Dissertations / Theses on the topic 'The immune response of T lymphocyte cell'
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Vargas, Cuero Ana Laura. "Study of CD8'+T lymphocyte responses against human herpesviruses." Thesis, Open University, 2000. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.342897.
Full textDebock, Isabelle. "Study of the development of Th17-type immune response in early life." Doctoral thesis, Universite Libre de Bruxelles, 2012. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/209700.
Full textRécemment, de nouveaux lymphocytes T auxiliaires ont été décrits, les lymphocytes Th17, producteurs d’IL-17A, d’IL-17F et d’IL-22, d’une part, et les lymphocytes Tfh, sécrétant de l’IL-21 et exprimant CXCR5, ICOS et PD-1, d’autre part. La différenciation des lymphocytes Th17 dépend de la présence d’IL-6 ou d’IL-21 et de TGF-β, et est inhibée par l’IL-4 ;tandis que les lymphocytes Tfh sont induits en présence d’IL-21, d’IL-6 et du répresseur transcriptionnel Bcl6. Alors que les lymphocytes Th17 sont associés à des réponses inflammatoires par le recrutement de neutrophiles, les lymphocytes Tfh aident les lymphocytes B à produire des anticorps de haute affinité.
L’objectif principal de notre travail est l’étude du développement potentiel de réponses de type Th17 chez le nouveau-né de souris soumis à une stimulation allogénique et au manque d’IL-4. De plus, l’existence potentielle de lymphocytes Tfh induits chez le nouveau-né immunisé avec un vaccin constitué d’ovalbumine de poulet et d’Alum, sera investiguée.
Dans notre modèle de tolérance néonatale, l’immunisation de nouveau-nés BALB/c à l’aide de cellules spléniques semi-allogéniques F1 (AJAX x BALB/c) induit une polarisation de type Th2, associée à l’établissement d’un chimérisme lymphoïde et à l’acceptation d’une greffe de peau présentant les alloantigènes rencontrés à la naissance. Des nouveau-nés soumis à cette immunisation allogénique et à la privation d’IL-4, réalisée par l’utilisation d’anticorps monoclonaux ou de souris IL-4-/-, rejettent de façon aiguë les greffons de peau et présentent une proportion réduite de cellules chimériques. Cette rupture de la tolérance néonatale est associée à l’inhibition de la réponse allospécifique de type Th2 et au développement de lymphocytes Th17 alloréactifs, produisant de l’IL-17A. L’inhibition de la voie Th17 ne conduit toutefois pas à l’acceptation des allogreffes de peau. Par contre, la neutralisation de l’IL-6 ou de l’IL-17A et la réduction du nombre de neutrophiles restaurent la proportion de cellules chimériques présentes dans la rate, démontrant que la réponse de type Th17 allospécifique néonatale contrôle le chimérisme lymphoïde.
En réponse au vaccin OVA-Alum, les nouveau-nés présentent une proportion accrue de lymphocytes Tfh CXCR5+ PD-1+, bien que cette proportion lymphocytaire soit significativement diminuée par rapport aux adultes. Les lymphocytes Tfh néonataux expriment en outre des taux moindres des ARNm d’IL-21, d’IL-4 et de Bcl6, suggérant que la génération de lymphocytes Tfh est altérée en début de vie. En parallèle, les titres et la maturation des anticorps produits suite à la vaccination sont réduits chez les nouveau-nés, en comparaison avec les adultes. Cependant, qu’ils soient déficients en IL-4 ou non, des lymphocytes T CD4+ néonataux activés in vitro en présence d’IL-6 induisent une production d’anticorps par des lymphocytes B compétents, suggérant qu’il n’y a pas de défaut intrinsèque des lymphocytes T du nouveau-né à développer une capacité d’aide aux lymphocytes B.
En conclusion, nous avons montré que la polarisation de type Th2 néonatale inhibe la différenciation de lymphocytes Th17 alloréactifs contrôlant le rejet de cellules allogéniques, un mécanisme pouvant intervenir dans la relation immunitaire entre la mère et l’enfant. Nos résultats indiquent également que le nouveau-né est capable de différencier des lymphocytes Tfh, bien que le développement de ces derniers semble réduit. \
Doctorat en Sciences biomédicales et pharmaceutiques
info:eu-repo/semantics/nonPublished
Galle, Cécile. "Inflammatory and helper T lymphocyte responses in human abdominal aortic aneurysm." Doctoral thesis, Universite Libre de Bruxelles, 2006. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/210815.
Full textAbdominal aortic aneurysm (AAA) is a chronic degenerative disease that usually affects men over 65 years with an estimated prevalence of 5%. Aneurysm rupture represents a catastrophic event which carries a mortality rate of almost 90%. Current therapeutic options for AAAs measuring 5.5 cm in diameter or larger are based on prophylactic surgery, including conventional open reconstruction and endovascular stent-graft insertion. For patients with small asymptomatic AAAs (4.0 up to 5.5 cm in diameter), evidence from two recent large randomized controlled trials indicates no long-term survival benefit from immediate elective surgical repair as compared to imaging surveillance until aneurysm expands to 5.5 cm. This highlights the need for development of novel medical management strategies, including selective pharmacologic approaches, directed at preventing aneurysm expansion. In this regard, it is expected that a detailed knowledge of the pathobiology of human AAA lesion and a better understanding of pathophysiological mechanisms underlying initiation and progression of aneurysmal degeneration, particularly the specific involvement of T lymphocytes, will have special relevance to this challenging issue.
Inflammatory and helper T-cell responses in abdominal aortic aneurysm :controversial issues
Innate and inflammatory responses to endovascular versus open AAA repair. The occurrence of early acute systemic inflammatory responses after conventional open AAA repair is widely recognized and is thought to lead to the development of organ dysfunction and multiple organ failure, responsible for a large proportion of morbidity and mortality associated with aortic surgery. New therapeutic strategies designed to avoid ischemia-reperfusion injury related to aortic cross-clamping and to minimize the degree of tissue damage have thus been developed recently. Specifically, the advent of endovascular techniques has radically extended management options for patients with AAA. Although the method is believed to offer a clear short-term benefit over open repair, notably as regards restricted perioperative haemodynamic parameter fluctuations, reduced blood loss, briefer duration of surgery, shorter hospital stay, and lower 30-day mortality and complication rates, conflicting data are available regarding the exact nature and extent of the inflammatory events arising after such endoluminal procedures ;while several authors have indeed reported that endovascular AAA repair can determine a less intense and extensive inflammatory response, others have unexpectedly observed that the method may elicit a strong inflammatory response, the so-called « postimplantation syndrome ».
Adaptive cellular immune responses in human aneurysmal aortic lesion.
The inflammatory nature of AAA disease has long been suggested by the presence of a great number of CD4+ T lymphocytes in the outer media and adventitia of human AAA lesion. Interestingly, such infiltrating T-cell populations may have significant implications in the process of aneurysm dilation, since cytokines produced by T cells, notably IFN-gamma, have previously been shown to modulate production of matrix-degrading enzymes by resident macrophages and to induce apoptosis of medial SMCs. Through these key pathological mechanisms, T cells could potentially contribute to orchestrate aortic wall connective tissue disordered remodeling and degradation, and promote extensive disruption of elastic media, ultimately leading to aneurysmal degeneration. Nevertheless, despite their relative abundance in human AAA wall tissues, there is limited and controversial information as regards the functional profile of lesional lymphocytes, the exact nature of aortic wall adaptive cellular responses, and the etiologic role of T cells and their cytokines in initiation and progression of the aneurysmal process. Indeed, both Th1-type and Th2-type responses have been identified in human studies and experimental animal models of AAA.
Aims of the work
The main objectives of our work were to explore the innate and adaptive cellular immune responses in human AAA. In the first part of our work, we aimed to examine prospectively innate and inflammatory responses arising in a non-randomised cohort of patients undergoing endovascular versus open AAA repair. In the second part of our work, we focused our efforts on characterizing the nature of adaptive cellular immune responses and the phenotypic and functional repertoire of T cells in human AAA wall tissues obtained from a consecutive series of patients undergoing open AAA repair. Specifically, we sought to determine whether type 1 or type 2 responses occur predominantly in advanced AAA lesion.
Main experimental findings
Limited inflammatory response after endovascular AAA repair. Serial peripheral venous blood samples were collected preoperatively, immediately after declamping or insertion of endograft, and after 1, 3, 6, 12, 24, 48, and 72 hours. We first examined the acute phase reaction and liberation of complement cascade products using turbidimetric method and nephelometry. We found that endovascular repair produced lower postoperative CRP, leucocytosis, neutrophilia, and C3d/C3 ratio as compared to open surgery. We next analyzed surface expression of activation markers on peripheral CD3+ T cells using flow cytometry. We observed a strong upregulation of CD38 after open but not endovascular repair. Analysis of CD69 and CD25 molecules revealed no perioperative fluctuations in any group. We then investigated release of various circulating soluble cell adhesion molecules, proinflammatory cytokines, and chemokines using enzyme-linked immunosorbent assays. We demonstrated that both procedures are characterized by similar increases in ICAM-1 and IL-6 levels. Finally, tendency towards high levels of TNF-alpha and IL-8 was detected in endovascular repair, but data failed to reach statistical significance.
Predominance of type 1 CD4+ T cells in human aneurysmal aortic lesion. We have developed a tissue enzymatic digestion and cell extraction procedure to isolate intact mononuclear cells from aortic wall segments. This original cell isolation protocol enabled us to examine ex vivo the presence, phenotype, and cytokine secretion profile of infiltrating T lymphocytes freshly isolated from human AAA tissues for comparison with their circulating counterparts using flow cytometry. We found that both populations of infiltrating CD4+ and CD8+ T cells display a unique activated memory phenotype, as assessed by an increased expression of CD69 and HLA-DR activation antigens, downregulation of CD62L molecule, and predominant expression of the CD45RO isoform characteristics of memory cells. In addition, we identified the presence in human aneurysmal aortic wall lesion of CD4+ T cells producing high levels of IFN-gamma but not IL-4, reflecting their type 1 nature. In an additional series of experiments, cytokine gene expression was determined in whole aneurysmal and non-diseased aortic samples using LightCycler-based quantitative real-time reverse transcription-polymerase chain reaction. The molecular basis of type 1 or type 2 dominant responses was further specified by analyzing mRNA levels of transcription factors specifically involved in Th1 or Th2 differentiation such as T-bet and GATA-3. We demonstrated that aneurysmal aortic specimens exhibit high transcript levels of IFN-gamma but not IL-4, and consistently overexpressed the IFN-g-promoting cytokine IL-12 and the type 1-restricted transcription factor T-bet, further establishing the prominent type 1 nature of aortic wall responses. Moreover, such selective tissue expression of IL-12 and T-bet in the vessel microenvironment points to a potential role for these signals in directing aortic wall responses towards a type 1 phenotype.
Conclusions
Our findings indicate that endovascular AAA repair is associated with a lesser degree of acute phase reaction, peripheral T-cell activation, and release of complement proteins as compared to conventional open surgery, suggesting that the innate and inflammatory responses to AAA repair are significantly attenuated by the endovascular approach as compared to the traditional open reconstruction. These results support the view that the endoluminal procedure represents an attractive alternative to open surgery for the treatment of large aneurysms. On the other hand, we have demonstrated that Th1 cell infiltrates predominate in human end-stage AAA lesion. These observations are relevant for helping clarify the pathobiology of human AAA tissues and defining prospects for the prevention of aneurysm expansion. Indeed, identification of such infiltrating populations of IFN-gamma-producing CD4+ T cells not only provide new insights into the pathogenesis of the disorder, but could also serve as a basis for the development of novel medical management strategies directed at preventing aneurysm formation and progression, including therapeutic approaches based on the modulation of aortic wall responses and designed to selectively target T-cell activation and cytokine production. In this respect, the present work provides experimental evidence in support of the emerging concept that, although multifactorial, aneurysm disease may be regarded as a Th1-driven immunopathological condition, and suggests that strategies targeting IFN-gamma could be a particularly exciting and fruitful avenue for further investigation. Ongoing clinical and basic research in these areas can be expected to yield design of promising pharmacologic approaches to control AAA expansion. From a clinical perspective, such efforts have the potential to dramatically influence both the outcome and management of this common and life threatening condition.
Doctorat en sciences médicales
info:eu-repo/semantics/nonPublished
Jin, Siya. "Quantitative comparison of the human immunodeficiency virus-1 and Epstein-Barr virus specific cytotoxic T lymphocyte responses." Thesis, Open University, 1995. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.283078.
Full textFulton, Jonathan Reid. "Intestinal and systemic cytotoxic T lymphocyte and humoral immune responses to oral and parenteral reovirus infection." Morgantown, W. Va. : [West Virginia University Libraries], 2006. https://eidr.wvu.edu/etd/documentdata.eTD?documentid=4474.
Full textTitle from document title page. Document formatted into pages; contains xi, 288 p. : ill. Vita. Includes abstract. Includes bibliographical references.
Shi, Zheng Isabelle. "Prolifération et capacité cytotoxique des lymphocytes T infiltrant les tumeurs induites par les cellules malignes autologues de lymphomes B : étude de 85 clones T issus de 9 patients." Université Joseph Fourier (Grenoble ; 1971-2015), 1994. http://www.theses.fr/1994GRE10215.
Full textHuygens, Ariane. "Fetal T cell response to human congenital cytomegalovirus infection." Doctoral thesis, Universite Libre de Bruxelles, 2013. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/209450.
Full textLes lymphocytes T CD4+ Th1 et les lymphocytes T CD8+ cytotoxiques jouent un rôle crucial dans le contrôle des pathogènes intracellulaires dont le HCMV fait partie. La littérature montre une capacité limitée des enfants congénitalement infectés par le HCMV à développer des réponses T CD4+ spécifiques du HCMV. En contraste, des réponses de lymphocytes T CD8+ spécifiques du HCMV ont été rapportées chez des enfants infectés in utero, mais ces réponses n’ont pas été comparées en détails à celles de l’adulte. De plus, notre connaissance des réponses T spécifiques du HCMV durant l’infection primaire par ce virus est limitée. Des études antérieures ont rapporté un défaut de prolifération et de production d’IL-2 des lymphocytes T spécifiques du HCMV chez des adultes avec durant la phase primaire de l’infection, mais les mécanismes restent non-élucidés.
Nous avons caractérisé les réponses de lymphocytes T CD4+ et CD8+ spécifiques du HCMV provenant du sang de cordon de nouveau-nés congénitalement infectés par le HCMV, et nous avons comparé ces réponses à celles de leurs mamans diagnostiquées avec une infection primaire par le HCMV durant la grossesse. En plus, nous avons comparé les réponses T CD4+ et CD8+ de ces mamans à celles d’adultes infectés chroniquement par le virus. Chez les nouveau-nés, nous avons démontré que des lymphocytes T CD4+ de sang de cordon exprimant un phénotype de différentiation spécifique du HCMV (CD27-CD28-) ainsi qu’un phénotype Th1 similaire à celui des cellules maternelles étaient induits in utero lors de l’infection congénitale par le HCMV. De plus, la détection d’expansions oligoclonales suggérait fortement une expansion antigène-spécifique de ces cellules. Cependant, les T CD4+ de nouveau-nés présentaient une capacité fortement réduite à produire des cytokines anti-virales (IFN-γ, TNF-α et MIP-1β) en réponse à une stimulation ex vivo avec les antigènes du HCMV, par rapport aux cellules maternelles. Les lymphocytes T (CD27-CD28-) CD4+ de nouveau-nés produisaient également des niveaux plus bas de cytokines antivirales en réponse à des stimulations polyclonales avec l’anti-CD3 et la PMA/ionomycine, suggérant des altérations en amont et en aval de la voie de signalisation du TCR. Nos résultats suggèrent que ces altérations pourraient impliquer la diminution de l’expression de molécules impliquées dans cette voie de signalisation. De la même manière, nous
avons montré que chez le nouveau-né, la fonction des T CD8+ spécifiques du HCMV était altérée par rapport à celle de l’adulte. Nous avons observé des proportions similaires de T CD8+ (CD27-CD28-) chez les nouveau-nés et les adultes. De plus, l’analyse du répertoire du TCR Vβ de ces cellules par séquençage haut-débit a révélé une capacité similaire à générer un répertoire T diversifié dans les deux groupes. Comme rapporté précédemment, nous avons détecté des fréquences similaires de lymphocytes T CD8+ spécifiques pour l’antigène immunodominant pp65. Cependant, lorsque les stimulations ont été étendues à d’autres antigènes du HCMV, nous avons observé que le répertoire antigénique reconnu par ces cellules était significativement réduit chez les nouveau-nés, en association avec une diminution de la polyfonctionalité et de la production de cytokines par cellule.
Nous avons également montré que, dans une moindre mesure, la fonction des lymphocytes T spécifiques du HCMV était diminuée durant l’infection primaire chez l’adulte. Comme reporté précédemment, les T CD4+ spécifiques du HCMV proliféraient moins et produisaient moins d’IL-2 par rapport à des individus dans la phase chronique de l’infection. Ce défaut de production d’IL-2 affectait à la fois les populations de cellules CD28+ et CD28-, montrant que l’accumulation de lymphocytes T CD4+ ayant perdu l’expression de la molécule CD28 (un signal de co-stimulation important pour la production d’IL-2) est seulement un des facteurs contribuant à la diminution de la production d’IL-2 par les cellules spécifiques du HCMV. En accord avec cette observation, nous avons montré une diminution de la production par cellule d’IFN-γ et de TNF-α touchant également à la fois les populations de T CD4+ CD28+ et CD28- durant la phase primaire de l’infection, un défaut associé avec une avidité fonctionnelle diminuée de ces cellules. De la même manière, la polyfonctionalité et la production de cytokines par cellule des lymphocytes T CD8+ spécifiques du HCMV étaient également diminuées chez les adultes durant la phase d’infection primaire.
En résumé, nos résultats montrent que la fonction des lymphocytes T spécifiques du HCMV de nouveau-nés et d’adultes est altérée durant l’infection primaire par rapport à des individus infectés chroniquement par le virus. Nous montrons que cette régulation fonctionnelle ressemble à l’exhaustion fonctionnelle des lymphocytes T observée durant les infections virales chroniques associées à des charges virales élevées. L’infection primaire par le HCMV est caractérisée par une réplication virale intense qui dure pendant plusieurs mois suivant l’infection. Nous émettons l’hypothèse que les hauts taux de réplication virale observés durant l’infection congénitale et chez l’adulte durant l’infection primaire par le HCMV pourraient interférer avec certaines fonctions des lymphocytes T./Neonates and young infants have a higher susceptibility to infections compared to older infants or adults. This feature is in part attributed to the immaturity of their immune system associated with a limited capacity to mount cellular-mediated immune responses. Congenital human cytomegalovirus (HCMV) infection is the most common cause of congenital infection worldwide and a major cause of hearing loss and mental retardation. In Belgium, antenatal screening of pregnant women for primary HCMV infection offers an opportunity to study neonatal immune responses to the virus and to compare them to those of their mother.
T lymphocytes are major players of the immune system. In particular, Th1 CD4+ T cells and CD8+ cytotoxic T cells play a crucial role in the control of intracellular pathogens, including HCMV infection. Previous literature has reported a limited capacity of infants born with congenital HCMV infection to mount HCMV-specific CD4+ T cell responses. In contrast, fetal antigen-specific CD8+ T cell responses have been reported following in utero HCMV infection, but these responses have not been compared in detail to those of adults with primary infection. In addition, our knowledge regarding adult HCMV-specific T cell responses during primary HCMV infection is limited. Previous studies have reported defective T cell proliferation and IL-2 production in adults with primary HCMV infection, showing that some of the T cell functions are altered during primary infection.
In this study, we have characterized neonatal HCMV-specific CD4+ and CD8+ T cell responses from the cord blood of newborns with congenital HCMV infection, and we have compared these responses to that of their mothers diagnosed with primary HCMV infection during pregnancy. Also, we compared CD4+ and CD8+ T cell responses of adults with primary HCMV infection to that of adults with chronic infection.
In newborns, it was not known if the defective CD4+ T cell responses could be attributed to the absence of HCMV-specific cells or to the induction of dysfunctional cells. We demonstrate that neonatal CD4+ T cells with a differentiation phenotype typical of HCMV infection (CD27-CD28-) and expressing a Th1 phenotype similar to that of maternal cells can differentiate in utero following HCMV infection. In addition, the detection of oligoclonal expansions by spectratyping and flow cytometry analyses strongly suggests antigen-specific responses. However, neonatal CD4+ T cells were markedly less able to produce antiviral cytokines (IFN-γ, TNF-α and MIP-1β) following ex vivo stimulation with HCMV antigens, compared to maternal cells. Also, neonatal CD27-CD28- CD4+ T cells produce lower levels of antiviral cytokines in response to polyclonal stimulations with anti-CD3 and PMA/ionomycin, suggesting alterations up-stream and down-stream of the TCR signaling pathway. Our results suggest that these alterations could involve the down-regulation of the expression of molecules that are part of the TCR signaling pathway. Similarly, we show that the function of
neonatal HCMV-specific CD8+ T cells is impaired compared to adults. Similar proportions of (CD27-CD28-) CD8+ T cells, typical of HCMV infection, were detected in newborns and adults. Analysis of the TCR Vβ repertoire of neonatal and maternal (CD27-CD28-) CD8+ T cells by high-throughput sequencing revealed a similar capacity to generate a diverse clonal repertoire. As previously reported, we detected similar frequencies of HCMV-specific CD8+ T cells specific for the immunodominant viral antigen pp65. However, when extending ex vivo stimulations to other HCMV antigens, we observed that the antigenic repertoire recognized by these cells was significantly reduced in newborns. In addition, neonatal CD8+ T cells had a reduced polyfunctionality and per cell cytokine production.
To a lower extent, the function of adult HCMV-specific T cells was also impaired during primary infection. As previously reported, maternal HCMV-specific CD4+ T cells were markedly less able to produce IL-2 and to proliferate compared to individuals in the chronic stage of the disease. Both CD28+ and CD28- T cell subsets produced decreased levels of IL-2. This observation shows that the accumulation of HCMV-specific CD4+ T cells having lost the expression of the CD28 molecule (an important co-stimulatory signal for IL-2 production) during primary infection is only one of the factors contributing to the decreased IL-2 production. Accordingly, both CD28+ and CD28- CD4+ T cell subsets had a decreased per cell production of IFN-γ and TNF-α during primary HCMV infection. This defect was associated with a lower functional avidity of these cells. Similarly, the polyfunctionality and per cell cytokine production of adult HCMV-specific CD8+ T cells was also impaired compared to adults with chronic infection.
Altogether, our results show that adult and neonatal HCMV-specific T cell responses are impaired during primary infection, compared to individuals with chronic infection. We show that this functional regulation resembles that of functional T cell exhaustion observed during chronic viral infections that are associated with high levels of viral replication. Primary HCMV infection is characterized by an intense viral replication lasting for several months post-infection. We hypothesize that the high levels of viral replication observed during congenital and adult primary HCMV infection could interfere with some of the T cell functions.
Doctorat en Sciences biomédicales et pharmaceutiques
info:eu-repo/semantics/nonPublished
Zuccolotto, Peter. "T-cell development in the Tammar wallaby (Macropus eugenii)." Thesis, View thesis, 2000. http://handle.uws.edu.au:8081/1959.7/391.
Full textZuccolotto, Peter. "T-cell development in the Tammar wallaby (Macropus eugenii)." View thesis, 2000. http://library.uws.edu.au/adt-NUWS/public/adt-NUWS20030828.145055/index.html.
Full textFrenati, Melania. "Role of CYBR, a cytohesin binder and regulator scaffold protein, in cell-mediated immune response in vivo." Doctoral thesis, Università degli studi di Padova, 2013. http://hdl.handle.net/11577/3423114.
Full textCybr (cytohesin binder and regulator) è una proteina adattatrice coinvolta nell’assemblaggio e nel reclutamento di complessi proteici associati con il trafficking intracellulare e la trasduzione del segnale. Grazie alla sua esclusiva espressione in cellule di origine ematopoietica, Cybr ha attirato l’attenzione come potenziale proteina chiave nei meccanismi molecolari che controllano le cellule del sistema immunitario. Cybr interagisce con i membri della famiglia delle citoesine attivanti gli ADP ribosylation factors (ARF), specialmente con citoesina-1, e regola l’adesione citoesina-1 mediata di LFA 1 a ICAM-1. La sua espressione è rapidamente regolata da molte citochine e da altri effettori solubili del sistema immunitario. Alcuni ruoli funzionali proposti per questa molecola sono la partecipazione nella formazione delle vescicole, nel trafficking endocitico, nella regolazione del signaling del TCR e nell’interazione tra cellule dendritiche e cellule T durante la presentazione dell’antigene. Al fine di caratterizzare il ruolo fisiologico di questa molecola in vivo, è stato creato un ceppo di topi deficienti per Cybr. Questi topi, nonostante un normale sviluppo del sistema immunitario, mostrano una ridotta o ritardata capacità di rispondere a diversi stimoli e in condizioni di stress. Questo progetto di ricerca si è prefisso di investigare la funzione biologica di Cybr nella risposta immunitaria cellulo-mediata nei confronti di tumori indotti dal complesso retrovirale costituito dai virus sarcomatogeno e leucemogeno murini di Moloney (M-MSV/MuLV, in seguito indicato come M-MSV). L’inoculo intramuscolare di M-MSV in topi C57BL/6 (B6) immunocompetenti causa lo sviluppo di sarcomi che regrediscono spontaneamente grazie ad una forte risposta immunitaria mediata principalmente da linfociti T citotossici (CTL) specifici per gli antigeni virali. Al contrario, topi Cybr-deficienti inoculati con M-MSV sviluppano tumori di dimensioni maggiori e che regrediscono più lentamente rispetto ai controlli. Per comprendere i motivi di questo diverso andamento, dopo l’inoculo del complesso retrovirale in topi Cybr-deficienti e wild type, sono stati caratterizzati a livello fenotipico e funzionale i linfociti presenti nei tumori, nei linfonodi drenanti e nelle milze al momento della massima crescita tumorale (giorni 11-15). Abbiamo riscontrato un ridotto numero di linfociti T CD4+ e CD8+ e di CTL antigene specifici nella popolazione infiltrante il tumore nei topi Cybr-deficienti. Tuttavia questa differenza si è ridotta alla fine del periodo analizzato. Inoltre, un ritardo simile è stato riportato nello sviluppo dell’attività litica nei CTL provenienti da topi Cybr-KO rispetto a topi wild type. Al contrario, linfociti T memoria wild type e Cybr-KO non hanno mostrato nessuna differenza in termini di attività litica. Complessivamente, questi dati indicano che la deficienza di Cybr ha un significativo impatto nell’attivazione delle cellule T naive e nella loro espansione dopo il priming, ma non definiscono se questa proteina influenzi maggiormente la fase di priming e/o adesione cellulare o il trafficking e la migrazione delle cellule del sistema immunitario. Per chiarire questi aspetti, sono stati trasferiti linfociti T naive provenienti da topi Cybr-KO/GFP o B6/GFP in topi RAG2-/-γc-/- inoculati con il complesso retrovirale. Questi topi mancano di cellule T, B e NK e non regrediscono spontaneamente i tumori M-MSV indotti. Nonostante l’infusione di cellule T, i tumori hanno continuato a crescere, indicando che le cellule T naive non sono state in grado di montare una risposta immune pienamente efficace in questo modello, un aspetto probabilmente dovuto ad un reclutamento e priming sub ottimali nei linfonodi, che sono risultati ipoplastici. Al fine di rispondere a questi quesiti biologici, topi B6 nu/nu atimici ricostituiti con tessuto midollare depleto di linfociti T provenienti da topi wild type o Cybr-KO e successivamente infusi con linfociti T naive o memoria provenienti da topi Cybr-KO/GFP o B6/GFP, dovrebbero costituire un modello sperimentale ottimale per investigare il ruolo di Cybr sia nel comparto T che nel comparto APC. Nell’insieme, i risultati ottenuti indicano che la deficienza di Cybr ha un significativo impatto nella risposta immune antigene-specifica, ma studi addizionali devono essere condotti al fine di definire con maggior precisione il ruolo di Cybr nella fase di priming e nel ritardo dello sviluppo dell’attività litica
Rizzuto, Gabrielle Ann. "Self-antigen specific CD8+ T cell precursor : frequency determines the quality of the anti-tumor immune response /." Access full-text from WCMC, 2008. http://proquest.umi.com/pqdweb?did=1621818951&sid=3&Fmt=2&clientId=8424&RQT=309&VName=PQD.
Full textHernandez, Maria Genevieve H. "The Role of CD40 in Naïve and Memory CD8+ T Cell Responses: a Dissertation." eScholarship@UMMS, 2007. https://escholarship.umassmed.edu/gsbs_diss/346.
Full textCarré, Thibault. "Analyse des bases moléculaires de la résistance tumorale à la cytotoxicité spécifique et naturelle dans le contexte microenvironnemental." Thesis, Paris 11, 2012. http://www.theses.fr/2012PA11T057.
Full textDuring antitumor immune response, cancer cells genetic instability combined with immune system selective pressure may drive to the emergence of tumor variant resistant to lysis by cytotoxic effector cells through a phenomenon called immunoediting. A better understanding of those mechanisms putatively involved in tumor susceptibility to natural and/or specific lysis would enable new integrative and more effective immunotherapeutic strategies. In this context, we studied a model of resistance to specific lysis linked to actin cytoskeleton remodeling (i). We showed that combined inhibition of actin interacting protein (caldesmone, ezrin, radixin and moesin) reduced tumor cells susceptibility to cytotoxic T lymphocytes (CTLs) lysis. Moreover, we identified microRNAs differentially expressed between parental cell line and resistant variant and are currently studying their impact on tumor susceptibility to CTLs lysis. In order to depict the role of innate immunity Natural Killer (NK) cells selective pressure, on tumor cells and on the emergence of resistant variants, we also established a maintained coculture model of melanoma cells with NK cells (ii). Selected cells obtained were resistant to NK cells-mediated lysis (but still susceptible to CTLs-mediated specific lysis) and formed less contact and immune synapse with NK cells than parental cell line. Transcriptomic analysis revealed the reduced expression of B7-H6 (ligand of an NK cells activating receptor) partially contributing to the resistance phenotype. The expression of several genes involved in migration/invasion/adhesion is also modulated and some cell characteristics (cell growth in semi-solid medium, adhesion, migration) tend to reflect the acquisition through coculture of an increased aggressiveness. Finally, we evaluated the impact of connexin-43 (Cx43), involved in the establishment of Gap Junctions (GJs), on antitumor response (iii). We showed that despite localization at the immune synapse between tumor target cell and CTL, Cx43 and GJs do not modulate susceptibility to CTL-mediated specific lysis. Nevertheless, GJs contribute to the emergence of highly reactive specific CD8+ T lymphocytes following antigen stimulation
Varga, Steven Michael. "The Virus-Specific CD4+ T Cell Response During Acute Lymphocytic Choriomeningitis Virus Infection and into Long Term Memory: a Dissertation." eScholarship@UMMS, 1999. https://escholarship.umassmed.edu/gsbs_diss/116.
Full textBashyam, Hema Sundara. "Serotype Cross-Reactive CD8+ T Cell Response to Heterologous Secondary Dengue Virus Infections in Humans: a Dissertation." eScholarship@UMMS, 2006. https://escholarship.umassmed.edu/gsbs_diss/258.
Full textPesce, John Thomas. "Early events leading to the host protective Th2 immune response to an intestinal nematode parasite /." Download the dissertation in PDF, 2005. http://www.lrc.usuhs.mil/dissertations/pdf/Pesce2005.pdf.
Full textAli, Qasim. "Contribution to the mathematical modeling of immune response." Phd thesis, Ecole Nationale Supérieure des Mines de Saint-Etienne, 2013. http://tel.archives-ouvertes.fr/tel-00905603.
Full textIferroudjene, Djedjiga. "Complément et réponse immune : effet comitogénique du composant C3 et du facteur H sur les lymphocytes T." Rouen, 1988. http://www.theses.fr/1988ROUES011.
Full textAnderson, Kathleen. "CD25+ CTLA-4+ T Cell-Dependent Induction of Anergic CD25- T Cells Limits the Immune Response to H. pylori Infection Resulting in Mild Gastritis and Persistent Colonization." Connect to text online, 2006. http://rave.ohiolink.edu/etdc/view?acc%5Fnum=case1144332338.
Full textBartolo, Laurent. "Réponses immunitaires et induction de tolérance pour la thérapie génique rAAV du muscle basée sur le ciblage des hépatocytes : induction de tolérance et mécanismes immunitaires liés à la transduction des hépatocytes Liver-based tolerance induction of CD8+ and CD4+ T cells responses in rAAV muscle gene therapy." Thesis, Sorbonne Paris Cité, 2018. http://www.theses.fr/2018USPCB198.
Full textIt is increasingly realized that immune responses to rAAV gene therapy treatments, not only to the vector capsid but also to reparative transgenes can cause adverse effects of importance in the case of muscle gene delivery in monogenic muscle disorders. These responses to "foreign" sequence elements of the reparative transgene that are not initially present or insufficiently expressed in the host represent a threat which can eliminate the transduced cells of interest. It is therefore highly desirable to design immune tolerance protocols able to impose transgene-specific immunological unresponsiveness. We explored here how liver-based recombinant adeno-associated viral vector (rAAV) mediated expression of foreign transgene imposes immune tolerance after immunogenic rAAV muscle transduction. We found that liver transgene expression driven with the hAAT hepatocyte specific promotor is effective to promote robust muscle-associated transgene expression, nullifying transgene-specific CD8+ T cell responses as well as humoral responses. Liver transgene expression equally promotes immune tolerance to subsequent rAAV muscle injections despite the presence of transgene-specific memory responses. Importantly, the CD8+ T cell tolerization process leads to partial deletion and conversion into PD-1+ CD8+ T cells, a hallmark of T cell exhaustion. Likewise, CD4+ T cell responses elicited in muscle do not compromise liver-based tolerance induction. Our results demonstrate that liver transduction with rAAV vectors using hepatocyte specific hAAT promotor imposes immune tolerance to transgene-specific T cells elicited from the naïve T cell repertoire after muscle transduction. Confronting our results with others, we suggest that CD8+ T cell depletion occurs after antigen recognition through direct capture and internalization of T cell corpses by hepatocyte in a mechanism already described and referred to as suicidal emperipolesis. Alternatively, BIM-dependent apoptotic process may also occur as a result of T cell-hepatocyte interactions. Regarding transgene-specific CD4+ T cells, we presume that they undergo phenotypic conversion such as Treg conversion as evidenced in multiple sclerosis models. Our results also suggest that the retention time and affinity of transgene-specific T cells next to transduced hepatocytes is critical for their fate. Last, considering applications for muscle gene therapies, control of local muscle immune response is of crucial importance in the treatment of several muscular dystrophies including Duchenne's muscular dystrophy. In this context our liver-based tolerance induction protocol is relevant, provided that the transgene of interest does not alter hepatocytes functions and is beneficial against adverse immune responses
Barrientos, Lorena. "Modulation fonctionnelle des cellules dendritiques par les " Neutrophil Extracellular Traps "." Phd thesis, Université Paris Sud - Paris XI, 2013. http://tel.archives-ouvertes.fr/tel-01016696.
Full textMarechal, Yoann. "Itpkb and Ins (1,3,4,5) P4 control proapoptotic Bim gene expression and survival in B cells." Doctoral thesis, Universite Libre de Bruxelles, 2008. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/210450.
Full textLes lymphocytes B déficients en Itpkb présentent un défaut de survie car ils ne peuvent activer correctement les protéines kinases Erk1/2 suite à la stimulation du BCR de surface. Cela conduit à la surexpression anormale de la protéine pro-apoptotique Bim. La diminution de l’expression de Bim est suffisante dans ce modèle pour restaurer une fonction normale des lymphocytes B. In vitro, Nous avons montré que l’Ins(1,3,4,5)P4 est nécessaire à la translocation de Rasa3, protéine favorisant l’inactivation de la voie de Ras, de la membrane vers le cytoplasme. L’étude de lymphocytes invalidés pour Itpkb dans un modèle de BCR transgénique semble montrer que des anomalies de réponse calcique ne participent pas au phénotype.
En conclusion, nos résultats indiquent qu’une des voies de signalisation préférentielle de l’Ins(1,3,4,5)P4 passe par la modulation de la localisation subcellulaire de protéines possédant un domaine d’affinité pour l’Ins(1,3,4,5)P4 telle que Rasa3.
Doctorat en Sciences médicales
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Pino, Steven C. "Role of Endoplasmic Reticulum Stress Response Signaling in T Cells: A Dissertation." eScholarship@UMMS, 2008. https://escholarship.umassmed.edu/gsbs_diss/381.
Full textAntoine, Pierre. "Etude de la réponse des lymphocytes T CD4+ au cours de l'infection primaire par le cytomégalovirus." Doctoral thesis, Universite Libre de Bruxelles, 2014. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/209148.
Full textAprès l’infection primaire, le virus persiste tout au long de la vie à l’état latent mais peut se réactiver de manière intermittente. Ceci est associé à l’expansion de lymphocytes T CD4+ fortement différenciés ayant des fonctions auxiliaires et cytolytiques. L’infection primaire est, par contre, caractérisée par une réplication virale intense qui dure plusieurs mois. Il a été montré que l’exposition prolongée à des concentrations élevées d’antigènes entraine une perte progressive de fonction par les lymphocytes T appelée épuisement et caractérisée par l’expression de récepteurs inhibiteurs. L’impact de la réplication virale intense observée au cours de l’infection primaire par le CMV sur la fonction des lymphocytes T CD4+ n’est pas bien connu.
La fonctionnalité des lymphocytes T CD4+ a été explorée chez l’humain et le singe rhésus au cours de l’infection primaire et comparée à celle de sujets porteurs chroniques du virus.
Les résultats montrent que l’infection primaire par le CMV est associée à la détection de lymphocytes T CD4+ circulants ayant une faible capacité de prolifération et de production de cytokines et d’IL-2 en particulier.
L’impact de la différenciation sur la fonction des lymphocytes a été exploré en détail chez l’humain. Il a été observé qu’un degré de différenciation plus élevé des lymphocytes T CD4+ spécifiques du CMV joue un rôle dans la production réduite d’IL-2. Toutefois, la fraction moins différenciée (exprimant la molécule CD28) présente également une sécrétion d’IL-2 moindre au cours de l’infection primaire. Ceci fait partie d’une diminution globale de la production de cytokines au cours de l’infection primaire qui affecte également la sécrétion d’IFNγ et TNFα, entraine une polyfonctionnalité réduite et est indépendante de la différenciation. L’épuisement des lymphocytes T CD4+ spécifiques du CMV contribue à leur fonctionnalité moindre comme l’indique l’expression accrue du récepteur inhibiteur PD-1 et l’augmentation des réponses prolifératives en présence d’anticorps bloquant PD-1.
Le lien entre excrétion virale et fonction lymphocytaire a été étudié chez le macaque rhésus. L’infection par le CMV est observée chez les singes juvéniles et adultes mais pas chez les nourrissons. L’excrétion urinaire et salivaire est significativement plus fréquente et intense chez les singes juvéniles par rapport aux adultes. Comme chez l’humain au cours de l’infection primaire, les lymphocytes T CD4+ spécifiques du virus sont moins
polyfonctionnels et prolifèrent moins efficacement chez les singes juvéniles par rapport aux singes adultes. Ceci est associé à l’expression accrue du récepteur inhibiteur PD-1 chez les singes juvéniles. La réponse proliférative des lymphocytes T CD4+ est accrue en présence d’anticorps bloquant PD-1 ou d’IL-2 exogène. Enfin, une association inverse entre fonction lymphocytaire et excrétion urinaire a été mise en évidence chez les macaques adultes.
Ces résultats indiquent que l’infection par le CMV présente des caractéristiques semblables chez l’humain et le singe rhésus. L’infection primaire est associée à la détection de lymphocytes T CD4+ ayant une fonctionnalité moindre qu’au cours de l’infection chronique. L’expression du récepteur inhibiteur PD-1 typique des cellules épuisées est l’un des mécanismes impliqués et pourrait être la cible de stratégies immunomodulatrices visant à améliorer les fonctions lymphocytaires et le contrôle de la réplication virale. Les résultats présentés indiquent que l’infection naturelle chez le singe rhésus constitue un modèle potentiellement utile à l’étude de la réponse immune au CMV humain et à l’évaluation de stratégies immunomodulatrices.
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Cytomegalovirus infection is mostly asymptomatic in immunocompetent hosts but leads to severe morbidity and mortality in immunocompromised subjects and foetuses.
After primary infection, CMV establishes lifelong persistence but can reactivate intermittently. This is associated with the expansion of highly differentiated CD4+ T lymphocytes exhibiting helper functions and cytolytic activity.
Primary infection is characterised by an intense viral replication lasting several months. It has been shown that prolonged exposure to elevated antigen concentrations induces a progressive loss of function by T lymphocytes called exhaustion. This state of functional impairment is associated to the expression of inhibitory receptors. The consequence of the intense viral replication seen in primary CMV infection on CD4+ T cell function is unknown.
CD4+ T cell function has been studied in human and rhesus macaque during primary CMV infection. Chronic CMV carriers have been used as controls.
The results show that primary CMV infection is associated to the detection of circulating CD4+ T lymphocytes exhibiting weak proliferative capacities and reduced cytokine production affecting IL-2 in particular.
The impact of differentiation on lymphocyte function has been explored in detail in human. An increased proportion of terminally differentiated CD4+ T cells (CD28-) is observed during primary infection. These lymphocytes are unable to secrete IL-2 in response to CMV antigens. Interestingly, CD28+ CMV-specific CD4+ T cells also exhibit reduced IL-2 production during primary infection. This is part of a global reduction of cytokine production affecting IFNγ and TNFα as well. The impaired cytokine production is associated to reduced polyfunctionality and is independent of differentiation. Exhaustion of CMV-specific CD4+ T lymphocytes contributes to the reduced functionality as shown by an increased expression of the inhibitory receptor PD-1 and improved proliferative responses in the presence of PD-1 blocking antibodies.
The relationship between viral replication and lymphocyte function has been explored in rhesus macaques. CMV infection is observed in juvenile and adult monkeys but not in newborns. Excretion in urine and saliva is significantly more frequent and intense in juvenile monkeys than adults. As in primary infection in human, CMV-specific CD4+ T lymphocytes are less polyfunctional and have lower proliferative capacities in juveniles as compared to adults. This is associated with an increased expression of PD-1 in juvenile monkeys. CD4+ T cell proliferative responses are increased when PD-1 blocking antibodies or exogenous IL-2 are added to the culture medium. Finally, an inverse association between lymphocyte function and urinary excretion has been observed in adult macaques.
These results indicate that CMV infection shares common features in human and rhesus macaque. Primary infection is associated to the detection of CD4+ T lymphocyte displaying lower functional capacities as compared to chronic infection. Exhaustion contributes to the functional impairment and the inhibitory receptor PD-1 could be targeted by immunomodulatory strategies aiming at improving lymphocyte functions and controlling viral replication. Natural CMV infection in rhesus macaque might be useful as a model to evaluate the efficacy and safety of immunomodulatory approaches.
Doctorat en Sciences médicales
info:eu-repo/semantics/nonPublished
Régnier, Paul. "Effet des interactions homéostatiques entre cellules dendritiques, lymphocytes effecteurs et régulateurs sur les réponses immunitaires anti-tumorales : étude du rôle de différentes cellules dendritiques in vivo chez la souris, et étude algorithmique des relations complexes entre transcriptome tumoral, populations immunitaires et survie in silico chez les patients A paradoxical role for Flt3 ligand in tumor immune response reveals homeostatic control of NK and treg cells by dentritic cells Tumor infiltration by immune cells favors patient survival in some cancers bur is highly detrimental in immune-privileged sites." Thesis, Sorbonne Paris Cité, 2018. https://wo.app.u-paris.fr/cgi-bin/WebObjects/TheseWeb.woa/wa/show?t=2244&f=15657.
Full textThe cancer, one of the main causes of death in the world, can appear in almost any type of tissue, and is characterized by an anarchic proliferation of cells and the establishment of a tolerogenic immune response favouring the tumour growth, leading to low efficiency of drug interventions. Dendritic cells (DCs), real sentinels of the body, seem to play a role in the establishment of both efficient anti-tumoral immune response and tolerance against cancer. Nevertheless, the role of the different DCs subtypes in the tumoral development stays poorly known. During this thesis, I studied different dendritic and lymphocytic cellular actors, their relationships and their involvement in the immune response or tolerance to tumours. During the first part of my thesis, I studied the effect of the artificial modulation of DCs homeostasis on other immune cells and also on anti-tumoral response in vivo in mice. I proved the existence of a paradoxical role of the Flt3-L (FL) cytokine - a growth factor essential to the differentiation and the homeostasis of classical/conventional dendritic cells (cDCs) and plasmacytoid dendritic cells (pDCs) - on the B16 melanoma growth. In fact, its overexpression or absence both lead to a better control of the tumoral development, accompanied by an increased survival of mice. FL deficiency induces, together with the loss of both cDCs and pDCs, a drastic reduction of regulatory T lymphocytes (Tregs) protecting the tumour, and also a global reinforcement of the anti-tumoral adaptive immune response via helper T lymphocytes. Its overexpression induces an increase of the numbers of cDCs and pDCs, and despite a raised presence of Tregs, also a strong intra-tumoral recruitment of activated natural killer (NK) cells, one of the major actors of the anti-tumoral innate response. The study of cDCs-deficient mice allowed me to demonstrate the existence of a DCs-mediated control of the NK cells homeostasis. Furthermore, the combination of both FL treatment and antibody-mediated Tregs depletion has an exacerbated therapeutic effect in mice. Next, using bioinformatic analysis of transcriptomes of 35 different cancer types, I showed that the FL paradox also exists in humans, at least for some cancers, and that gene signatures specific of DCs subsets can be correlated in a paradoxical, beneficial or detrimental manner to survival. In parallel, I evaluated the presence of several immune cells in the tumour infiltrate and their effects on patients survival. Thanks to R language algorithms I developed, I was able to analyse for each studied cancer the immune cell populations-specific gene signatures and the most involved or dysregulated genes and biological functions (pathways) in the control of the 5 years survival of patients. My results indicate that the immune cells of the tumour infiltrate can play, according to the cancer, a beneficial or deleterious role. This immune infiltrate and the associated pathways were generally of bad prognosis in cancers of immune-privileged organs, but on the other hand were beneficial in skin and breast cancers. For each cancer type, I determined the individual impact on survival of several types of immune cells and established correlations between involved pathways and some of these cell populations. Altogether, the results allow to better understand the complex relationships between each cancer and the associated immune infiltrate, and will later lead to help the development of immunotherapeutic strategies more adapted to a given tumour environment, by targeting the immune populations that could really impact the survival of patients
Österberg, Johanna. "Inflammatory Reactions in Peritonitis and Malignant Obstructive Jaundice : Clinical and Experimental Studies with Special Emphasis on the Cellular Immune Response." Doctoral thesis, Uppsala University, Department of Surgical Sciences, 2005. http://urn.kb.se/resolve?urn=urn:nbn:se:uu:diva-4767.
Full textPatients with peritonitis or malignant obstructive jaundice (HPB+) have an increased morbidity and mortality due to sepsis. An altered cell-mediated immunity in the intestinal mucosa might promote gut barrier failure, increased endotoxin and cytokine release and bacterial translocation (BT) in these conditions. A clinically relevant rat model of polymicrobial peritonitis induced sepsis by cecal ligation and puncture (CLP) was used. Septic animals demonstrated a superficial injury in the small intestinal mucosa, and a significant reduction in T lymphocytes in the villi, as well as increased number of macrophages in the villi and in the MLNs as compared to sham. CLP caused increased concentration of TNF-α and IL-6 in ascitic fluid. CLP + the immunomodulator Linomide decreased the TNF-α level, reduced mucosal damage and attenuated the changes in T lymphocytes and macrophages observed following CLP. CLP + selective cyclooxygenase (COX)-2 inhibitor (SC-236) or nonselective COX inhibitor (indometacin) decreased the amount of macrophages in the mucosa and the MLNs compared to untreated CLP. CLP + indometacin decreased T lymphocytes in the villi and MLNs. SC-236 + CLP reduced mucosal injury and cytokine release as compared to indometacin. An increased rate of apoptosis in both the mucosa and MLNs was seen following CLP; COX inhibitors enhanced this phenomenon in the MLNs.
BT occurred infrequently in patients with acute peritonitis and in HPB+ there was no evidence of BT. Peritonitis and HPB+ causes significant inflammatory cellular reactions as increased endotoxin and cytokine plasma levels and an altered immune cell distribution in MLNs, in HPB+ a high rate of apoptosis in MLNs was observed.
An altered pattern of immunocompetent cells within the mucosa and in MLNs was found in experimental and clinical peritonitis as in HPB+. Lymphocyte depletion may be a result of increased apoptosis, which could reduce the ability of septic or jaundice patients to eradicate infection.
Hespel, Cindy. "Régulation de la réponse immunitaire adaptative par les cellules dendritiques conventionnelles et inflammatoires." Doctoral thesis, Universite Libre de Bruxelles, 2012. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/209702.
Full textNous avons donc évalué le rôle de l’IDO exprimé par les cellules dendritiques conventionnelles dans la régulation de la réponse adaptative. L’ensemble des résultats in vitro révèle que l’expression d’IDO par les cellules dendritiques conventionnelles au cours de leur maturation n’influence celle-ci ni au niveau de l’expression des molécules MHCII et CD86 ni au niveau de leur capacité à induire la différenciation des lymphocytes Th1. De plus, dans des modèles d’immunisation in vivo par transfert de cellules dendritiques conventionnelles, l’expression d’IDO par ces dernières ne semble pas leur permettre de contrôler les réponses T CD4+ ou T CD8+. Cependant, nous avons constaté qu’en absence de lymphocytes T régulateurs naturels l’expression d’IDO par les cellules de l’hôte constitue un mécanisme important limitant la réponse Th1.
En cas d’inflammation ou d’infection, de profonds changements affectent le compartiment des cellules dendritiques où émerge une nouvelle sous-population qui se différencie à partir des monocytes inflammatoires du sang et qui portent le nom de cellules dendritiques inflammatoires. Alors que les cellules dendritiques conventionnelles forment une population hétérogène où chaque sous-population semble se spécialiser dans la différenciation d’un type particulier de lymphocyte T auxiliaire ou « helper », la littérature met en évidence une incroyable plasticité phénotypique des cellules dendritiques inflammatoires qui les rend capables de s’adapter au type d’infection auquel l’hôte est confronté en intervenant directement au niveau de la réponse innée mais aussi en participant à l’initiation et la régulation de la réponse T la plus adaptée.
Le modèle d’immunisation in vivo par transfert de cellules dendritiques inflammatoires présentant l’antigène OVA nous a permis de démontrer la capacité de ces cellules à promouvoir spécifiquement la différenciation de lymphocytes de type Th17. Dans le cadre d’une immunisation classique par un adjuvant, le défaut dans le recrutement des cellules dendritiques inflammatoires dans les souris CCR2-/- nous a permis de mettre en évidence le rôle indispensable des cellules dendritiques inflammatoires pour l’induction des réponses Th1 et Th17. Finalement, envisageant la possibilité d’une collaboration entre DCs conventionnelles et inflammatoires pour l’induction des réponses de type Th17, nous avons constaté que le transfert de cellules dendritiques conventionnelles présentant l’antigène KLH provoque in vivo le recrutement de cellules dendritiques inflammatoires au sein des ganglions drainant le site d’injection et que ces cellules dendritiques inflammatoires semblent nécessaires pour la différenciation des lymphocytes de type Th17.
La collaboration entre cellules dendritiques via le transfert d’informations pourrait être un évènement fréquent permettant de réguler la réponse immunitaire adaptative à trois niveaux principaux :au niveau quantitatif, en augmentant le nombre de cellules dendritiques présentant l’antigène, au niveau de la durée, en transmettant l’information aux cellules dendritiques inflammatoires colonisant les tissus desquels les cellules dendritiques conventionnelles disparaissent après activation/maturation et au niveau qualitatif, en combinant les propriétés intrinsèques des différentes sous-populations de cellules dendritiques afin de réguler la différenciation des lymphocytes T helper.
Doctorat en Sciences
info:eu-repo/semantics/nonPublished
Lewalle, Philippe. "Quelle place pour la greffe de cellules souches haploidentiques et comment améliorer son efficacité clinique en manipulant, en post-transplantation, l'environnement cellulaire au moyen de l'utilisation de populations cellulaires sélectionnées ou de facteurs solubles modulant l'immunité ?" Doctoral thesis, Universite Libre de Bruxelles, 2011. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/209973.
Full textThe aim of the work described in this thesis has been to implement a strategy to transplant a patient using a HLA haploidentical donor. The strategy is to try to improve DFS that could be applied both in the autologous or allogeneic context: first, by using nonspecific immune manipulation post transplant and then, by developing specific strategies directed against leukemia antigens. Particularly in the allogeneic situation, the aim was to increase the GVL effect without inducing or aggravating the deleterious GVHD. The first part of this thesis described our own clinical results, consisting of three consecutive phase I/II studies, in which we tried to determine the feasibility of giving prophylactic donor lymphocyte infusions (DLI) post transplant and the effect of replacing granulocyte colony-stimulating factor (G-CSF), typically used to speed up neutrophil recovery, with granulocyte macrophage colony-stimulating factor (GM-CSF), which is known for its immunomodulatory properties. The slow immune reconstitution in haploidentical transplant is chiefly responsible for the high incidence of early lethal viral and fungal infections, and most probably for early relapses; therefore, we sought to accelerate and strengthen the post transplant immune reconstitution without increasing the GVHD rate. Thus, we have studied the impact of post transplant growth factor administration and of unselected DLI in haploidentical transplant. We have also implemented, in our center, anti-cytomegalovirus (CMV) specific T cell generation and infusion to improve anti-CMV immune reconstitution. Since then, our results have been pooled in a multi-center analysis performed by the European Bone Marrow Transplantation group (EBMT) allowing us to compare our results with those of the entire group. We have also participated in the design of an ongoing study aimed at selectively depleting the graft from alloreactive T cells, and improving post transplant T cell add-backs. In our attempts to generate and expand ex vivo lymphocytes (directed against pathogens (CMV) and leukemia-associated antigens, Wilms' tumor gene 1 (WT1) and to use them in vivo, we found inconsistent results (in the case of WT1) using classical clinical grade dendritic cells (DC) generated and matured in bags, as was the case for the majority of the teams worldwide. This led us to question the full functionality of these DC and we undertook a thorough comparative analysis of DC generated and differentiated in bags and in plates (typical for most pre-clinical studies). This analysis showed us that one cannot transpose pre-clinical studies (using culture plates) directly to clinical protocols (generally using clinical grade culture bags) and that DC generated in bags are functionally deficient. We learned that, if we want to use a DC vaccine to improve the GVL effect in haploidentical transplant, we will have to be careful about the technique by which they are generated. To improve immunotherapeutic approaches, the understanding of the mechanisms underlying tumor tolerance and how to manipulate them is critical in the development of new effective immunotherapeutic clinical trials. This is why we currently focus on how to obtain effective in vivo anti-leukemia immune reactions using an ex-vivo manipulated product to trigger the immunotherapeutic response. More specifically, we are analyzing the impact of regulatory T cell (Tregs) depletion and function for an adequate anti-leukemic immune response. This pre-clinical work aims at improving the outcome of leukemia patients who have relapsed and been put back into second remission and at decreasing the RR after HSCT, especially in the field of haploidentical transplantation.
In conclusion, haploidentical transplantation has become a valuable tool. The results are at least similar to those obtained using MUD when performed in the same group of patients. Specific immunomodulation post transplant can affect events such as GVHD and GVL, but clinically we are still at the level of nonspecific manipulations. It is our hope that ongoing pre-clinical work will enable us to perform specific anti-pathogen and anti-leukemia immune manipulation that will favorably influence the patient outcome.
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Dans la majorité des situations, le système immunitaire autologue est incapable d’éradiquer les cellules leucémiques résiduelles qui échappent à la radiothérapie et à la chimiothérapie, cependant un équilibre peut s’établir entre les cellules leucémiques et immunitaires aboutissant à une rémission pouvant durer plusieurs mois ou années. Si cet équilibre se rompt, une rechute clinique peut se déclarer. Dans ce contexte, il est prouvé que la greffe allogénique de cellules souches hématopoïétiques est le moyen le plus efficace de renforcer les réactions immunitaires contre la leucémie par la réaction du greffon contre la leucémie et ainsi d’obtenir une éradication définitive de la maladie résiduelle chez un nombre significatif de patients. En effet, le concept global de l’allogreffe de cellules souches hématopoïétiques a évolué du concept de transplantation d’organe (remplacement d’un organe malade par un nouvel organe sain) vers celui de créer une extraordinaire plateforme d’immunothérapie à travers laquelle le système immunitaire du donneur contribue à l’éradication des cellules leucémiques persistantes. Donc, la problématique reste celle de trouver les meilleures modalités d’immunomodulation pour achever une prise du greffon, un effet anti-leucémique puissant du greffon, et l’absence ou un minimum d’effet du greffon contre l’hôte. Différentes stratégies existent pour atteindre cet objectif, comme l’utilisation de cytokines pour moduler la reconstitution immunitaire, des déplétions cellulaires globales ou spécifiques du greffon et l’infusion de cellules immunes «globales» ou spécifiques du donneur après greffe. Ces stratégies sont encore largement à l’étude. Néanmoins, la persistance d’un taux de rechute élevé observé chez les patients leucémiques, après allogreffe reste la cause principale de décès, avant celle liée à la toxicité de la greffe. De plus, étant donné que seulement environ 40 à 70% (dépendant de l’origine ethnique) des patients avec une hémopathie à haut risque, éligibles pour une greffe allogénique, ont un donneur familial ou non familial complètement HLA compatible, des efforts importants ont été développés pour rendre faisable l’utilisation de donneurs familiaux alternatifs, haploidentiques. L’avantage de cette approche est l’accès immédiat à un donneur pour quasiment tous les patients.
Le but du travail décrit dans cette thèse a été l’implémentation d’une stratégie d’allogreffe utilisant un donneur haploidentique. Le travail vise également à développer de façon plus large des stratégies qui peuvent améliorer le taux de survie sans rechute, non seulement dans le contexte des greffes haploidentiques, mais également dans le cadre des greffes allogéniques en général, ainsi que dans les situations autologues :premièrement, par la manipulation immunitaire non spécifique après greffe et ensuite par le développement de stratégies spécifiques dirigées contre des antigènes leucémiques. En particulier dans la situation allogénique, le but a été d’augmenter l’effet du greffon contre la leucémie sans induire ou aggraver l’effet délétère du greffon contre l’hôte. La première partie de la thèse décrit les résultats cliniques de notre propre protocole de greffe haploidentique, qui a consisté en trois études consécutives de phase I/II. Dans ces études, nous avons voulu déterminer la faisabilité de réaliser des infusions prophylactiques de lymphocytes du donneur après transplantation, et l’impact du remplacement du « granulocyte colony-stimulating factor » (G-CSF), largement utilisé pour permettre une récupération en polynucléaires neutrophiles plus rapide, par du « granulocyte-macrophage colony-stimulating factor » (GM-CSF), lequel est connu pour ses propriétés immunomodulatrices différentes. La reconstitution immunitaire très lente après greffe haploidentique est majoritairement responsable de l’incidence élevée de décès par infections virales et fungiques précoces, et très probablement des rechutes précoces. C’est pourquoi nous avons cherché à accélérer et à renforcer la reconstitution immunitaire post-greffe sans augmenter la fréquence de réaction du greffon contre l’hôte. Nous avons donc étudié l’impact de l’administration de facteurs de croissance et l’infusion de lymphocytes non sélectionnés du donneur en post greffe haploidentique. Nous avons également implémenté dans notre centre, la génération et l’infusion de lymphocytes T spécifiques anti-cytomégalovirus (CMV) afin d’améliorer la reconstitution immunitaire anti-CMV. D’autre part, nos résultats ont été regroupés dans une étude multicentrique menée par le groupe européen de transplantation de moelle osseuse (EBMT), ce qui nous a permis de comparer nos résultats avec ceux de l’entièreté du groupe. Nous avons parallèlement participé à la conception d’une étude actuellement en cours ayant pour but d’améliorer la reconstitution immunitaire après greffe par la déplétion sélective du greffon en lymphocytes T alloréactifs et par l’infusion après greffe de lymphocytes T du donneur également sélectivement déplétés en lymphocytes T alloréactifs. Afin d’optimaliser l’effet anti-leucémique du système immunitaire, nous avons débuté un protocole de vaccination par cellules dendritiques (DCs). Ces cellules dendritiques étaient chargées en lysat de blastes leucémiques dans le cas de patients présentant au diagnostic une leucémie aigue surexprimant l’oncogène 1 de la tumeur de Wilms (WT1). Néanmoins dans nos travaux de génération et d’expansion ex-vivo de lymphocytes T spécifiques de l’antigène WT1, utilisant les DCs de grade clinique, générées et maturées en poches, nous avons rencontré des résultats inconsistants, comme c’était le cas dans la majorité des protocoles cliniques internationaux de vaccination. Nous nous sommes alors posé la question de la fonctionnalité globale de ces cellules et nous avons entrepris une analyse comparative poussée des DCs générées et différenciées en poches ou en plaques. Les DCs générées en plaques sont celles utilisées dans la plupart des travaux précliniques. Cette analyse nous a montré que l’on ne pouvait pas directement transposer les résultats précliniques basés sur des DCs générées en plaques dans des protocoles cliniques basés sur des DCs générées en poches, car ces dernières présentent des déficits fonctionnels importants. Nous avons appris que si l’on voulait utiliser un vaccin à base de cellules dendritiques pour améliorer l’effet du greffon contre la leucémie dans les greffes allogéniques, nous devions être très attentifs quant au protocole utilisé pour la génération de ces vaccins cellulaires. Pour améliorer les approches immunothérapeutiques, la connaissance des mécanismes qui établissent la tolérance tumorale et des façons de manipuler ceux-ci, est critique dans le développement de nouveaux protocoles efficaces. C’est pourquoi nous nous concentrons actuellement sur les conditions nécessaires à l’obtention in vivo d’une réaction immune anti-leucémique efficace lors de l’utilisation d’un produit cellulaire manipulé ex vivo. Plus spécifiquement, nous analysons l’impact de la déplétion en lymphocytes T régulateurs (Tregs) sur la réponse anti-leucémique. Ce travail préclinique a pour but d’améliorer le devenir de patients leucémiques qui ont rechutés et ont été mis en seconde rémission, ainsi que de diminuer le taux de rechute après allogreffe, spécifiquement après greffe haploidentique.
En conclusion, la transplantation haploidentique est actuellement un outil précieux pour de nombreux patients. Les résultats sont au minimum similaires à ceux qui sont obtenus par les greffes non-familiales HLA identiques lorsqu’elles sont pratiquées dans les mêmes groupes de patients. L’immunomodulation spécifique après greffe peut affecter des événements comme la réaction du greffon contre l’hôte et la réaction du greffon contre la leucémie, mais en pratique clinique nous en sommes encore au niveau de la manipulation aspécifique. Nous espérons que les travaux précliniques actuels vont nous permettre d’appliquer des stratégies spécifiques et d’obtenir une manipulation immune anti-leucémique qui aura une influence favorable significative sur le devenir des patients.
Doctorat en Sciences médicales
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Gilardin, Laurent. "Identification des épitopes T d’ADAMTS13 chez les patients atteints de Purpura Thrombotique Thrombocytopénique The ADAMTS13¹²³⁹-¹²⁵³ peptide is a dominant HLA-DR1-restricted CD4⁺ T-cell epitope Purpura Thrombotique Thrombocytopénique : physiopathologie, clinique, pronostic et traitement In silico calculated affinity of FVIII-derived peptides for HLA class II alleles predicts inhibitor development in haemophilia A patients with missense mutations in the F8 gene In silico prediction of immuno-dominant T-cell epitopes on human therapeutic factor VIII Predictive immunogenicity of Refacto AF Complement C3 is a novel modulator of the anti-factor VIII immune response Anti-ADAMTS13 Autoantibodies against Cryptic Epitopes in Immune-Mediated Thrombotic Thrombocytopenic Purpura." Thesis, Université Paris-Saclay (ComUE), 2019. http://www.theses.fr/2019SACLS520.
Full textThrombotic thrombocytopenic purpura (TTP) is a rare and severe disease characterized by auto-antibodies directed against ADAMTS13 (A13), a plasmatic protein involved in haemostasis. The implication of CD4⁺ T cells in the pathogenesis of the disease is suggested by the existence of a restriction to particular HLA-DR alleles and by the IgG isotype of the antibodies. In this study, we wished to determine the T cell epitopes of A13. First, we selected in silico the immunodominant peptides, based on their binding capacity to HLA-DR11 molecules. Second, their binding capacity to purified HLA-DR11 molecules using a ELISA competitive assay led us to identify the best binder peptides. Finally, we determined the peptides recognized by human CD4⁺ T cells from DR11 healthy donors and patients. These results were reproduced for the HLA-DR1 haplotype and in a transgenic humanized HLA-DR1 mouse model. In a perspective point of view, our results will allow us to further isolate the specific CD4⁺ T cells in order to characterize them at different steps of the disease and during follow-up to better anticipate relapses
CHEVALIER, SYLVIE. "Etude de la tolerance induite par des transfusions sanguines dans un modele de rat : etude de la forme soluble du recepteur a l'il2 dans un modele de rat, etude du deuxieme recepteur t : tcr gamma/delta chez l'homme." Nantes, 1988. http://www.theses.fr/1988NANT2011.
Full textDubois, Aurore. "Régulation des réponses Th2, induite en début de vie, dans un modèle murin d'inflammation pulmonaire." Doctoral thesis, Universite Libre de Bruxelles, 2011. http://hdl.handle.net/2013/ULB-DIPOT:oai:dipot.ulb.ac.be:2013/209971.
Full textTant les nouveaux nés humains que murins ont une plus forte capacité que l’adulte à développer des lymphocytes T CD4+ régulateurs induits par une reconnaissance antigénique. La période néonatale serait donc particulièrement appropriée à l’induction de circuits régulateurs.
Dans le cadre de ce travail, nous avons étudié le rôle des lymphocytes T CD8+, induits à la naissance, dans le contrôle de la réponse des lymphocytes T CD4+ de type Th2.
Des souris BALB/c sont immunisées à la naissance à l’aide de cellules spléniques semi-allogéniques hybrides F1 (AJAX x BALB/c). Ces cellules persistent dans l’animal, au sein des organes lymphoïdes et stimulent ainsi de manière chronique les lymphocytes T CD4+ et T CD8+ du receveur et induisent une réponse de type Th2. Suite à l’injection des cellules spléniques semi-allogéniques au nouveau né de souris, nous avons observé l’expansion d’une population de lymphocytes T CD8+CD25+, dont le phénotype se caractérise par l’expression de Foxp3 et la production conjointe d’IFN-&61543; et l’IL-10. Nous avons pu observer que ces cellules sont capables d’inhiber la production de cytokines Th2 produites par les lymphocytes T CD4+ allospécifiques activés. Par contre, ces cellules régulatrices aggravent des réponses Th2 non apparentées. En effet, suite à une sensibilisation à l’ovalbumine, à l’âge adulte, ces souris développent de plus fortes réponses asthmatiques.
D’autre part, les nouveaux nés de souris BALB/c ont été immunisés à la naissance à l’aide de cellules dendritiques semi-allogéniques hybrides F1 (AJAX x BALB/c) qui activent de manière aigüe leurs lymphocytes T. Ces souris présentent une forte réponse Th1 et Tc1/Tc2 spécifique de l’alloantigène et sont protégées contre le développement d’un asthme induit. Il a aussi été montré dans ce travail que suite à l’immunisation néonatale à l’aide de cellules dendritiques semi-allogéniques, le nombre de lymphocytes T CD8+CD44high, CD8+CD62Lhigh et CD8+CD25+ producteurs d’IFN-&61543; augmente significativement. L’IFN-&
Doctorat en Sciences biomédicales et pharmaceutiques
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Winter, Sarah. "Identification and characterization of new genetic defects involved in Epstein-Barr virus immune response and T-cell proliferation Loss of RASGRP1 in humans impairs T-cell expansion leading to Epstein-Barr virus susceptibility RASGRP1 is a negative factor of EOMES expression in T cells in association with an exhausted phenotype IL-27RA deficiency in humans, a new cause of susceptibility to Epstein-Barr virus infection Association of bi-allelic loss-of-function mutations in PIK3CD and TNFRSF9 causes fatal chronic active Epstein-Barr virus infection with T-cell lymphoproliferation." Thesis, Sorbonne Paris Cité, 2018. http://www.theses.fr/2018USPCB180.
Full textEpstein-Barr virus (EBV) is a gamma-herpes virus that infects 90% of humans without any symptoms in most cases. Some individuals, mostly adolescents, can develop infectious mononucleosis. In immunocompromised individuals, EBV can lead to lymphoproliferative disorders, lymphomas or virus-associated hemophagocytic syndrome. In the past 30 years, several primary immunodeficiencies associated with a high risk to develop EBV-associated disorders have been identified, including SAP, XIAP, ITK, MAGT1, CTPS1, CD27 or CD70 deficiencies. Their characterization has highlighted specific pathways required for efficient immunity to EBV. The objective of this work was to identify new genetic defects associated to a peculiar susceptibility to EBV infection. In two consanguineous families 3 patients developed EBV-associated B cell lymphomas and other EBV-associated lymphoproliferative disorders. By while exome sequencing (WES) we identified two homozygous mutations in RASGRP1 leading to a premature stop codon (A638GfsX16 and S314X). Immunologically these patients presented with CD4+ lymphopenia, low number of naïve T cells and absence of MAIT and iNKT cells. RASGRP1 codes for a diacylglycerol-regulated exchange factor preferentially expressed in T and NK cells, which acts as an activator of the small G protein RAS and the downstream RAF-MEK-ERK kinases cascade (or MAP kinases pathway). Analysis of patients' T cells or control T cells in which RASGRP1 expression was downregulated by short-hairpin RNA technique has highlighted the crucial role of RASGRP1 in T cell proliferation and in the expression of genes known to be involved in cell proliferation or replication such as CTPS1, PCNA or RECQL4. Furthermore, RASGRP1 seems to be a negative regulator of the transcription factor EOMES involved in T cell differentiation. EOMES was found overexpressed in T cells in the absence of RASGRP1. This might explain the skewed effector-memory and exhausted phenotype observed in RASGRP1-deficient patients. In another large consanguineous family two patients developed symptomatic EBV primary infection requiring for one or them anti-CD20 and corticosteroids treatment. Homozygous nonsense mutation leading to a premature stop codon in IL-27RA (G96X) was identified by exome sequencing. No protein expression could be detected in patients' cells. IL-27RA codes for the subunit of IL-27 receptor involved T cell proliferation and Th1 CD4+ development through JAKs/STATs pathway. Stimulation of patients' T cells with IL-27 led to absent JAK/STAT activation pathway and did not enhance their proliferation after anti-CD3 stimulation (contrary to healthy control T cells). Furthermore, Th1 functional defect was found in one patient. These results demonstrate that IL-27RA pathway is deficient is these two patients and that this genetic defect causes their immunodeficiency. Characterization of these two new primary immunodeficiencies associated with a high susceptibility to EBV infection has confirmed the crucial role of T cell proliferation and activation in EBV immune response but has also highlighted new pathways involved in T cell expansion
Olsen, Daniel S. "Nuclear BMP2 and the Immune Response." BYU ScholarsArchive, 2013. https://scholarsarchive.byu.edu/etd/4171.
Full textLeggat, Jamie Alexander. "Innate immunity & CD8+ T lymphocyte regulation of the immune response." Thesis, King's College London (University of London), 2005. http://kclpure.kcl.ac.uk/portal/en/theses/innate-immunity--cd8-t-lymphocyte-regulation-of-the-immune-response(7795ae39-e852-4841-9d6d-18abc9ca849c).html.
Full textHuseby, Eric Sigurd. "Helper and cytotoxic T cell responses specific for myelin basic protein /." Thesis, Connect to this title online; UW restricted, 2000. http://hdl.handle.net/1773/8361.
Full textGodoy, Ramirez Karina. "Flow cytometric methods for assessment of cell-mediated immune responses /." Stockholm, 2005. http://diss.kib.ki.se/2005/91-7140-409-0/.
Full textNoble, Peter Richard. "CD4 T lymphocyte responses to human papillomavirus type 16." Thesis, University College London (University of London), 1999. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.314205.
Full textMarshall, Heather D. "Sensitization of CD8 T Cells During Acute Viral Infections Impacts Bystander and Latecomer CD8 T Cell Responses : A Dissertation." eScholarship@UMMS, 2009. https://escholarship.umassmed.edu/gsbs_diss/440.
Full textMelo, Félix Joana. "Anti-CTLA-4 antibody / CTLA-4 molecule immuno-modulator mechanisms and its consequences on the reinforcement of anti-melanoma immune responses." Thesis, Sorbonne Paris Cité, 2016. http://www.theses.fr/2016USPCC212/document.
Full textMelanoma is a skin cancer with incidence increasing at dramatic rates worldwide. Ipilimumab, an anti-CTLA-4 therapy developed in the view of counter-balancing the inhibitory role of CTLA-4 in T lymphocytes, was the first immune checkpoint inhibitor demonstrating to extend overall survival in patients with metastatic melanoma, with FDA approval in 2011. However, biomarkers allowing the identification of the subset of patients that will more likely benefit from this immunotherapy or that may allow a good monitoring of patient clinical management during treatment are lacking. The principal objective of this work was to identify potential and early predictive biomarkers of ipilimumab response and/or survival in a cohort of 77 metastatic melanoma patients. Firstly, serum levels of melanoma markers such as LDH, S100B and soluble MICA (and its counter-part anti-MICA antibody), tumour markers associated with tumour development and/or immune escape, were assessed. A correlation between lower baseline levels of LDH and S100B, sustained after the first and second doses of ipilimumab, and treatment response and survival was observed, suggesting their potential utility in treatment monitoring. In addition, higher baseline levels of soluble MICA were found to be associated with a less frequency of immune-related adverse events, which might provide important information for the management of frequent ipilimumab-related adverse events. Secondly, immune markers with a special focus on transcription factors, cytokine secretion and chemokine receptors of T lymphocytes and memory T subsets were assessed. An association between baseline absolute lymphocyte counts and extended overall survival as well as better treatment response was found. In addition, a global effect of ipilimumab on the expansion of conventional memory T cells was observed, which was associated with treatment response. By contrast, frequencies of the recently described stem-cell memory T cells were shown to decrease despite increased proliferation, suggesting a process of differentiation. Additionally, ipilimumab induced the expansion of CXCR3, CCR4 and CCR6-expressing T lymphocytes and effector cytokines secretion capacity. Early increased levels of Eomes-expressing CD8+ T cells were found to be associated with disease control. Lastly, and based on the previous results, we investigated the ability of patients’ memory T cells to proliferate under in vitro stimulation. We found that, in contrast to healthy subjects, patients possess a defect in the ability of stem-cell memory T cells expansion in vitro, that might be related to a defect in Eomes and Ki-67 regulation
Beaulieu, Brian L. "Cytotoxic T-Lymphocyte Responses During Acute Epstein-Barr Virus Infection." eScholarship@UMMS, 1996. https://escholarship.umassmed.edu/gsbs_diss/43.
Full textDaigneault, Marc Romeyn. "The characterisation of T-lymphocyte death during the immune response to Streptococcus pneumoniae." Thesis, University of Sheffield, 2011. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.548471.
Full textCallan, Margaret Fiona Clare. "T cell selection in the immune response to antigen." Thesis, University of Oxford, 1996. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.318783.
Full textHoward, Jennifer Ruth. "Role of human gamma-delta T lymphocytes in the instruction of the adaptive immune response against Plasmodium falciparum infection." Thesis, Bordeaux, 2015. http://www.theses.fr/2015BORD0110/document.
Full textP. falciparum derived phosphoantigens (P‐Ag) induce potent activation and expansion of Vγ9Vδ2 T-cells by a poorly described mechanism. Activated Vγ9Vδ2 T cells inhibit the Plasmodium falciparum blood cycle through soluble cytotoxic mediators, abrogating merozoite invasion capacity. In vitro, P-Ag activated Vγ9Vδ2 T lymphocytes have been shown to present antigens and induce αβ T lymphocyte responses, i.e. to act as an antigen presenting cell (APC). Whether this activity can be involved in a pathophysiological context is unknown. The aim of this PhD project is to a) investigate the mechanisms of Vγ9Vδ2 T cell activation by blood stage P. falciparum and b) assess the potential of P. falciparum activated Vγ9Vδ2 T cells to display APC functionality. We show that Vγ9Vδ2 T-cell activation by intact iRBCs is independent of iRBC contact and butyrophilin expression. Blood stage culture supernatants can potently activate Vγ9Vδ2 T-cells and bioactivity is found to be attributable to P-Ags released at the time of parasite egress from the RBC. In vitro iRBC stimulated Vγ9Vδ2 T cells up-regulate surface expression of APC associated markers and can cross-present a model antigen to specific CD8 T cell responders. In vivo we demonstrate an increase in surface expression of APC makers on Vγ9Vδ2 T cells from P. falciparum infected patients.Altogether, these data outline a framework whereby P‐Ag release by iRBC into extracellular milieu can promote activation of distant Vγ9Vδ2 T cells, and opens the door to a new aspect of Vγ9Vδ2 T cell contribution to P. falciparum adaptive immune responses
Broadbent, Suzanne, and n/a. "The Effects of Age and Aerobic Training on T Helper Lymphocyte Proliferation." Griffith University. School of Physiotherapy and Exercise Science, 2004. http://www4.gu.edu.au:8080/adt-root/public/adt-QGU20050113.115912.
Full textBroadbent, Suzanne. "The Effects of Age and Aerobic Training on T Helper Lymphocyte Proliferation." Thesis, Griffith University, 2004. http://hdl.handle.net/10072/366869.
Full textThesis (PhD Doctorate)
Doctor of Philosophy (PhD)
School of Physiotherapy and Exercise Science
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O'Hehir, Robyn Elizabeth. "Polyclonal and monoclonal analysis of the human T lymphocyte immune response to Dermatophagoides spp." Thesis, Imperial College London, 1989. http://hdl.handle.net/10044/1/47596.
Full textMathers, Alicia R. "The effects of the route of viral infection on the balance of T helper immune responses." Morgantown, W. Va. : [West Virginia University Libraries], 2005. https://etd.wvu.edu/etd/controller.jsp?moduleName=documentdata&jsp%5FetdId=3825.
Full textTitle from document title page. Document formatted into pages; contains ix, 155 p. : ill. Vita. Includes abstract. Includes bibliographical references.
Jevon, Marc. "Quality control of the T-cell immune response by tapasin." Thesis, Queen Mary, University of London, 2005. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.422282.
Full textMathew, Anuja. "Human T Cell Responses to Dengue Virus Infections: CD8+CTL and Acute Immunosuppression: a Dissertation." eScholarship@UMMS, 1999. https://escholarship.umassmed.edu/gsbs_diss/18.
Full textANDALUR, NANDAGOPAL Saravanan. "Microfluidics-assisted investigation of T-lymphocyte Migration in lymph node relevant chemokine gradients." PLoS ONE, 2011. http://hdl.handle.net/1993/23247.
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