Some Effects of X-irradiation on the Plasma Corticosterone, Adrenal Weights, and Differential Leukocyte Count in the Rat

Gaugl, John F.

08 1900

The purpose of the present study was twofold: (1) to determine if X-irradiation can be considered a direct stress agent, and if so, to what extent it differs from other stressors; and (2) to further elucidate the role of the adrenal cortex in the radiation syndrome by determining the more immediate responses of this system to X-irradiation.

X-irradiation

plasma corticosterone

adrenal weights

differential leukocyte count

rats

Immunomodulation by Shark Cartilage Extracts

Merly, Liza

12 July 2011

The immune system is composed of innate and adaptive mechanisms. Innate immune responses are significantly modulated by immunomodulatory factors that act through the induction of specific patterns of cytokine production in responding cells. Human leukocytes have been shown to respond to substance(s) present in acid extracts of commercial shark cartilage (SC). Shark cartilage is a food supplement taken by consumers as a prophylaxis and for the treatment of conditions ranging from arthritis to cancer. No reliable scientific evidence in the literature supports the alleged usefulness of shark cartilage supplements, but their use remains popular. Cartilage extracts exhibit immunomodulatory properties by inducing various inflammatory, Th1-type cytokines and potent chemokines in human peripheral blood leukocytes (HPBL) in vitro. The objectives of the study were to (1) to determine the nature of the active component(s), (2) to define the scope of cellular response to SC extract, and (3) to elucidate the molecular mechanisms underlying bioactivity. Results showed that there are at least two cytokine-inducing components which are acid stable. One anionic component has been identified as a small (14-21 kDa) glycoprotein with at least 40% carbohydrate content. Shark cartilage stimulated HPBL to produce cytokines resembling an inflammatory, Th1 polarized response. Leukocyte-specific responses consist of both initial cytokine responses to SC directly (i.e., TNF-a) and secondary responses such as the IFN-γ response by lymphocytes following initial SC stimulation. Response of RAW cells, a murine macrophage cell line, indicated that TNF-α could be induced in macrophages of another mammalian species in the absence of other cell types. The results suggest that the human monocyte/macrophage is most likely to be the initial responding cell to SC stimulation. Stimulation of cells appears to engage at least one ligand-receptor interaction with TLR 4, although the role of TLR 2 cannot be ruled out. Initial activation is likely followed by the activation of the JNK and p38 MAPK signal transduction pathways resulting in activation, release, and translocation of transcription factor nuclear factor κB (Nf-kB). This dissertation research study represents the first in-depth study into characterizing the bioactive component(s) of commercial shark cartilage responsible for its immunomodulating properties and defining cellular responses at the molecular level.

shark

cartilage

cytokine

glycoprotein

innate immunity

leukocyte

arthritis

The mode of action of the synthetic peptides Os and Os-C derived from the soft tick Ornithodoris Savignyi

Taute, Helena

January 2017

Antimicrobial peptides (AMPs) have been identified as important therapeutic agents that can be developed as new multifunctional antibiotic compounds, which may address antibiotic resistance. AMPs have a wide range of bioactivities, including antimicrobial, antioxidant, anti-inflammatory and anticancer properties. Os and Os-C (a derivative of Os, lacking cysteine residues) are two synthetic AMPs derived from the tick defensin OsDef2 which have been shown to have antibacterial, antioxidant and anti-inflammatory activity. Differences in bacterial killing times between these peptides indicate differences in the modes of bacterial killing. For the further development of Os and Os-C for therapeutic application, the aim of this study was to establish the mode of bacterial killing, to determine if these peptides are cytotoxic to human erythrocytes and leukocytes. Lastly, to determine if these peptides have additional beneficial cellular effects such as antioxidant activity. Ultrastructural analysis with electron microscopy techniques revealed that both peptides adversely affected the membranes and intracellular structures of both Gram-negative Escherichia coli and Gram-positive Bacillus subtilis bacteria. Effects included membrane ruffling, cytoplasmic retraction, intracellular granulation and the formation of dense fibres. At the minimum bactericidal concentrations (MBCs) of 0.77 μM for Os and 1.74 μM for Os-C membrane permeabilisation measured with the SYTOX green assay was found not to be the principle mode of action. In stationary phase bacteria, fluorescent triple staining showed that both peptides caused permeabilisation. Studies using fluorescently labelled peptides revealed that the membrane penetrating activities of Os and Os-C were similar to buforin II, a cell-penetrating peptide. Os was able to enter stationary phase E. coli and B. subtilis while Os-C was unable to enter E. coli cells and accumulated on B. subtilis septa. Using plasmid binding and fluorescence displacement assays both peptides could bind DNA, while a dosage effect was only observed for Os. Evaluation of cytotoxicity revealed that Os and Os-C caused no erythrocyte haemolysis or changes to erythrocyte morphology. Only the highest concentration of Os (100 μM), which is 130 fold greater than the MBC for E. coli and B. subtilis, caused cellular damage to peripheral mononuclear (MN) and polymorphonuclear (PMN) cells. In contrast, Os-C caused leukocyte activation identified by associated morphological features and reactive oxygen species (ROS) formation. Chemical and erythrocyte antioxidant assays indicated that both Os and Os-C had antioxidant activity. Both peptides provided extracellular protection of erythrocytes against 2,2'-azobis(2-amidinopropane) dihydrochloride induced oxidative damage. In MN and PMN cells Os showed low levels of antioxidant activity while Os-C had minimal activity. In conclusion, both peptides showed a dual mechanism of bacterial killing, targeting both the membrane and intracellular elements. Os had a predominant membrane effect while Os-C targeted the septa of B. subtilis and had a higher affinity for DNA. Cytotoxicity in erythrocytes and leukocytes was minimal. In addition, Os exhibited antioxidant properties while Os-C caused leukocyte activation. Both peptides have been identified as promising therapeutic agents although activity in plasma and the effect on coagulation must still be determined. / Thesis (PhD)--University of Pretoria, 2017. / Anatomy / PhD / Unrestricted

UCTD

Antimicrobial peptide (AMP)

Mechanism of action

Antioxidant

Leukocyte activation

Morphometric determination of endometrial leukocyte migration during different stages of the equine oestrous cycle

Gerber, David

27 May 2008

Uterine defences against bacterial challenge are more efficient during oestrus than during dioestrus. The exact reasons and mechanisms responsible for this difference are, however, still incompletely understood. The leukocyte reaction is one of the defence mechanisms that has been cited as being able to respond better to a bacterial challenge during oestrus than during dioestrus. The aim of the present study was to test the hypothesis that the magnitude of endometrial leukocyte migration following the instillation of semen into the uterine lumen is greater during oestrus than during dioestrus. Eight Nooitgedacht mares of normal fertility, aged between 8 and 16 years (11.5 ± 2.7; mean ± SD), were used in the study. Each mare received a different treatment during each of four oestrous cycles, with a rest cycle after each treatment. Two treatments were performed during dioestrus and two during oestrus. One treatment for each stage of the cycle was a control treatment without challenge to the endometrium. At time zero of challenged cycles a single aliquot of 13 ml raw semen, frozen-thawed without addition of any cryoprotectant or extender, was instilled into the uterus. An endometrial biopsy was taken 6 and 48 h after time zero and a swab for cytology and culture (if cytology was positive) was collected 48 and 120 h after time zero. An image analyzer was used to record the total number of cells, round cells, neutrophils and eosinophils per unit surface area of epithelium, stratum compactum (SC) and stratum spongiosum (SS). The relative number of round cells, neutrophils and eosinophils were expressed as proportions of the number of each cell type to the total number of cells. The use of an image analyser made the collection of quantitative data from histologic sections possible. However, the operator still had to make some critical decisions, namely to choose the field of the section for analysis and to assign individual cells to a chosen category. The total numbers of cells in the epithelium and the SS were greater during dioestrus than during oestrus, while no such difference could be demonstrated for the SC. The stage of the oestrous cycle had no meaningful influence on any other (measured or calculated) variable. During challenged cycles, absolute and relative numbers of neutrophils were significantly greater in the epithelium, SC and SS than during control cycles. There was an interaction (not always reaching significance) between treatment and time with regard to the absolute and relative numbers of neutrophils in epithelium and SS and round cells in the epithelium. Numbers of neutrophils and round cells were significantly higher 6 h after treatment than 48 h after treatment in challenged cycles, but did not differ during control cycles. During challenged cycles, the stage of the oestrous cycle when treatment occurred had no effect on the duration of the induced endometritis, the occurrence of positive cytology or culture results, or the type of bacteria that were cultured. Regardless of the stage of their cycles when they were challenged, all mares rid themselves of the opportunistic pathogens placed into the uterine lumen within one oestrous cycle. The hypothesis was rejected and it is therefore concluded that the stage of the oestrous cycle did not influence the magnitude of the endometrial leukocyte response to a standardized challenge with semen in these reproductively sound mares. A similar study will be required to test whether this conclusion also holds true for mares that are susceptible to endometritis. / Dissertation (MMedVet (Gyn))--University of Pretoria, 2006. / Production Animal Studies / unrestricted

Endometrial leukocyte migration

Oestrous cycles

Round cells

UCTD

Défenses innées antivirales du poisson zèbre : de la signalisation aux cellules specialisées / Innate antiviral defense of zebrafish : from signalling to specialized cells

Aleksejeva, Elina

20 January 2016

Cette thèse est basée sur deux projets principaux: (1) l'étude de la réponse innée antivirale du poisson zèbre, en particulier des voies de signalisation des interférons de type I et (2) l'étude de leucocytes particuliers localisés au voisinage des neuromastes, structures permettant au poisson de percevoir le flux d'eau qu'il traverse et constituant potentiellement des brèches dans la peau de l'animal. La voie des IFN de type I est le principal composant de l'immunité antivirale innée. Dans cette thèse, deux types de protéines de poisson-zèbre capables d'augmenter l'induction des IFN de type I ont été étudiés. Nous avons montré que les deux orthologues chez le poisson zèbre du facteur de transcription à domaine BTB/POZ nommé PLZF (Promyelocytic leukemia zinc finger) augmentent l'induction de l'Ifn par différents stimuli. Ce travail montre que l'implication de PLZF dans la régulation de la voie IFN est ancienne et peut intervenir à différents niveaux de la voie Ifn. Le second modèle étudié est le gène Ftr83 (finTRIM83), qui appartient à un groupe de TRIM très diversifié et spécifique des poissons. L'expression de cette protéine TRIM induit une très forte induction des Ifn de type I et une protection contre différents virus, via la surexpression de différents ISGs. Ftr83 est exprimé dans la peau et dans les branchies, régions très exposées aux pathogènes, et son niveau d'expression est fortement corrélé au niveau d'expression de l'Ifn. Dans cette thèse, une lignée transgénique où les cellules spécifiquement fluorescentes évoquent des leucocytes localisés à proximité des neuromastes a été étudiée. Ces cellules ont été observées, leurs mouvements suivis et leur transcriptome analysé par séquençage profond après tri au FACS. Cette analyse a identifié des marqueurs typiques de cellules myéloides (macrophages, dendritiques); ces observations sont cohérentes avec l'idée de cellules sentinelles autour des neuromastes. / This thesis is based on the studies of two aspects of innate immunity in zebrafish: 1) proteins involved in the regulation of type I interferon (Ifn) and 2) specialized myeloid cells that patrol neuromasts – mechano-sensory organs embed in the skin that could be pathogen entry sites. In this thesis two different proteins are described for the capability to enhance Ifn production. In one part, two zebrafish orthologues of mammalian transcription factor PLZF (Promyelocytic leukemia zinc finger) are shown to augment type I Ifn and ISG in response to double-stranded RNA viruses. PLZF is a BTB/POZ transcription factor that was recently shown to induce a subset of ISG, in human and mouse. Thus, zebrafish Plzf proteins can operate at multiple steps in the Ifn system. Furthermore, their activity was not dependent on the presence of BTB-domain implying that the underlying mechanism is different from the usual mode of action of BTB/POZ transcription factors. In the second part, fish-specific TRIM ubiquitin ligase - Ftr83 (Fish novel tripartite motif protein 83), mounted a strong anti-viral protection through the upregulation of Ifn. Interestingly a strong correlation between the expression of Ftr83 and Ifn was seen in the gills suggesting that Ftr83 might maintain a low basal level of Ifn signalling in organs constantly exposed to pathogens. In the second part, a GFP reporter transgenic line called medaktin:EGFP has been characterized. It marks leukocytes in the skin surrounding neuromasts. Deep sequencing revealed that these cells express several macrophage and dendritic cell markers, including genes involved in autophagy, microbicidial functions and antigen presentation, thus highlighting them as possible sentinel cells.

Poisson zèbre

Interferon

Neuromaste

Leucocyte

Zebrafish

Interferon

Neuromast

Leukocyte

572.8

Characterizing human receptor-mediated cytotoxicity by staphylococcal bi-component leucocidins in S. aureus pathogenesis

Rutter, Jaime

07 August 2020

Staphylococcus aureus employs an array of virulence factors to aid in its pathogenesis. A subset of cytotoxins termed bi-component leucocidins have been characterized as important determinants in the host-pathogen interaction in S. aureus infections. While they have been studied over a century, bi-component leucocidins’ complex mechanisms in pathogenesis have not been fully elucidated. Secreted as monomers, with the exception of LukAB/GH, many combinations of the S- (HlgA, HlgC, LukE, LukS, LukA/H) and F- (HlgB, LukD, LukF, LukB/G) components have demonstrated cell lysis via pore formation and a magnified proinflammatory response at sublytic concentrations. While studies have described various host cellular receptors and therapeutic strategies to evade leucocidin binding, a common receptor for all the leucocidins has yet to be classified. Challenges in data extrapolation have occurred due to non-native protein expression methods and species specificity of the leucocidin components. In turn, developing successful therapeutic strategies has proven problematic with a need for multimodal therapy. Thus, our studies aimed to clarify the bi-component leucocidins’ cytotoxic effects on multiple subsets of leukocytes using a native protein expression system and to identify a novel human leukocyte receptor common to all leucocidins. Overall, combinations with HlgA and LukE demonstrated the highest degrees of cytotoxicity against PMNs and PBMCs. Coronin 1A was discovered as a common receptor for all cognate pairs of bi-component leucocidins, except LukAB/GH. In conclusion, our results have expanded the knowledge of the cellular targets for leucocidin cytotoxicity and have described a common leucocidin receptor as a potential therapeutic target against the bi-component leucocidins.

bi-component leucocidins

cytotoxin

Staphylococcus aureus

cytotoxicity

leukocyte

receptor

Leukocyte P(2) purinergic receptors: Expression and characterization in Xenopus oocytes

Nuttle, Louise Cathell

January 1994

No description available.

Biology, Animal Physiology

Transcription Inhibitors as Anti-Adhesion Agents

Dagia, Nilesh M.

14 July 2004

No description available.

Engineering, Chemical

Inflamation

Leukocyte

Endothelium

Adhesion

Targeted Drug Delivery

Acute stress as a psycho-physiological adjuvant: cellular and molecular mediators of stress-induced enhancement of primary immunization

Viswanathan, Kavitha

09 March 2005

No description available.

LNs

ACUTE STRESS

STR

antigen

STR animals

leukocyte

cell

Etude de la dynamique de l’axe inhibiteur LILRB2/CMH-I et de sa régulation au cours de l’infection par le VIH/SIV / Dynamic and regulation of LILRB2/MHC-I inhibitory axis during HIV/SIV infection

Alaoui, Lamine

05 December 2017

Les cellules dendritiques classiques (cDC) jouent un rôle crucial dans l’efficacité des réponses immunitaires précoces conduisant au contrôle ou à la persistance virale. A cet égard, il a été montré que l’infection par le VIH induit des dysfonctions des cDC caractérisées par une inhibition de leur capacité à stimuler les cellules T et associées à la progression de la maladie. Parmi les mécanismes moléculaires impliqués dans ces dysfonctions, des études in vitro ont mis en évidence le rôle du récepteur inhibiteur LILRB2. Néanmoins, la dynamique d’expression de LILRB2 ainsi que son rôle dès les premiers stades de l'infection restent à démontrer. Chez des patients en primo-infection VIH-1, nous observons une augmentation de l’expression de LILRB2 et de ses ligands HLA-I à la surface des cDC. Par ailleurs, la cinétique d’expression de LILRB2 et CMH-I au cours de l’infection de macaques cynomolgus par le SIVmac251 montre une augmentation transitoire de l'expression de LILRB2 et du CMH-I sur les cDC du sang et des ganglions lymphatiques dès les premiers jours de l’infection. Parmi les mécanismes qui pourraient être impliqués dans la régulation de l’expression de LILRB2, nos résultats indiquent que la réplication du VIH-1, l'activation de voies TLR7/8 ainsi que la présence d’IL-10 et d’IFN-I induisent une forte expression de LILRB2. Enfin, cette expression exacerbée de LILRB2 sur les cDC semble être spécifique à l'infection par le VIH/SIV. En effet, l’infection de macaques cynomolgus par le virus chikungunya, qui est caractérisée par une réponse immunitaire antivirale robuste aboutissant à un contrôle de la virémie, est associée à une expression diminuée de LILRB2 sur les cDC dès les premiers jours de l’infection. L’ensemble de nos données suggèrent un rôle majeur de l’axe inhibiteur LILRB2/MHC-I dans les mécanismes de dérégulations des cDC qui pourrait participerait à l’inefficacité des réponses immunitaires adaptatives et à la persistance du VIH/SIV. / Conventional dendritic cells (cDCs) play a crucial role in setting up early immune responses leading to viral control or persistence. In this regard, it has been shown that HIV-1 infection induces cDC dysfunctions characterized by inhibitions in their ability to stimulate T-cells and associated with disease progression. In vitro studies have shown the implication of LILRB2 inhibitory receptor in cDC dysfunctions. However, the dynamic of LILRB2 expression and its role in the early stages of infection are yet to be characterized. In primary HIV-1 infected patients, we observe an increased expression of LILRB2 and its ligands, HLA-I, on the surface of cDCs. Kinetics of LILRB2 and MHC-I expressions during SIV infection of Cynomolgus macaques shows a transient increase in LILRB2 and MHC-I expressions on blood and lymph node cDCs during the first days of infection. We also show that HIV replication, activation of TLR7/8 pathways, and presence of IL-10 and IFN-I drive upregulated expression of LILRB2. Finally, this strong induced LILIRB2 expression seems specific to HIV/SIV infections. Indeed, chikungunya virus infection of cynomolgus macaques, which characterized by a robust antiviral immune response leading to viral control, is associated with decreased expression of LILRB2 on cDCs in the first days of infection. Taken together, our data suggest a major role of the LILRB2/HLA-I inhibitory axis, mediating cDC dysfunctions and thus contributing to inefficient adaptive immune responses and viral persistence.

Hiv/siv

Réponse immunitaires Innée

Hiv/siv

Innate Immune Responses