Cloning and Characterization of IL-1β, IL-8, IL-10, and TNFα from Golden Tilefish (<em>Lopholatilus chamaeleonticeps</em>) and Red Snapper (<em>Lutjanus campechanus</em>)

Deak, Kristina L.

04 November 2014

Cytokines are pleiotropic and redundant signaling molecules that govern the inflammatory response and immunity, a critical ecological parameter for organism success and population growth. Produced at the site of injury or pathogen intrusion by a variety of cell types, cytokines mediate cell-signaling in either an autocrine or paracrine manner. The type and magnitude of the cytokine milieu produced subsequently dictates the strength and form of immune response. As the most diverse vertebrate group, with a high sensitivity to contaminants, fish represent an important foci for the evaluation of immune system evolution, function, and alteration upon toxicant exposure. While many cytokines have been identified in teleosts, primary study has been limited to model species (e.g. zebrafish and fugu). However, evidence exists for several variations of cytokine genes within taxa, underscoring the need for species-specific evaluation. In this study, two pro-inflammatory cytokines (IL-1β and TNFα ), one chemokine (IL-8), and one anti-inflammatory cytokine (IL-10) were cloned, sequenced, and characterized for the first time in two commercially relevant Perciformes in the Gulf of Mexico, golden tilefish (Lopholatilus chamaeleonticeps) and red snapper (Lutjanus campechanus). The complete amino acid sequence was obtained and confirmed for IL-β and IL-8 from golden tilefish and for IL-8, IL-10, and TNFα from red snapper, with partial sequences obtained for the remaining proteins. The results indicate high homology among Perciformes for all cytokines studied, but divergence with other teleost orders, and low conservation when compared to birds, amphibians, and mammals. The sequences will be used to create a multi-plexed antibody-based assay for the routine detection of cytokines in teleost serum. This would allow the biochemical response to fish health challenges, such as oil spills and other contamination events, to be monitored at the protein level, building upon the current regime of genetic biomarkers. Thus, this work will aid in the understanding of how oil spills and other contamination events may alter the immune response in fishes.

Cytokine

deepwater horizon

immunotoxicity

oil spill

snapper

tilefish

Genetics

Oceanography

Regulation of allergic asthma by fatty acid-binding proteins

Shum, Bennett Oh Vic, St. Vincent's Clinical School, UNSW

January 2007

Fatty acid-binding proteins are small intracellular proteins with poorly defined functions in intracellular fatty acid transport. The adipocyte fatty acid-binding protein aP2 regulates systemic glucose and lipid metabolism. Using Affymetrix microarrays, we found that aP2, in addition to being abundantly expressed by adipocytes, is also expressed by airway epithelial cells. aP2 expression was markedly increased following stimulation of epithelial cells with the Th2 cytokines IL-4 and IL-13, and downregulated by the Th1 cytokine IFN-gamma. Regulation of aP2 mRNA expression by Th2 cytokines was dependent on STAT6, a transcription factor with a major regulatory role in allergic inflammation. We examined aP2 deficient mice in a model of allergic airway inflammation, and found that infiltration of leukocytes, especially eosinophils, into the airways was highly aP2 dependent. T cell priming and peritoneal allergy was unaffected by aP2 deficiency suggesting that aP2 was acting locally within the lung, and analysis of bone marrow chimeras implicated non-haematopoietic cells, most likely airway epithelial cells, as the site of aP2 action in allergic airway inflammation. Expression of the pro-inflammatory cytokines MCP-1 and IL-6 was impaired in cytokine activated aP2 deficient airway epithelial cells, while levels of the anti-inflammatory arachidonic acid metabolite 15-HETE was increased, providing a mechanism for the reduced airway inflammation in aP2 deficient mice. In addition to the immune functions of aP2, we found that the related fatty acid-binding protein mal1 was also upregulated by IL-4/IL-13 in airway epithelial cells, and mal1 deficient mice were protected against airway eosinophilia. Significantly, in comparison to single aP2 deficiency, mice with combined aP2-mal1 deficiency had augmented protection against airway inflammation, and bone marrow chimera experiments demonstrated that aP2-mal1 deficiency affected both non-haematopoeitic and haematopoeitic cells. In T cell priming experiments, aP2-mal1 deficiency resulted in defective cytokine profiles in antigen recall responses, suggesting compromised sensitisation to antigen as one mechanism for aP2-mal1 action in airway inflammation. Together, our data therefore demonstrates the crucial roles of fatty acid-binding proteins in airway epithelium, T cell priming and airway inflammation, and provides a new link between fatty acid signalling and allergy.

asthma

inflammation

Th2

cytokine

airway

airway epithelium

fatty acid

diet

allergy

Génération et analyse fonctionnelle d'antagonistes de l'oncostatine m et de l'interleukine-31, cytokines impliquées dans l'inflammation cutanée et le développement tumoral

Venereau, Emilie

24 June 2008

L'oncostatine M (OSM) et l'interleukine-31 (IL-31), cytokines de la famille de l'IL-6, sont impliquées dans l'inflammation cutanée associée à des pathologies telles que la dermatite atopique ou le psoriasis. Dans une perspective thérapeutique, deux premières études sont basées sur la génération d'antagonistes agissant comme des récepteurs solubles et destinés à piéger ces cytokines. Afin de disposer d'un nouveau modèle d'étude de l'IL-31 in vivo, nous avons également identifié et cloné cette protéine chez le rat. Dans une dernière étude, nous avons mis en évidence l'implication de l'IL-31 dans le développement tumoral en démontrant son activité cytostatique sur certaines lignées tumorales, de manière similaire à l'OSM. Cette étude nous a également amenés à analyser les voies de signalisation intracellulaires impliquées dans ces effets anti-tumoraux et nous avons ainsi démontré l'activation d'un nouveau facteur de transcription en réponse à ces deux cytokines.

[SDV:IMM] Life Sciences/Immunology

cytokine

antagoniste

interleukine-31

oncostatine M

signalisation

cancer

Thérapie génique non virale de variants du gène du récepteur soluble de type I du TNF-alpha humain. Application à différents modèles de pathologies inflammatoires

Bloquel, Carole

06 1900

Le TNF-α est une cytokine pro-inflammatoire jouant un rôle délétère dans de nombreuses pathologies. Nous nous sommes intéressés à l'inhibition du TNF-α à l'aide de variants du récepteur soluble de type I du TNF-α (hTNFR-Is) administrés par thérapie génique non virale. Trois variants ont été étudiés: un monomère hTNFR-Is, correspondant au récepteur soluble physiologique, une protéine chimérique hTNFR-Is/mIgG1, dont l'efficacité par administration protéique est reconnue, et une forme dimérique obtenue par association de deux fragments hTNFR-Is à l'aide d'un espaceur polyglycine. La vectorisation des plasmides codant ces variants a été étudiée par différentes voies afin d'obtenir un effet systémique (électrotransfert intramusculaire, greffe de cellules autologues), ou un effet local (électrotransfert intra-articulaire (genou de souris), électrotransfert intra-oculaire). L'électrotransfert intramusculaire permettait d'obtenir une expression de protéine à long terme (supérieure à 6 mois) et dose-dépendante. La protéine chimérique était très stable dans la circulation, et était sécrétée à un taux élevé. Cette procédure n'induisait pas de réponse immune contre la protéine transgénique. Nous avons démontré l'obtention, par électrotransfert intra-articulaire, d'une expression dosedépendante du transgène durant deux semaines. Le passage de la protéine dans la circulation était faible, ce qui était l'objectif de cette approche locale. Aux fortes doses, une réponse immune contre la protéine chimérique était observée. Nous avons montré la faisabilité de l'électrotransfert dans un muscle lisse, le muscle ciliaire de l'œil. L'expression obtenue était uniquement localisée dans le muscle ciblé, et la procédure était sûre (pas d'inflammation ni de dommages observables). L'expression du transgène était supérieure à un mois, sans passage de la protéine dans la circulation. L'électrotransfert intramusculaire de variants du hTNFR-Is était efficace (forme chimérique principalement) dans un modèle de polyarthrite rhumatoïde (arthrite expérimentale au collagène) sur les signes cliniques et histologiques de la maladie, par un unique électrotransfert à l'apparition des signes cliniques de la maladie. La comparaison de ce traitement à l'injection répétée de protéine recombinante illustrait la potentialité d'une approche par thérapie génique, de part son efficacité à long terme. Les approches locale et cellulaire restent à tester dans ce modèle. L'électrotransfert intramusculaire de plasmide codant les hTNFR-Is ne permettait pas d'améliorer la récupération des fonctions motrices après un traumatisme crânien, dans un modèle murin, même si la protéine était détectée dans le cerveau, et capable d'inhiber le TNF-α. Ces résultats sont cependant très préliminaires. L'électrotransfert intra-oculaire du plasmide codant la forme chimérique hTNFR-Is/mIgG1 permettait d'inhiber efficacement les signes cliniques et histologiques dans un modèle expérimental d'uvéite (uvéite expérimentale aux endotoxines). Nos résultats mettent en évidence l'efficacité de l'électrotransfert pour délivrer un gène thérapeutique et obtenir une production locale ou systémique (selon la stratégie utilisée) de protéine thérapeutique. Nos résultats illustrent le potentiel de nouvelles cibles (articulation, muscle lisse de l'œil) pour cette technologie, ce qui est encourageant pour l'application future de l'électrotransfert à d'autres tissus/organes cibles et à d'autres pathologies.

[SDV] Life Sciences

Thérapie génique non virale

électrotransfert

Inflammation

Cytokine

TNF-alpha

Polyarthrite rhumatoïde

Uvéite

Traumatisme crânien

Experimental Studies Aiming to Prevent Type 1 Diabetes Mellitus

Rydgren, Tobias

January 2007

<p>Type 1 diabetes mellitus (T1DM) is an autoimmune disease in which T-cells and macrophages invade the islets of Langerhans and selectively destroy the insulin producing β-cells, either directly or through the secretion of e.g. cytokines and nitric oxide (NO). This thesis has studied possible strategies to prevent T1DM. In β-cells and macrophages, NO is produced by inducible nitric oxide synthase (iNOS). </p><p>In the first study, we found that 1400W, a highly selective inhibitor of iNOS could prevent interleukin (IL)-1β induced suppression of rat islet function <i>in vitro</i>, but not diabetes induced by multiple low dose streptozotocin (MLDS), a well established animal model for autoimmune diabetes, <i>in vivo</i>. </p><p>Next, we wanted to test a new type of high affinity blocker of IL-1 action, called IL-1 trap, <i>in vitro</i>. Here we found that an IL-1 trap could prevent the suppressive effects by IL-1β on rat pancreatic islet function. Also, it was sufficient to block the action of IL-1β to prevent islet cell death induced by a combination of IL-1β, tumor necrosis factor-α and interferon-γ.</p><p>In study III, a murine IL-1 trap was found to prolong islet graft survival in the recurrence of disease (ROD) model, a T1DM model that involves syngeneic transplantation of healthy pancreatic islets to diabetic nonobese diabetic mice. Mice treated with IL-1 trap displayed an increased mRNA level of the cytokine IL-4 in isolated spleen cells. This suggests a shift towards Th2-cytokine production, which in part could explain the results. </p><p>Finally, simvastatin an anti-hypercholesterolemic drug that possesses anti-inflammatory properties e.g. by interfering with transendothelial migration of leukocytes to sites of inflammation was studied. We found that the administration of simvastatin could delay, and in some mice prevent, the onset of MLDS-diabetes, and prolong islet graft survival in the ROD model. </p>

Cell biology

Diabetes

Interleukin-1 trap

Simvastatin

Nitric oxide synthase

Cytokine

Pancreatic islet

Streptozotocin

Transplantation

Cellbiologi

Early life cytokines, viral infections and IgE-mediated allergic disease

Larsson, Anna-Karin

January 2006

Background: The reasons why some individuals become IgE-sensitised and allergic are largely unknown, though genetic- and early life environmental factors seem to be of importance. Objective: The overall aim of this thesis was to investigate the relationship between IgE-sensitisation and allergic disease, viral infections, genetic markers and early life cytokines. Results: IgE-sensitised children were found to have reduced numbers of IL-12 producing cord blood mononuclear cells (CBMC), whereas children diagnosed with eczema were found to have reduced numbers of IFN-γ producing CBMC. When dividing the children into early onset of IgE-sensitisation and late onset of IgE-sensitisation we found that the children with an early onset had low numbers of PHA-induced IL-4, IL-12 and IFN-γ secreting CBMC. At the age of two there was a general exacerbation of cytokine responses in the IgE-sensitised children, and the results were similar for the children with early onset IgE-sensitisation. Children with a late onset IgE-sensitisation were more similar to the non-sensitised children, but with a specific increase in the response to cat allergen (IL-4 and IFN-γ). The mothers of IgE-sensitised children, were just as their children, found to have an exaggerated cytokine response as compared to mothers of non-sensitised children. Maternal responses correlated well to the responses seen in the child, though the samples were taken two years after delivery. Cytomegalovirus (CMV) infection in early life was associated to reduced numbers of IL-4, and increased numbers of IFN-γ producing cells at the age of two. No association between CMV seropositivity and IgE-sensitisation was seen. Epstein-Barr virus (EBV) infection, on the other hand, was inversely correlated with IgE –sensitisation, whereas no statistically significant association to cytokine production could be seen. We also showed that the IL12B 1188 C-allele was associated to having a positive skin prick test at the age of two. The rare alleles of the three SNPs investigated (IL12B 1188C, IL12RB1132C and IRF1 1688A) were all associated to low IL-12 production at birth. Conclusions: Our results indicate that allergic diseases are complex traits, and that both the genetic and the cytokine background differ between the different allergic diseases. We can also conclude that the time of onset seem to play a role when investigating IgE-sensitisation, and that perhaps early and late onset IgE-sensitisation have partly different causes. CMV and EBV infection early in life are associated to a protective cytokine profile and to protection from IgE-sensitisation, respectively, again indicating the heterogeneity and the complexity of allergic diseases.

IgE-sensitisation

childhood

cytokine

viral infection

atopy

single nucleotide polymorphism

cord blood

Immunology

Immunologi

Experimental Studies Aiming to Prevent Type 1 Diabetes Mellitus

Rydgren, Tobias

January 2007

Type 1 diabetes mellitus (T1DM) is an autoimmune disease in which T-cells and macrophages invade the islets of Langerhans and selectively destroy the insulin producing β-cells, either directly or through the secretion of e.g. cytokines and nitric oxide (NO). This thesis has studied possible strategies to prevent T1DM. In β-cells and macrophages, NO is produced by inducible nitric oxide synthase (iNOS). In the first study, we found that 1400W, a highly selective inhibitor of iNOS could prevent interleukin (IL)-1β induced suppression of rat islet function in vitro, but not diabetes induced by multiple low dose streptozotocin (MLDS), a well established animal model for autoimmune diabetes, in vivo. Next, we wanted to test a new type of high affinity blocker of IL-1 action, called IL-1 trap, in vitro. Here we found that an IL-1 trap could prevent the suppressive effects by IL-1β on rat pancreatic islet function. Also, it was sufficient to block the action of IL-1β to prevent islet cell death induced by a combination of IL-1β, tumor necrosis factor-α and interferon-γ. In study III, a murine IL-1 trap was found to prolong islet graft survival in the recurrence of disease (ROD) model, a T1DM model that involves syngeneic transplantation of healthy pancreatic islets to diabetic nonobese diabetic mice. Mice treated with IL-1 trap displayed an increased mRNA level of the cytokine IL-4 in isolated spleen cells. This suggests a shift towards Th2-cytokine production, which in part could explain the results. Finally, simvastatin an anti-hypercholesterolemic drug that possesses anti-inflammatory properties e.g. by interfering with transendothelial migration of leukocytes to sites of inflammation was studied. We found that the administration of simvastatin could delay, and in some mice prevent, the onset of MLDS-diabetes, and prolong islet graft survival in the ROD model.

Cell biology

Diabetes

Interleukin-1 trap

Simvastatin

Nitric oxide synthase

Cytokine

Pancreatic islet

Streptozotocin

Transplantation

Cellbiologi

White Spot Syndrome Virus Interaction with a Freshwater Crayfish

Jiravanichpaisal, Pikul

January 2005

Viruses are very abundant in water and hence diseases caused by viruses are common in marine organisms. These diseases create great problems for the commercial farming of crustaceans and mussels. One of the most common and most disastrous diseases for shrimp is caused by the white spot syndrome virus (WSSV), which is spread all around the world and also is infecting many different species of crustaceans including freshwater crayfish. Although during recent years knowledge has been gathered on the ways in which invertebrates defend themselves against bacteria and fungi virtually nothing is known about the defence processes elicited by virus. The aim of this work was to develop a model to use for studies of virus-host interactions in vivo and in vitro. Temperature was found to be important for the virus infectivity and at lower temperature the virus apparently did not replicate, but if animals kept at low temperature for more than 40 days were transferred to higher temperatures they died quickly due to an increased virus replication. In crayfish infected with the virus it was found that hemocytes did not degranulate and the melanization reaction was also inhibited in the hemocyes. Thus it is apparent that this virus interacts with the immune system and hemocytes in particular and to be able to study this in some greater detail it was necessary to develop a cell culture to study virus-host interactions at the molecular level. Hence, we have developed a stem cell culture from the hematopoietic tissue (hpt) that will differentiate and mature into hemocytes and which can be used to replicate the WSSV in the presence of an endogenous cytokine, astakine. Astakine is the first cytokine like-factor described which is directly involved in hematopoiesis in an invertebrate.

Biology

WSSV

crayfish

hematopoietic tissue

cytokine

innate immunity

hemocytes

Biologi

Biology

Biologi

Plasmin : a potent pro-inflammatory factor

Guo, Yongzhi

January 2008

Plasmin, the central molecule of the plasminogen activator system, is a broad-spectrum serine protease. Plasmin is important for the degradation of fibrin and other components of the extracellular matrix (ECM) during a number of physiological and pathological processes. The aim of this thesis was to elucidate the functional roles of plasmin during pathological inflammation and infection in autoimmune and non-autoimmune diseases. For this purpose, mouse models of rheumatoid arthritis (RA), bacterial arthritis, infection, and sepsis have been used. Previous studies from our laboratory have shown that plasminogen-deficient mice are resistant to the development of collagen type II-induced arthritis (CIA). In contrast, others have shown that plasmin plays a protective role in antigen-induced arthritis (AIA). To investigate the contrasting roles of plasminogen deficiency in models of CIA and AIA, a new animal model of arthritis called local injection-induced arthritis (LIA) was developed. In this model, we replaced methylated bovine serum albumin, which is normally used as an immunogen in the AIA model, with collagen type II (CII) to induce arthritis. When wild-type and plasminogen-deficient mice were injected intra-articularly with CII or 0.9% NaCl following CIA induction, plasminogen-deficient mice developed typical CIA, but the disease was less severe than in wild-type mice and was restricted to the injected joints. When the AIA model was used, plasminogen-deficient mice developed a much more severe arthritis than the wild-type mice. These results indicate that both the antigen and joint trauma caused by the local injection are critical to explaining the contrasting roles of plasminogen deficiency in CIA and AIA. This indicates that CIA and AIA have distinct pathogenic mechanisms and plasmin plays contrasting roles in different types of arthritis models. To study the functional roles of plasmin in the host inflammatory response during infectious arthritis, a Staphylococcus aureus-induced bacterial arthritis model was established. When wild-type mice were injected intra-articularly with 1 × 106 colony-forming units (CFU) of S. aureus per joint, all the bacteria were completely eliminated from the injected joints in 28 days. However, in the plasminogen-deficient mice, the S. aureus counts were 27-fold higher at day 28 than at day 0. When human plasminogen was given to the plasminogen-deficient mice daily for 7 days, the bacterial clearance was greatly improved and the necrotic tissue in the joint cavity was also completely eliminated. Supplementation of plasminogen-deficient mice with plasminogen also restored the expression level of interleukin-6 (IL-6) in the arthritic joints. In summary, plasmin has protective roles during S. aureus-induced arthritis by enhancing cytokine expression, removing necrotic tissue, and mediating bacterial killing and inflammatory cell activation. The functional roles of plasmin during infection and sepsis were also studied in mice. Infection was induced by injecting 1 × 107 CFU of S. aureus intravenously and the sepsis model was induced by injecting 1.6 × 108 CFU of S. aureus. In the infection model, the wild-type mice had a 25-day survival rate of 86.7%, as compared to 50% in the plasminogen-deficient group. However, when sepsis was induced, the average survival for plasminogen-deficient mice was 3 days longer than for wild-type mice. Twenty-four hours after the induction of sepsis, the serum levels of IL-6 and IL-10 as well as the bacterial counts in all organs investigated were significantly higher in wild-type mice than in plasminogen-deficient mice. In wild-type mice, blockade of IL-6 by intravenous injection of anti-IL-6 antibodies significantly prolonged the onset of mortality and improved the survival rate during sepsis. These data indicate that plasmin plays different roles during infection and sepsis. Furthermore, plasmin appears to be involved in the regulation of inflammatory cytokine expression during sepsis. Taken together, our data indicate that plasmin plays multifunctional pro-inflammatory roles in different autoimmune and non-autoimmune diseases. The pro-inflammatory roles of plasmin include activation of inflammatory cells, regulation of cytokine expression, and enhancement of the bacterial killing ability of the host.

plasmin

inflammation

rheumatoid arthritis

bacterial arthritis

infection

sepsis

cytokine

signal transduction

Pathology

Patologi

The bank vole (Myodes glareolus) – a novel animal model for the study of diabetes mellitus

Blixt, Martin

January 2010

The bank vole (Microtus arvalis) develops glucose intolerance both when kept in captivity and in the wild state. Glucose intolerant bank voles kept in captivity exhibited polydipsia, polyuria, hyperglycemia, hyperinsulinemia, islet autoantibodies and a markedly changed islet structure resembling so–called hydropic degeneration. Islets showing hydropic degeneration have reduced β–cell mass. However, the relative islet size to total pancreas area was not changed. Pancreatic islet isolated from glucose intolerant bank voles had an altered islet function showing signs of being exposed to an increased functional demand on their β–cells. Also, islets from male bank voles seem more affected than the islets from females. Islets isolated from glucose tolerant male bank voles cultured for 5 days at 28 mM glucose did not reveal any change in insulin gene expression or insulin biosynthesis rate. However, islets from female bank voles displayed a glucose concentration dependent response. This suggests that there is gender difference in that, islets of female more easily than islets of males adapt to elevated glucose concentration. Furthermore, islets isolated from glucose tolerant males had reduced insulin gene expression after exposure to proinflammatory cytokines for 48 hrs. This effect seemed to be NO-independent since only a minor elevation of nitrite accumulation in the medium was seen, and the use of iNOS inhibitor could not counteract the cytokine effect. The observed response seen in bank vole islets upon exposure to various glucose concentrations or proinflammatory cytokines is similar to those seen in studies of human islets. The bank vole may therefore represent a novel animal model for the study of diabetes. An unresolved issue is the role of the Ljungan virus which is found in the bank vole colony. Bank voles developing glucose intolerance display features of both human type 1 and type 2 diabetes, where environmental factors seems to play an important role as determinant. Our findings suggest that bank voles bred in the laboratory may develop more of a type 2 diabetes. However, bank voles caught in nature instead may rather develop a type 1 form of the disease.

Bank vole

pancreatic islets

diabetes mellitus

hydropic degeneration

proinflammatory cytokine

Diabetology

Diabetologi

Endocrinology

Endokrinologi