropathic pain
KW  - miRNA
KW  - miR-21
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-156004
ER  - 
TY  - JOUR
A1  - Hofmann, Sigrun Ruth
A1  - Böttger, Fanny
A1  - Range, Ursula
A1  - Lück, Christian
A1  - Morbach, Henner
A1  - Girschick, Hermann Joseph
A1  - Suttorp, Meinolf
A1  - Hedrich, Christian Michael
T1  - Serum interleukin-6 and CCL11/eotaxin may be suitable biomarkers for the diagnosis of chronic nonbacterial osteomyelitis
JF  - Frontiers in Pediatrics
N2  - Objectives: Chronic recurrent multifocal osteomyelitis (CRMO), the most severe form of chronic nonbacterial osteomyelitis (CNO), is an autoinflammatory bone disorder. In the absence of diagnostic criteria or biomarkers, CNO/CRMO remains a diagnosis of exclusion. The aim of this study was to identify biomarkers for diagnosing multifocal disease (CRMO).

Study design: Sera from 71 pediatric CRMO patients, 11 patients with osteoarticular infections, 62 patients with juvenile idiopathic arthritis (JIA), 7 patients with para-infectious or reactive arthritis, and 43 patients with acute leukemia or lymphoma, as well as 59 healthy individuals were collected. Multiplex analysis of 18 inflammation- and/or bone remodeling-associated serum proteins was performed. Statistical analysis included univariate ANOVA, discriminant analysis, univariate receiver operating characteristic (ROC) analysis, and logistic regression analyses.

Results: For 14 of 18 blood serum proteins, significant differences were determined between CRMO patients, at least one alternative diagnosis, or healthy controls. Multi-component discriminant analysis delivered five biomarkers (IL-6, CCL11/eotaxin, CCL5/RANTES, collagen Iα, sIL-2R) for the diagnosis of CRMO. ROC analysis allowed further reduction to a core set of 2 biomarkers (CCL11/eotaxin, IL-6) that are sufficient to discern between CRMO, healthy controls, and alternative diagnoses.

Conclusion: Serum biomarkers CCL11/eotaxin and IL-6 differentiate between patients with CRMO, healthy controls, and alternative diagnoses (leukemia and lymphoma, osteoarticular infections, para-infectious arthritis, and JIA). Easily accessible biomarkers may aid in diagnosing CRMO. Further studies testing biomarkers in larger unrelated cohorts are warranted.
KW  - medicine
KW  - chronic nonbacterial osteomyelitis
KW  - chronic recurrent multifocal osteomyelitis
KW  - inflammation
KW  - biomarker
KW  - autoinflammation
KW  - diagnosis
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-172744
VL  - 5
ER  - 
TY  - JOUR
A1  - Koeniger, Tobias
A1  - Kuerten, Stefanie
T1  - Splitting the "unsplittable": Dissecting resident and infiltrating macrophages in experimental autoimmune encephalomyelitis
JF  - International Journal of Molecular Sciences
N2  - Macrophages predominate the inflammatory landscape within multiple sclerosis (MS) lesions, not only regarding cellularity but also with respect to the diverse functions this cell fraction provides during disease progression and remission. Researchers have been well aware of the fact that the macrophage pool during central nervous system (CNS) autoimmunity consists of a mixture of myeloid cells. Yet, separating these populations to define their unique contribution to disease pathology has long been challenging due to their similar marker expression. Sophisticated lineage tracing approaches as well as comprehensive transcriptome analysis have elevated our insight into macrophage biology to a new level enabling scientists to dissect the roles of resident (microglia and non-parenchymal macrophages) and infiltrating macrophages with unprecedented precision. To do so in an accurate way, researchers have to know their toolbox, which has been filled with diverse, discriminating approaches from decades of studying neuroinflammation in animal models. Every method has its own strengths and weaknesses, which will be addressed in this review. The focus will be on tools to manipulate and/or identify different macrophage subgroups within the injured murine CNS.
KW  - CNS
KW  - distinction
KW  - experimental autoimmune encephalomyelitis
KW  - inflammation
KW  - macrophages
KW  - markers
KW  - microglia
KW  - monocytes
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285067
SN  - 1422-0067
VL  - 18
IS  - 10
ER  - 
TY  - JOUR
A1  - Schmid, Tobias
A1  - Falter, Lena
A1  - Weber, Sabine
A1  - Müller, Nils
A1  - Molitor, Konstantin
A1  - Zeller, David
A1  - Weber-Steffens, Dorothea
A1  - Hehlgans, Thomas
A1  - Wajant, Harald
A1  - Mostböck, Sven
A1  - Männel, Daniela N.
T1  - Chronic inflammation increases the sensitivity of mouse Treg for TNFR2 costimulation
JF  - Frontiers in Immunology
N2  - TNF receptor type 2 (TNFR2) has gained attention as a costimulatory receptor for T cells and as critical factor for the development of regulatory T cells (Treg) and myeloid suppressor cells. Using the TNFR2-specific agonist TNCscTNF80, direct effects of TNFR2 activation on myeloid cells and T cells were investigated in mice. \(In\) \(vitro\), TNCscTNF80 induced T cell proliferation in a costimulatory fashion, and also supported \(in\) \(vitro\) expansion of Treg cells. In addition, activation of TNFR2 retarded differentiation of bone marrow-derived immature myeloid cells in culture and reduced their suppressor function. \(In\) \(vivo\) application of TNCscTNF80-induced mild myelopoiesis in naïve mice without affecting the immune cell composition. Already a single application expanded Treg cells and improved suppression of CD4 T cells in mice with chronic inflammation. By contrast, multiple applications of the TNFR2 agonist were required to expand Treg cells in naïve mice. Improved suppression of T cell proliferation depended on expression of TNFR2 by T cells in mice repeatedly treated with TNCscTNF80, without a major contribution of TNFR2 on myeloid cells. Thus, TNFR2 activation on T cells in naïve mice can lead to immune suppression \(in\) \(vivo\). These findings support the important role of TNFR2 for Treg cells in immune regulation.
KW  - molecular medicine
KW  - inflammation
KW  - immune regulation
KW  - costimulation
KW  - MDSC
KW  - TNFR2
KW  - regulatory T cell
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-173259
VL  - 8
ER  - 
TY  - JOUR
A1  - Oehler, Beatrice
A1  - Mohammadi, Milad
A1  - Perpina Viciano, Cristina
A1  - Hackel, Dagmar
A1  - Hoffmann, Carsten
A1  - Brack, Alexander
A1  - Rittner, Heike L.
T1  - Peripheral interaction of Resolvin D1 and E1 with opioid receptor antagonists for antinociception in inflammatory pain in rats
JF  - Frontiers in Molecular Neuroscience
N2  - Antinociceptive pathways are activated in the periphery in inflammatory pain, for instance resolvins and opioid peptides. Resolvins are biosynthesized from omega-3 polyunsaturated fatty acids such as eicosapentaenoic acid and docosahexaenoic acid. Resolvin D1 (RvD1) and resolvin E1 (RvE1) initiate the resolution of inflammation and control of hypersensitivity via induction of anti-inflammatory signaling cascades. RvD1 binds to lipoxin A4/annexin-A1 receptor/formyl-peptide receptor 2 (ALX/FPR2), RvE1 to chemerin receptor 23 (ChemR23). Antinociception of RvD1 is mediated by interaction with transient receptor potential channels ankyrin 1 (TRPA1). Endogenous opioid peptides are synthesized and released from leukocytes in the tissue and bind to opioid receptors on nociceptor terminals. Here, we further explored peripheral mechanisms of RvD1 and chemerin (Chem), the ligand of ChemR23, in complete Freund’s adjuvant (CFA)-induced hindpaw inflammation in male Wistar rats. RvD1 and Chem ameliorated CFA-induced hypersensitivity in early and late inflammatory phases. This was prevented by peripheral blockade of the μ-opioid peptide receptor (MOR) using low dose local naloxone or by local injection of anti-β-endorphin and anti-met-enkephalin (anti-ENK) antibodies. Naloxone also hindered antinociception by the TRPA1 inhibitor HC-030031. RvD1 did not stimulate the release of β-endorphin from macrophages and neutrophils, nor did RvD1 itself activate G-proteins coupled MOR or initiate β-arrestin recruitment to the membrane. TRPA1 blockade by HC-030031 in inflammation in vivo as well as inhibition of the TRPA1-mediated calcium influx in dorsal root ganglia neurons in vitro was hampered by naloxone. Peripheral application of naloxone alone in vivo already lowered mechanical nociceptive thresholds. Therefore, either a perturbation of the balance of endogenous pro- and antinociceptive mechanisms in early and late inflammation, or an interaction of TRPA1 and opioid receptors weaken the antinociceptive potency of RvD1 and TRPA1 blockers.
KW  - transient receptor potential channels
KW  - pain behavior
KW  - resolvin
KW  - opioid receptors
KW  - opioid peptides
KW  - inflammation
KW  - animals
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158642
VL  - 10
IS  - 242
ER  - 
TY  - JOUR
A1  - Schuhmann, Michael K.
A1  - Fluri, Felix
T1  - Effects of fullerenols on mouse brain microvascular endothelial cells
JF  - International Journal of Molecular Sciences
N2  - Fullerenols, water-soluble C60-fullerene derivatives, have been shown to exert neuroprotective effects in vitro and in vivo, most likely due to their capability to scavenge free radicals. However, little is known about the effects of fullerenols on the blood–brain barrier (BBB), especially on cerebral endothelial cells under inflammatory conditions. Here, we investigated whether the treatment of primary mouse brain microvascular endothelial cells with fullerenols impacts basal and inflammatory blood–brain barrier (BBB) properties in vitro. While fullerenols (1, 10, and 100 µg/mL) did not change transendothelial electrical resistance under basal and inflammatory conditions, 100 µg/mL of fullerenol significantly reduced erk1/2 activation and resulted in an activation of NFκB in an inflammatory milieu. Our findings suggest that fullerenols might counteract oxidative stress via the erk1/2 and NFκB pathways, and thus are able to protect microvascular endothelial cells under inflammatory conditions.
KW  - mouse brain microvascular endothelial cell cultur
KW  - adhesion molecules
KW  - fullerenes
KW  - blood-brain barrier
KW  - inflammation
KW  - tight junctions
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158072
SN  - 1422-0067
VL  - 18
IS  - 8
ER  -