Určení dárcovsky specifické T buněčné aloreaktivity u pacientů po transplantaci ledviny s diagnózou hraničních změn / Donor specific T cell alloreactivity in kidney transplant recipients with borderline changes

Šilhová, Markéta

January 2020

After kidney transplantation the recipient's immune system responds to the donor's antigens and the graft rejection occurs. Borderline changes are a frequent diagnosis after kidney transplantation, representing only mild rejection signs. Some patients with borderline changes undergo progression to rejection. The identification of these at- risk patients by biomarkers will allow enhanced treatment and help to prevent the development of rejection. The aim of my work was to verify biomarkers of rejection in patients with borderline changes. Chemokines CXCL9, CXCL10 and CCL17 in urine/serum of 40 patients with subclinical borderline changes at 3 months and in 25 patients with early borderline changes were determined by ELISA. At 3 months, the higher CXCL10 level predicted rejection with AUC=0.749, p=0.024. High levels of CXL10 had also been found in patients with BKV infection. We did not confirm the relationship between rejection and the CXCL9 and CCL17. In the early posttransplant period the levels of CXCL10 and CXCL9 were elevated in all patients and therefore couldn't be used to predict rejection. The alloreactivity was examined using IFN-γ ELISPOT (n=38). No association between the frequency of IFN-γ producing cells after stimulation with donor cells or CMV peptides and the development of...

Untersuchungen zur Eignung von Interferon-gamma release assays zum Nachweis von M. tuberculosis-reaktiven T-Lymphozyten

Müller, Bert

28 May 2021

Gegenstand dieser Arbeit ist die Untersuchung zellulärer Testsysteme bei Patienten mit Verdacht auf latente Infektion mit M. tuberculosis. Eine latente Tuberkulose kann unter Immunsuppression zu einer aktiven Tuberkulose werden. Deshalb wird bei immunsuppressiven Therapien insbesondere mit TNF-alpha-Blockern eine Chemoprävention empfohlen. Daher ist es sehr wichtig, latente Infektionen zu erkennen. Ist ein Patient mit M. tuberculosis infiziert, reagieren seine T-Zellen auf Stimulation mit Antigenen wie ESAT-6 und CFP-10. Diese Immunantwort ist die Grundlage der modernen IFN-γ release Assays (IGRA). ESAT-6 und CFP-10 fehlen bei allen BCG-Stämmen und bei den meisten nicht-tuberkulösen Mykobakterien mit Ausnahme von M. kansasii, M. szulgai und M. marinum (Andersen et al. 2000; Behr et al, 1999; Lalvani 2003). Im Gegensatz dazu haben Personen, die mit M. tuberculosis-Komplex-Organismen infiziert sind, in der Regel T-Zellen im Blut, die diese und andere mykobakterielle Antigene erkennen. Ziel der vorliegenden Arbeit war es, die Nutzung von IGRA in der medizinischen Labordiagnostik dahingehend zu analysieren, ob es Unterschiede zwischen ELISPOT-basierten Tests und Röhrchen-Tests als Testformat gibt, inwieweit diese Tests im klinischen Alltag verlässlich sind und ob sich mit einem anderen Auswertealgorithmus eine sicherere Aussage zum Vorliegen einer latenten Tuberkulose treffen lässt. Im Einzelnen wurden dabei drei Ansätze verfolgt: 1. In einer retrospektiven Studie wurden die Ergebnisse von 2686 Patienten ausgewertet, die im Labor des Instituts für Klinische Immunologie des Universitätsklinikums Leipzig von 2013 bis 2016 als Routineuntersuchungen erhoben wurden. Bei klinisch unplausiblen Ergebnissen wurden bei einem Teil der Patienten eine Wiederholungsuntersuchungen durchgeführt. Die analytische Sensitivität und Spezifität sowie den positiven und negativen prädiktiven Wert konnten wir nur unter der Annahme abschätzen, dass der Ausfall in der Wiederholungsuntersuchung einen Hinweis auf falsch- oder richtig-positive oder -negative Werte zulässt. Wir kommen damit zu einer Sensitivität von nur 28 %, einer Spezifität von immerhin 91 %, einem positiven prädiktiven Wert von 32 % und einem negativen prädiktiven Wert von 90 %. Damit sind 68 % der positiven Werte falsch positiv und 10 % der negativen Werte falsch negativ. Unsere Untersuchungen zur Wiederholbarkeit der ELISPOT-Tests im eigenen Labor bestätigen, dass negative Ergebnisse meist wiederholbar sind, positive Werte jedoch skeptisch betrachtet werden müssen. 2. Seit 2012 sendet Instand e.V. zweimal jährlich Ringversuchsproben für den IGRA aus (Ringversuch 650, https://www.instand-ev.de/). Wir analysierten, wie viele Labors bei Teilnahme an der externen Qualitätssicherung (sogenannten Ringversuchen) für IGRA ein korrektes Ergebnis erzielt hatten und ob Unterschiede zwischen ELISPOT-Assay und Röhrchen-Test bestehen. Im Ringversuch waren die Ergebnisse von ELISPOT (z.B. TB-Spot, Oxford Immunotec) und Röhrchentest (Quantiferon Gold bzw. Gold-Plus, Qiagen oder Diasorin) bis auf den 2. Ringversuch 2019 vergleichbar und unterschieden sich nicht. 3. Obwohl die meisten Labore an den Ringversuchen erfolgreich teilnehmen, ist die recht häufige Anzahl vor allem falsch positiver Ergebnisse im diagnostischen Alltag problematisch. Wir haben daher in einem dritten Untersuchungsschritt die Validierungsdaten eines Labors detailliert untersucht, um ein definiertes Verfahren zur Ermittlung positiver Testergebnisse vorzuschlagen. Zwischen 2011 und 2013 erfolgte im Labor Ettlingen eine umfangreiche Qualitätssicherung des ELISPOT unter Nutzung von 70 Proben in Doppelbestimmung. Dabei wurden jeweils die Messungen für die Positiv- und die Negativkontrolle sowie die Werte nach Stimulation mit ESAT-6 und CFP-10 analysiert. Um relevante Unterschiede zwischen Negativkontrolle und der eigentlichen Messung zu bewerten, wurden die Unterschiede mit der Wiederholpräzision in Beziehung gesetzt: Die Unterschiede sollten größer sein als die daraus abgeleitete Ungenauigkeit (Impräzision) der Messungen. Daraus wurde ein Cut-off-Wert kalkuliert, der unmittelbar auf den Daten des Labors beruht. Hierzu ist die Homogenität der Standardabweichungen über alle Proben erforderlich. Sie wird durch die Wurzeltransformation aller Daten erreicht. Für die verwendeten Daten ist sie anwendbar (Altman 1991, Bland 2000). Dies bedeutete bei den untersuchten Daten, dass bei Doppelbestimmungen die Unterschiede zwischen dem Testergebnis immer um den Faktor 0,76 größer sein muss als die Negativkontrolle. Dazu sind allerdings zwei Voraussetzungen zu erfüllen: 1. die Werte müssen vor Analyse wurzeltransformiert werden. 2. benötigt werden mindestens Doppelbestimmungen. Da keine Doppelbestimmungen vorliegen, konnte das Verfahren nicht an einem eigenen Datensatz verifiziert werden. Wir schlussfolgern daraus zusammenfassend: 1. in der Praxis gibt es keine wesentlichen Unterschiede zwischen ELISPOT und Röhrchen-Test als Testformat, was Sensitivität und Spezifität anbelangt 2. IGRAs sind ein verlässliches Werkzeug im klinischen Alltag, insbesondere wenn es um den Ausschluss einer latenten Tuberkulose geht 3. die Auswertung von ELISPOT-Daten lässt sich über Mehrfachbestimmung und quadratwurzeltransformierte Auswertung optimieren (wobei das noch in einer Folgearbeit zu beweisen ist).:Inhalt Abkürzungsverzeichnis 3 1 EINFÜHRUNG 5 1.1 Epidemiologie der Tuberkulose 5 1.2 Pathogenese der Tuberkulose 8 1.3 Prävention der Tuberkulose 10 1.4 Diagnostik der Tuberkulose 11 1.4.1 Radiologische Untersuchungen 12 1.4.2 Mikrobiologische Untersuchungen 12 1.4.3 Molekularbiologischer Nachweis 13 1.5 Nachweis der Immunreaktion gegenüber M. tuberculosis 14 1.5.1 Tuberkulin-Hauttest 14 1.5.2 Serologische Tests auf M. tuberculosis-Infektion 16 1.5.3 Zelluläre Labortests auf M. tuberculosis-Reaktivität 18 2 AUFGABENSTELLUNG 22 3 MATERIAL UND METHODEN 23 3.1 Patienten 23 3.2 Blutentnahme und Zellpräparation 23 3.3 ELISPOT 25 3.4 Ringversuch zur externen Qualitätssicherung 26 3.5 Retrospektive Analyse der Daten des eigenen Labors und der Ringversuchsdaten 26 3.6 Analyse der Validierungsdaten aus Ettlingen 27 4 ERGEBNISSE 29 4.1 Analyse der ELISPOT-Daten des eigenen Labors 29 4.2 Ergebnisse des Instand-Ringversuchs 33 4.3 Analyse der ELISPOT-Wiederholungsmessungen 35 5 DISKUSSION 41 6 Zusammenfassung 48 Literaturverzeichnis 52 Lebenslauf 63 Danksagung 64 Erklärung über die eigenständige Abfassung der Arbeit 65

info:eu-repo/classification/ddc/610

ddc:610

AUTOANTIBODIES AND AUTOREACTIVE B CELLS IN THE BONE MARROW AND THE PERIPHERAL BLOOD OF PATIENTS WITH IMMUNE THROMBOCYTOPENIA / AUTOREACTIVE B CELLS IN IMMUNE THROMBOCYTOPENIA

Shrestha, Sabrina

January 2019

Introduction: Immune thrombocytopenia (ITP) is an autoimmune bleeding disorder characterized by a platelet count less than 100 x 109/L. Platelet-bound autoantibodies are detected in the peripheral blood of only 40-50% of ITP patients. The subset of ITP patients who do not have detectable autoantibodies may truly be seropositive, but autoantibodies may not be detected due to limitations of the assays. Studies have also suggested that autoantibodies might be sequestered in the bone marrow where autoantibodies may impair platelet production. In addition, detecting autoreactive antibody-secreting B cells using the Enzyme-linked Immunospot (ELISPOT) assay was shown to be highly sensitive. In this study, the bone marrow and the peripheral blood compartments of ITP patients were tested for the presence of anti-GPIIbIIIa and anti-GPIbIX IgG autoantibodies and autoreactive B cells. Methods: Bone marrow aspirate and peripheral blood samples were collected from ITP patients (n=12), non-immune thrombocytopenic patient controls (n=3), and healthy controls (n=5). Mononuclear cells were isolated and tested for the presence of anti-GPIIbIIIa and anti-GPIbIX IgG autoreactive B cells before stimulation and after stimulation with R848 and IL-2 using the ELISPOT assay. Anti-GPIIbIIIa and anti-GPIbIX IgG autoantibodies were detected in the bone marrow and the peripheral blood using the direct antigen capture assay. Results: In our study, we detected autoantibodies and autoreactive B cells of known specificity in the bone marrow of a subset of ITP patients. Detecting anti-GPIIbIIIa and anti-GPIbIX autoantibodies in the bone marrow or the peripheral blood had a sensitivity of 42% and testing both compartments increased the sensitivity to 58%, while maintaining 100% specificity. Autoreactive B cells were detected at low frequencies with low specificity in the bone marrow and the peripheral blood of a subset of ITP patients. The majority of the ITP patients without detectable autoantibodies in the peripheral blood did not have autoantibodies in the bone marrow, and autoreactive B cells were not detected in either compartment. Conclusion: Examining both the bone marrow and the peripheral blood compartments for autoantibodies or autoreactive B cells increased the sensitivity. Furthermore, detecting autoantibodies using the antigen capture assay is more sensitive and specific than detecting autoreactive B cells using the ELISPOT assay. / Thesis / Master of Science (MSc)

Immune thrombocytopenia

Autoantibodies

Bone Marrow

B Cells

Platelets

Translational

Hematology

ELISPOT assay

Funcionalidade das células Natural Killer  T -- NKT - na fisiopatogenia da Mielopatia associada ao HTLV/ Paraparesia Tropical Espástica (HAM/TSP) / Functionality of natural killer T cells - NKT - on physiopathogeny of HTLV Associated Myelopathy/Tropical Spastic Paraparesis (HAM/TSP)

Semeão, Lucas Emmanuel da Silva

05 March 2015

A HAM/TSP é uma doença de caráter neurológico que acomete aproximadamente 5% dos infectados pelo vírus HTLV, afetando-os principalmente em sua capacidade locomotora. Não são conhecidos até o momento os fatores que fazem o indivíduo infectado desenvolver ou não as patologias associadas ao vírus. Nesse contexto, estudamos a participação das células natural killer T (NKT) visando contribuir na elucidação da patogênese da paraparasia espática tropical HAM/TSP. As células natural killer T (NKT) são um subtipo de linfócitos T, com capacidade efetora e auxiliar, e está associado à doenças infecciosas, alergias e a doenças autoimunes, e a hipótese deste trabalho é que elas participem da progressão da HAM/TSP. Após realizarmos testes para avaliação da ativação das NKT (PD-1), bem como avaliar sua capacidade de secretar IFN- y e Granzima B concluimos que as mesmas não possuem potencial de ativação na periferia e pressupomos que estas podem estar no sítio acometido pela patologia, o SNC. Neste contexto, nosso estudo acrescenta informações quanto à patogenia da HAM/TSP e contribui com conhecimento para a futura elucidação da doença / The HAM/TSP is a neurological disease that affects approximately 5% of HTLV infected individuals, especially in their locomotor capacity. They are not known yet the factors that make the infected individual to develop or not the pathologies associated with virus. In this context, we study the participation of natural killer T cells (NKT), trying to contribute to clarify the HAM/TSP pathogenesis. NKT cells are a subtype of lymphocytes with effector and helper capacities, and are associated with infectious, allergies and autoimmune diseases. Our hypothesis is that they participate in the progression of HAM/TSP. After evaluate the activation of NKT through PD-1 marker, as well evaluate assess their ability to secrete IFN-y and Granzyme B, we conclude that the NKT cells lack periphery in activation potential, and presuppose that they are present at the central nervous system, the site affected by the disease. In this context, our study adds information on the pathogenesis of HAM / TSP and contributes knowledge for future elucidation of disease

Células T matadores naturais

Citometria de fluxo

Elispot

Elispot

Flow cytometry

Human T-lymphotropic virus 1

Immunology

Imunologia

Natural killer T cells

Paraparesia espástica tropical

Paraparesis tropical spastic

Vírus 1 linfotrópico T humano

Funcionalidade das células Natural Killer  T -- NKT - na fisiopatogenia da Mielopatia associada ao HTLV/ Paraparesia Tropical Espástica (HAM/TSP) / Functionality of natural killer T cells - NKT - on physiopathogeny of HTLV Associated Myelopathy/Tropical Spastic Paraparesis (HAM/TSP)

Lucas Emmanuel da Silva Semeão

05 March 2015

A HAM/TSP é uma doença de caráter neurológico que acomete aproximadamente 5% dos infectados pelo vírus HTLV, afetando-os principalmente em sua capacidade locomotora. Não são conhecidos até o momento os fatores que fazem o indivíduo infectado desenvolver ou não as patologias associadas ao vírus. Nesse contexto, estudamos a participação das células natural killer T (NKT) visando contribuir na elucidação da patogênese da paraparasia espática tropical HAM/TSP. As células natural killer T (NKT) são um subtipo de linfócitos T, com capacidade efetora e auxiliar, e está associado à doenças infecciosas, alergias e a doenças autoimunes, e a hipótese deste trabalho é que elas participem da progressão da HAM/TSP. Após realizarmos testes para avaliação da ativação das NKT (PD-1), bem como avaliar sua capacidade de secretar IFN- y e Granzima B concluimos que as mesmas não possuem potencial de ativação na periferia e pressupomos que estas podem estar no sítio acometido pela patologia, o SNC. Neste contexto, nosso estudo acrescenta informações quanto à patogenia da HAM/TSP e contribui com conhecimento para a futura elucidação da doença / The HAM/TSP is a neurological disease that affects approximately 5% of HTLV infected individuals, especially in their locomotor capacity. They are not known yet the factors that make the infected individual to develop or not the pathologies associated with virus. In this context, we study the participation of natural killer T cells (NKT), trying to contribute to clarify the HAM/TSP pathogenesis. NKT cells are a subtype of lymphocytes with effector and helper capacities, and are associated with infectious, allergies and autoimmune diseases. Our hypothesis is that they participate in the progression of HAM/TSP. After evaluate the activation of NKT through PD-1 marker, as well evaluate assess their ability to secrete IFN-y and Granzyme B, we conclude that the NKT cells lack periphery in activation potential, and presuppose that they are present at the central nervous system, the site affected by the disease. In this context, our study adds information on the pathogenesis of HAM / TSP and contributes knowledge for future elucidation of disease

Células T matadores naturais

Citometria de fluxo

Elispot

Imunologia

Paraparesia espástica tropical

Vírus 1 linfotrópico T humano

Elispot

Flow cytometry

Human T-lymphotropic virus 1

Immunology

Natural killer T cells

Paraparesis tropical spastic

Suivi fonctionnel de la greffe d'îlots de Langerhans : interêt de l'imagerie IRM et de l'immuno-monitoring cellulaire / Monitoring of Langerhans islet transplantation : MRI imaging and cellular immune monitoring efficiency

Chopard-Lallier, Sophie

07 May 2013

La greffe d'îlots de Langerhans permet de traiter le diabète de type 1 en restituant une insuline-sécrétion. La moitié des patients reprend l'insuline dans les 5 ans. Cette perte de fonction s'explique par l'absence d'outils de monitoring. Le but de notre travail était de déterminer l'efficacité de l'IRM à diagnostiquer un rejet de greffe, et d'évaluer l'intérêt du monitoring cellulaire chez les patients.Imagerie IRM chez le ratMéthodes : Des îlots syngéniques, allogéniques ou xénogéniques ont été greffés par voie intra-portale à des rats diabétiques après marquage avec une nanoparticule de fer (ferucarbotran). Les IRM étaient réalisées dans une IRM clinique 3T.Résultats : La décroissance du signal était différente suivant les 3 types de greffes. Le signal IRM des greffes allogéniques était significativement plus bas à J4 alors que la glycémie était normale. En prenant un seuil de 84% à J4, l'IRM permet d'obtenir une sensibilité de 91% et une spécificité de 70% Innnuno-monitoring cellulaireMéthodes : Des réactions lymphocytaires mixtes étaient réalisées entre les PBMC des patients greffés, et les splénocytes des donneurs. La réaction immunitaire était évaluée par la sécrétion d'IFNy (ELISpot), par la prolifération cellulaire (cytométrie du flux du Ki67), et par le dosage des cytokines (Bioplex). Le résultat était corrélé à la fonction du greffon évaluée par le (3-score).Résultats : Les patients avec une mauvaise fonction montraient une plus grande réactivité anti-donneur avec l'ELISpot IFNy (p=0,007, r=-0,50) et l'index de prolifération (p=0,006, r=-0,51). Les patients avec une mauvaise fonction avaient des taux d'IFNy, IL-5 et IL-17 plus élevés. / Langerhans islet transplantation allows curingtype 1 diabetes by restoring an endogenous insulin secretion. Halfof patients will resume insulin withinyears. This loss of function may be explained by the lack of monitoring tools able to diagnose an ongoing graft failure. The aims of our work were toevaluate the efficiency of MRI to diagnose islet graft rejection, and to assess the feasibility of immune cellular monitoring in transplanted patients.MRI in the rat mortelMethods: Syngeneic, allogeneic and xenogeneic islets were transplanted intra-portally to diabetic rats after labeling with superparamagnetic ironoxide nanoparticles (ferucarbotran). Images were acquired on a clinical 3T MRI scanner.Results: The signal decreasing was different between the 3 types of transplantations. At day 4, the MRI signal in allogeneic group was significantlylower while glycaemia remained normal. With a cut-off value of 84% at day 4, sensitivity of 91% and specificity of 70% were obtained.Cellular immune monitoringMethods: Mixed lymphocyte cultures were performed with peripheral blood mononuclear cells from recipients and splenocytes from donors. Immunereactivity was assessed by the release of IFNy (ELISpot), cell prolifération (flow cytometry of Ki67), and cytokine quantification (Bioplex). Theresults were correlated to the islet graft function assessed by (5-score.Results: Patients with low islet function showed higher cellular reactivity against donor cells assessed by ELISpot IFNy ((p=0,007, r=-0,50) andproliferation index (p=0,006, r=-0,51). Patients with low graft function had higher levels of IFNy, IL-5 and 1L-17.

Greffe d'îlots

Diabète de type 1

IRM

Nanoparticules de fer

Ferucarbotran

ELISpot IFNv

Rejet de greffe

Monitoring immunologique

Blet Transplantation

Type 1 diabètes

MRI

Ferucarbotran

ELISpot IFNy

Graft rejection

Immune monitoring

612.4

The relationship between Cytomegalovirusspecific cellular immune response and CD4+ T cell count in HIV positive individuals in a South African setting

Arendse, Germaine Veronique

03 1900

Thesis (MScMedSc)--University of Stellenbosch, 2011. / ENGLISH ABSTRACT: Introduction: Reactivation of human cytomegalovirus (HCMV) infection in individuals infected with human immunodeficiency virus (HIV) may lead to life-threatening end-organ diseases (EOD). The EOD becomes clinically apparent when a critical number of cells in the affected organs become damaged as a consequence of HCMV-infection. Treatment of the HCMV-associated disease at this point may not be effective. Therefore, early detection of HCMV reactivation may be useful to guide pre-emptive therapy. Aim: The aim of this study was to determine whether there is a point at which the HCMV-specific cellular immune response breaks down, as determined by the interferon-gamma (IFN-γ) enzyme-linked immunospot (ELISPOT) assay, and HCMV reactivation occurs in HIV-positive, antiretroviral therapy (ART)-naïve individuals in a South African setting. This was done in relation to the CD4+ T cell count and the HCMV viral load as determined by real-time polymerase chain reaction (qPCR). Materials and methods: Fifty-two (52) HIV-infected, ART-naïve subjects were recruited from primary healthcare centres that they attended for the management of their HIV infection. Heparinised blood samples were collected to quantify the HCMV-specific cellular immune response using the IFN-γ-ELISPOT assay and to determine the HCMV IgG serostatus. Ethylenediaminetetraacetic acid (EDTA) blood samples were collected for the determination of the CD4+ T cell counts and the HCMV viral loads. Results: All 52 subjects recruited were confirmed to be HIV-HCMV co-infected based on their HCMV IgG serostatus. The results of 34 subjects with completed data sets were analysed. The CD4+ T cell counts of these subjects ranged from 10 to 784 cells/μl. Twenty-two (22) (65%) subjects had positive HCMV IFN-γ-ELISPOT results with 94% having no detectable HCMV viral loads. All subjects (28) with a CD4+ T cell count above 100 cells/μl had undetectable HCMV viral loads. Two of the six subjects with CD4+ T cell counts <100 cells/μl had detectable HCMV viral loads. There was no statistically significant association between the CD4+ T cell counts and the HCMV IFN-γ-ELISPOT results. Conclusion: No specific point could be determined when there is loss of integrity of the HCMV-specific cellular immune response in HIV-positive individuals. Low CD4+ T cell counts did not correlate with HCMV IFN-γ-ELISPOT results suggesting that the HCMV-specific cellular immunity did not necessarily break down at low CD4+ T cell counts. Nevertheless, a CD4+ T cell count above 100 cells/μl appeared to be protective against viraemia as determined by the HCMV viral load qPCR. The IFN-γ-ELISPOT assay was employed as a tool to determine the integrity of the HCMV-specific cellular immune response in HIV-positive individuals. However, the IFN-γ-ELISPOT assay should be used in conjunction with the CD4+ T cell count and the HCMV viral load qPCR to determine when there is loss of integrity of the HCMV-specific cellular immune response and HCMV reactivation occurs. This may assist clinicians in their choice of management and appropriate pre-emptive treatment in the HIV-HCMV co-infected individual at a risk for HCMV reactivation. / AFRIKAANSE OPSOMMING: Inleiding: Heraktivering van menslike sitomegaalvirus (MSMV) in menslike immuniteitsgebreksvirus (MIV)-MSMV ko-geïnfekteerde individue kan lei tot dodelike end-orgaan siektes (EOS). Die EOS word klinies duidelik wanneer 'n kritieke aantal selle in die organe beskadig raak as gevolg van die MSMV-infeksie. Behandeling van die MSMV-verwante siekte op hierdie punt mag moontlik nie meer effektief wees nie. Daarom kan die vroeë opsporing van MSMV heraktivering nuttig wees in die gebruik van voorkomende terapie. Doel: Die doel van hierdie studie is om die punt te bepaal wanneer die MSMV-spesifieke sellulêre immuun reaksie afgebreek word met behulp van die interferon gamma (IFN-γ) ensiem-gekoppelde immunospot (ELISPOT) toets en MSMV heraktivering voorkom in MIV-positiewe, antiretrovirale terapie (ART)-naïewe individue in' n Suid-Afrikaanse instelling. Dit word gedoen in verhouding met die CD4+ T sel telling en die MSMV virale lading. Materiale en metodes: Twee-en-vyftig (52) MIV-geïnfekteerde, ART-naïewe pasiënte is vanaf primêre gesondheidsentrums, wat hul bywoon vir die behandeling van hul MIV infeksie, genader. Gehepariniseerde bloedmonsters is gebruik om die MSMV-spesifieke sellulêre immuun reaksie met behulp van die IFN-γ-ELISPOT toets en die MSMV IgG serostatus te bepaal. Etileendiamientetra-asynsuur (EDTA) bloed monsters is versamel vir die bepaling van hul CD4+ T sel telling en hul MSMV virale lading met behulp van die ―real-time‖ polimerase kettingreaksie (qPKR) waardes. Resultate: Al 52 pasiënte is bevestigde MIV-MSMV ko-infeksies, gebasseer op hul serologiese status. Die resultate van 34 pasiënte met voltooide data is ontleed. Die CD4+ T sel tellings van hierdie pasiënte het gewissel 10-784 selle/μl. Twee-en-twintig (22) (65%) pasiënte het positiewe MSMV IFN-γ-ELISPOT resultate met 94% wat ‗n negatiewe qPKR resultate. Alle pasiënte (28) met 'n CD4+ T-seltelling bo 100 selle/μl het' n negatiewe qPKR resultate. Twee van die ses pasiënte met 'n CD4+ T-seltelling <100 selle/μl het waarneembare MSMV virale ladings oor die qPKR. Daar was geen statisties beduidende assosiasie tussen die CD4+ T sel tellings en die MSMV IFN-γ-ELISPOT resultate nie. Gevolgtrekking: Geen spesifieke punt wanneer die MSMV-spesifieke sellulêre immuun reaksie afgebreek word kon in MIV-positiewe individue bepaal word nie. Lae CD4+ T sel tellings het nie ooreengestem met die MSMV IFN-γ-ELISPOT resultate nie en dui daarop dat die MSMV-spesifieke sellulêre immuniteit nie noodwendig afgebreek word teen 'n lae CD4+ T sel tellings nie. Tog blyk 'n CD4+ T-seltelling bo 100 selle/μl om beskerming teen viremie te bied. Die meriete van die gebruik van die IFN-γ-ELISPOT toets die integriteit van die MSMV-spesifieke sellulêre immuun response in MIV-positiewe individue te bepaal, is waargeneem in die opgehoopte data. Tog kan die gebruik van die IFN-γ-ELISPOT toets in samewerking met die CD4+ T sel telling en die MSMV virale lading meer voordelig in die bepaling van 'n punt wanneer die MSMV-spesifieke sellulêre immuun reaksie afbreek en herstel plaasvind. Dit kan help om klinici in hul keuse van bestuur en gepaste voorkomende behandeling in die MIV-MSMV mede-geïnfekteerde individu op 'n risiko vir herstel.

HCMV HIV ELISPOT CD4+T-cell

HIV infections -- Management

Theses -- Virology

Dissertations -- Virology

Medical Virology

Role B buněk v transplantačních reakcích / The role of B cells in transplantation reactions

Brožová, Jitka

January 2014

Kidney transplantation is the best treatment for patients with end-stage renal failure. The main problem of kidney transplantation is however the development of a cellular and antibody-mediated (humoral) rejection. During the last decade, thanks to the advanced immunosuppression, prognosis of survival and function of transplanted organs has significantly improved. Nevertheless, humoral rejection remains very serious obstacle in high-risk patients, because it can permanently damage the graft. Therefore, before transplantation it is necessary to stratify patients into high and low risk groups for development of antibody-mediated rejection. Current immunogenetic tests performed before transplantation include, in addition to HLA typing, detection of panel-reactive antibodies. However, this test does not provide information about B cells which participate in the humoral response of the kidney recipient. Therefore, in the presented thesis we studied B cell reactivity and its regulation in transplanted patients. In this retrospective analysis we measured levels of the B cell activating factor, a cytokine regulating the function of B lymphocytes (BAFF). Current reports suggest that BAFF could serve as a marker of humoral rejection. Furthermore, we focused on B lymphocytes and their capacity to produce...

Resposta imune celular contra peptídeos crípticos do HIV-1 / Cellular immune response against HIV-1 cryptic peptides

Hong, Marisa Ailin

15 December 2014

INTRODUÇÃO E OBJETIVOS: Uma fonte secundária e não convencional de peptídeos que se ligam as moléculas MHC de classe I tem sido descrita como responsável por produzir peptídeos crípticos. Esses peptídeos são imunogênicos e portanto, capazes de induzir uma resposta imunológica por células T e assim, contribuir com a resposta total exercida pelas células T CD8+, colaborando na pressão que leva HIV-1 ao processo de mutação, e consequentemente ao escape viral. Alguns pacientes, que correspondem a menos de 5% da população infectada, são capazes de naturalmente controlar a progressão da doença, mantendo a contagem de célula T CD4+ acima de 500 células/uL ou mantendo a carga viral abaixo de 2.000 cópias/mL, por ao menos 12 meses, sem ser submetido a tratamento com antirretrovirais ou esquema HAART. Avaliar a resposta imunológica destes pacientes, controladores da infecção, contra peptídeos crípticos pode nos fornecer informações importantes que colaborem com o desenvolvimento de novas estratégias preventivas. METODOLOGIA: A resposta imunológica contra peptídeos crípticos, estes derivados da transcrição da seqüência consenso e da seqüência inversa do gene do HIV-1, foram avaliados em vários conjuntos (pools), utilizando amostras coletadas de pacientes controladores, tanto avirêmicos, também conhecidos como controladores de elite (carga viral < limite de detecção), bem como virêmicos (carga viral < 2.000 cópias/mL) e, de pacientes progressores. Foi observada que a resposta imunológica contra peptídeos crípticos é mais freqüente, com maior amplitude e magnitude entre os pacientes controladores comparados ao que foi observado entre pacientes progressores. Esta resposta, entretanto, parece inverter ao longo da infecção, como observada utilizando as amostras coletadas em momento tardio da infecção, onde os controladores parecem perder sua capacidade de responder aos peptídeos crípticos, enquanto que os progressores desenvolveram resposta, ressaltando que os pools indutores de resposta nas duas fases foram diferentes. Sugerindo que a resposta imunológica contra peptídeos crípticos pode exercer papel importante de pressão sobre o vírus, levando-o ao processo de escape viral. CONCLUSÔES E IMPORTÂNCIA: Peptídeos crípticos são capazes de induzir resposta imunológica e colaborar para explicar como ocorre a seleção de alguns vírus, seja este devido à mudança na expressão das proteínas principais do HIV-1, seja diretamente gerando vírus defeituoso e não infectante. Os peptídeos crípticos podem ser incluídos em desenhos de vacina, com o intuito de aumentar a amplitude e a magnitude da resposta imunológica por células T e consequentemente, aumentar a proteção contra infecção ou progressão da infecção pelo HIV-1 / BACKGROUND: A second and unconventional source of peptides that bind to MHC class I molecule has been described to produce cryptic peptides, which are immunogenic and are able elicit T cell response, that contributes to total CD8+ T cell immune response and then exert mutation pressure on HIV-1, leading to virus escape. Some rare patients, less than 5% of infected population, are naturally able to control disease progression, either maintaining CD4+ T cells over 500 cells/uL or viral load under 2,000 copies/mL, without being treated with HAART, for at least 12 months. Understanding their immune response to cryptic peptides might be a great value to help on developing better prevention strategies. METHODOLOGY: Immune response to cryptic peptides, derived from sense and antisense transcription of HIV-1, was evaluated in pools using samples from Elite (aviremic) or HIV (viremic, < 2,000 copies/mL) controllers and progressors. Immune response to cryptic peptides are more frequent, with a larger breadth and of greater magnitude in controllers than in progressors, and this response is inversed seen in a later time point, when controllers seems to lose this response, while progressors developed it, showing cryptic peptides immune response to different pools, suggesting that immune response to cryptic peptides might play some role in pressuring the virus mutation escape. CONCLUSIONS AND SIGNIFICANCE: cryptic peptides can elicit immune response and help to explain how some virus selection happens, either by changing expression of crucial HIV-1 proteins or generating defective virus. They can be included in vaccine design for enhancing the magnitude and breadth of T cell immune response and consequently the protection against infection or progression of HIV-1 infection

Antígenos HIV

ELISPOT

Enzyme-linked immunospot assay

HIV antigens

HIV infections

HIV-1

HIV-1

Infecções por HIV

Resposta imune celular contra peptídeos crípticos do HIV-1 / Cellular immune response against HIV-1 cryptic peptides

Marisa Ailin Hong

15 December 2014

INTRODUÇÃO E OBJETIVOS: Uma fonte secundária e não convencional de peptídeos que se ligam as moléculas MHC de classe I tem sido descrita como responsável por produzir peptídeos crípticos. Esses peptídeos são imunogênicos e portanto, capazes de induzir uma resposta imunológica por células T e assim, contribuir com a resposta total exercida pelas células T CD8+, colaborando na pressão que leva HIV-1 ao processo de mutação, e consequentemente ao escape viral. Alguns pacientes, que correspondem a menos de 5% da população infectada, são capazes de naturalmente controlar a progressão da doença, mantendo a contagem de célula T CD4+ acima de 500 células/uL ou mantendo a carga viral abaixo de 2.000 cópias/mL, por ao menos 12 meses, sem ser submetido a tratamento com antirretrovirais ou esquema HAART. Avaliar a resposta imunológica destes pacientes, controladores da infecção, contra peptídeos crípticos pode nos fornecer informações importantes que colaborem com o desenvolvimento de novas estratégias preventivas. METODOLOGIA: A resposta imunológica contra peptídeos crípticos, estes derivados da transcrição da seqüência consenso e da seqüência inversa do gene do HIV-1, foram avaliados em vários conjuntos (pools), utilizando amostras coletadas de pacientes controladores, tanto avirêmicos, também conhecidos como controladores de elite (carga viral < limite de detecção), bem como virêmicos (carga viral < 2.000 cópias/mL) e, de pacientes progressores. Foi observada que a resposta imunológica contra peptídeos crípticos é mais freqüente, com maior amplitude e magnitude entre os pacientes controladores comparados ao que foi observado entre pacientes progressores. Esta resposta, entretanto, parece inverter ao longo da infecção, como observada utilizando as amostras coletadas em momento tardio da infecção, onde os controladores parecem perder sua capacidade de responder aos peptídeos crípticos, enquanto que os progressores desenvolveram resposta, ressaltando que os pools indutores de resposta nas duas fases foram diferentes. Sugerindo que a resposta imunológica contra peptídeos crípticos pode exercer papel importante de pressão sobre o vírus, levando-o ao processo de escape viral. CONCLUSÔES E IMPORTÂNCIA: Peptídeos crípticos são capazes de induzir resposta imunológica e colaborar para explicar como ocorre a seleção de alguns vírus, seja este devido à mudança na expressão das proteínas principais do HIV-1, seja diretamente gerando vírus defeituoso e não infectante. Os peptídeos crípticos podem ser incluídos em desenhos de vacina, com o intuito de aumentar a amplitude e a magnitude da resposta imunológica por células T e consequentemente, aumentar a proteção contra infecção ou progressão da infecção pelo HIV-1 / BACKGROUND: A second and unconventional source of peptides that bind to MHC class I molecule has been described to produce cryptic peptides, which are immunogenic and are able elicit T cell response, that contributes to total CD8+ T cell immune response and then exert mutation pressure on HIV-1, leading to virus escape. Some rare patients, less than 5% of infected population, are naturally able to control disease progression, either maintaining CD4+ T cells over 500 cells/uL or viral load under 2,000 copies/mL, without being treated with HAART, for at least 12 months. Understanding their immune response to cryptic peptides might be a great value to help on developing better prevention strategies. METHODOLOGY: Immune response to cryptic peptides, derived from sense and antisense transcription of HIV-1, was evaluated in pools using samples from Elite (aviremic) or HIV (viremic, < 2,000 copies/mL) controllers and progressors. Immune response to cryptic peptides are more frequent, with a larger breadth and of greater magnitude in controllers than in progressors, and this response is inversed seen in a later time point, when controllers seems to lose this response, while progressors developed it, showing cryptic peptides immune response to different pools, suggesting that immune response to cryptic peptides might play some role in pressuring the virus mutation escape. CONCLUSIONS AND SIGNIFICANCE: cryptic peptides can elicit immune response and help to explain how some virus selection happens, either by changing expression of crucial HIV-1 proteins or generating defective virus. They can be included in vaccine design for enhancing the magnitude and breadth of T cell immune response and consequently the protection against infection or progression of HIV-1 infection

Antígenos HIV

ELISPOT

HIV-1

Infecções por HIV

Enzyme-linked immunospot assay

HIV antigens

HIV infections

HIV-1