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Development of novel vaccine strategies for duck Hepatitis B virus infection.Miller, Darren Scott January 2008 (has links)
Hepatitis B virus (HBV) is a life-threatening pathogen with major economic significance. Acute infection in adults is common, albeit usually self-limiting. Importantly, infection in infants typically results in chronic infection and increased incidence of hepatocellular carcinoma (HCC). Furthermore, the infectious carrier state is perpetuated in chronically infected individuals. Successful immuno-therapeutic vaccination would reduce the incidence of chronic infection and of HCC as well as reduce transmission of the disease. Recovery from acute and chronic HBV infection typically occurs in the presence of robust antigen-specific humoral and cellular immune responses (CMI), whereas these responses are low or absent in chronically HBV-infected individuals. Therefore, it was hypothesised that effective stimulation of both humoral and CMI responses, in conjunction with currently available antiviral therapies, may contribute significantly to development of vaccines for treatment of chronic HBV infection. The duck hepatitis B virus (DHBV) model of HBV infection was used to test novel vaccine strategies that could complement existing antiviral therapeutic approaches to treat chronically HBV-infected humans. To this end, three separate vaccine studies were conducted to investigate potential therapeutic regimes. Methods to assess the efficacies of the vaccine strategies included immunoperoxidase detection of viral antigen and immune cell markers within the liver and development of sensitive assays to monitor levels of DHBV DNA, duck hepatitis B virus surface antigen (DHBsAg), antibodies to duck hepatitis B core (anti-DHBc) and surface antigens (anti-DHBs) in serum were developed and validated which allowed monitoring of the kinetics of the humoral immune response following vaccination and the course and outcome of experimental DHBV infection. The first vaccine study tested the protective efficacy of DNA vaccines encoding either the small form of DHBsAg (DHBs) protein or the larger antigen (DHBpre-S/S), These were administered to ducks at day 4 and 14 of age. On the same day as the second vaccination, ducks were challenged intravenously with DHBV. Immunoperoxidase staining of biopsy tissue collected at day 4 p.i. showed significant decreases in the number of DHBV infected hepatocytes in ducks receiving the DNA vaccines compared to the mock-vaccinated control ducks. Significant protection against development of chronic DHBV infection was observed in ducks vaccinated with DNA vaccines expressing either pre-S/S or S protein. Although anti-DHBs antibodies were not detected prior to DHBV challenge, the decrease in the percentages of DHBV-infected hepatocytes at day 4 p.i is suggestive that neutralisation of the inoculum by low-level anti-DHBs antibodies in cohort with CMI responses induced by vaccination were the most probable mechanisms of action. The second vaccine study examined the protective efficacy of a novel whole-cell vaccine that expressed the DHBV core antigen (DHBcAg). Ducks were vaccinated on day 4 and 14 of age and DHBV challenge was administered 4 days later. Detectable anti-DHBc antibodies were generated as soon as 4 days after the initial vaccination suggesting that this regimen elicited increased immunogenicity than vaccination with DNA vaccines alone. In contrast to the first vaccine study with DNA vaccines expressing DHBsAg, no significant differences in the percentage of DHBV-infected hepatocytes were observed in biopsy tissue collected at day 4 p.i.This finding is confirmation that anti-DHBc antibodies were not neutralising to the initial DHBV inoculum. However, significant protection against development of chronic DHBV infection was observed in the whole-cell vaccinated ducks suggesting that the mechanism of protection was consistent immune-mediated killing of DHBV-infected hepatocytes following CMI responses to determinants of DHBcAg. The final vaccine study involved a combination strategy of antiviral drug Entecavir (ETV) and prime-boost vaccination with DNA vaccines and recombinant fowlpoxvirus (rFPV) expressing DHBV antigens. Immediately following DHBV infection, ducks were dosed by oral gavage with the antiviral drug Entecavir (ETV) and at the same time received the priming DNA vaccines encoding DHBV antigens. Seven days later the boosting vaccination consisting of recombinant fowlpox viruses (rFPV) also expressing DHBV antigens was administered. Extraordinary protection was observed, with 100% of ducks given combination therapy rapidly resolved their DHBV infection while 100% of non-treated ducks developed chronic infection. It was concluded that protection resulted from a combination of at least three factors. First, reduction and control of DHBV levels with the aid of ETV; secondly, stimulation of surface antigen-specific humoral immune responses resulting in neutralisation of newly produced virions; and finally, the combined up-regulation of CMI responses against DHBV core and surface antigens, resulting in elimination of infected hepatocytes. The four manuscripts that comprise this thesis provide insights into the viral kinetics and immune responses that follow DHBV infection and/or vaccination of ducks. The results provide new directions for future vaccine studies aimed at developing effective treatments for chronic HBV infection. / Thesis (Ph.D.) -- University of Adelaide, School of Molecular and Biomedical Science, 2008
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Molecular epidemiology of hepatitis A and hepatitis B virus in central America /Arauz-Ruiz, Patricia January 2002 (has links)
Diss. (sammanfattning) Stockholm : Karolinska institutet, 2002. / Härtill 5 uppsatser.
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Kan donörlerinde Hepatit B virus core antikorlarının saptanması /Kesbiç, Hasan. Kaya, Selçuk. January 2007 (has links) (PDF)
Tez (Tıpta Uzmanlık) - Süleyman Demirel Üniversitesi, Tıp Fakültesi, Tıbbi Mikrobiyoloji Anabilim Dalı, 2007. / Bibliyografya var.
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Low level hepatitis B virus carriers : its detection by polymerase chain reaction based assays and its clinical significance /Chung, Hau-tim. January 1995 (has links)
Thesis (M.D.)--University of Hong Kong, 1996. / Includes bibliographical references (leaf 102-116).
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Infectivity of lymphoid cell-derived woodchuck hepatitis virus in an in vitro experimental system /Lew, Yuan-Yee, January 1999 (has links)
Thesis (M.Sc.)--Memorial University of Newfoundland, Faculty of Medicine, 2000. / Typescript. Bibliography: leaves 219-243.
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Development of molecular diagnostic system for detection of hepatitis B virus in blood donationsFun, Sze-tat. January 2003 (has links)
Thesis (M.Med.Sc.)--University of Hong Kong, 2004. / Also available in print.
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Low level hepatitis B virus carriers its detection by polymerase chain reaction based assays and its clinical significance /Chung, Hau-tim. January 1995 (has links)
Thesis (M.D.)--University of Hong Kong, 1996. / Includes bibliographical references (leaf 102-116). Also available in print.
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Estudo da distribuição genotípica e de mutações no genoma do vírus da hepatite B, em pacientes co-infectados pelo vírus da hepatite B e HIV, na Casa da AIDS, do Hospital das Clínicas da Faculdade de Medicina da Universidade de São Paulo / Hepatitis B genotype distribution and frequency of resistance mutations in a group of patients co-infected with HIV and hepatitis B virus (HBV) at an AIDS Outpatient Clinic in Sao PauloAdriana Cristina da Silva 12 January 2011 (has links)
O objetivo deste estudo foi avaliar a distribuição genotípica e mutações no genoma do vírus da hepatite B (VHB) em um grupo de pacientes co-infectados pelo VHB e vírus da imunodeficiência humana (HIV). Foram incluídos pacientes AgHBs +/HIV+ , atendidos em um ambulatório de referência para pacientes infectados pelo HIV, na cidade de São Paulo. Para a detecção dos marcadores sorológicos para infecção pelo VHB utilizou-se técnica de ELISA através de kits comerciais. A detecção do DNA-VHB foi realizada através de nested-PCR e sua quantificação foi realizada por COBAS AMPLICOR. De acordo com a literatura, a infecção pelo VHB no Brasil varia de 0,4 a 8,5%. Os genótipos de VHB, as mutações na região do core, BCP, pré-core e na região da polimerase foram determinados por seqüenciamento. Cinqüenta e nove pacientes foram incluídos neste estudo e cinqüenta e seis pacientes relatavam uso prévio de lamivudina ou tenofovir. A presença do DNA-VHB foi detectada em 22 pacientes AgHBs positivos. A identificação dos genótipos foi realizada em 16 pacientes e a distribuição dos genótipos do VHB foi: A (12-75%); G (2-13%), D (1-6%) e F (1-6%). Em 10 dos pacientes com viremia presente para DNA-VHB, foram observadas mutações na região da polimerase (rtL180M + rtM204V, rtV173L + rtL180M + rtM204V) e no gene do envelope (sI195M, sW196L, sI195M/sE164D). Mutações na região do BCP (A1762T, G1764A) e do pré-core (G1896A) foram identificados em quatro pacientes. Em conclusão, entre os pacientes analisados observou-se uma alta prevalência de mutações associadas a resistência à lamivudina e associadas a resistência a anti-HBs. O genótipo G, raramente descrito em nosso meio, foi também observado nesse grupo de pacientes. / The objective of this study was to evaluate the genotype distribution and genomic mutations of hepatitis B virus (HBV) among a group of HIVHBV co-infected patients from an AIDS outpatient clinic in São Paulo. HBV serological markers were detected by commercially available enzyme immunoassay kits. HBV DNA was detected by using an in-house nested PCR and quantified by COBAS AMPLICOR. HBV genotypes, basal core promoter (BCP) / pre-core / core region and surface / polymerase genes mutations were determined by sequencing. Among the 59 patients included in this study, 56 reported previous use of lamivudine or tenofovir. According to the literature HBV infection in Brazil varies from 0,4 to 8,5%. HBV DNA was detected in 16/22 patients and the genotypes distribution was A (n=12, 75%); G (n=2, 13%); D (n=1, 6%), and F (n=1, 6%). In 10 patients with viremia, lamivudine-resistance mutations in the polymerase gene (rtL180M + rtM204V, rtV173L + rtL180M + rtM204V) were found, accompanied by changes in the envelope gene (sI195M, sW196L, and sI195M/sE164D). Mutations in the BCP and pre-core regions were identified in 4 patients. In conclusion, genotype G, rarely seen in Brazil, was observed in this group of patients. A high prevalence of mutations associated with lamivudine-resistance accompanied by mutations associated with anti-HBs resistance was also found among these patients.
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Protéine HBx du Virus de l’Hépatite B : impact sur la prolifération et la carcinogenèse hépatique / HBx protein of hepatitis B virus : impact on proliferation and carcinogenesis hepaticQuétier, Ivan 29 November 2012 (has links)
Avec près de 350 millions de personnes chroniquement infectées, et malgré l’existence de vaccins efficaces, le virus de l’Hépatite B (VHB) reste un problème majeur de santé publique. Parmi les protéines virales, la protéine régulatrice HBx possèdent des activités qui pourraient être particulièrement impliquées dans le développement de CHC. Au cours de ce travail, nous nous sommes intéressés aux différences biologiques entre la protéine HBx issue d’une région non tumorale (HBx-NT) et la protéine HBx issue d’une région tumorale (HBx-T) d’un même patient. En particulier, nous nous sommes intéressés à la régénération hépatique après hépatectomie partielle et à la carcinogenèse hépatique dans un modèle murin transgénique. Nous avons démontré l’absence d’impact de la forme tronquée de la protéine HBx sur la régénération hépatique. Nous avons démontré que la protéine HBx entière avait la capacité d’activer la sécrétion d’IL-6 dans la phase d’initiation de la régénération hépatique, conduisant à l’hyperactivation de STAT3, l’accumulation de SOCS3 et la diminution de phosphorylation de ERK. Au final, la protéine HBx entière induit un retard de régénération hépatique. Nous avons démontré une cinétique d’apparition de tumeurs plus rapide chez les souris HBx-T que chez les souris HBx-NT après injection d’un carcinogène chimique. Nous avons aussi pu observer que les deux formes HBx-T et HBx-NT sensibilisaient les hépatocytes à l’apoptose, au cours d’un dommage hépatique aigue, et que cette sensibilisation à l’apoptose pouvait en partie rendre compte de l’effet co-carcinogène observé chez les souris HBx-T et HBx-NT. L’ensemble de mes résultats a permis de mieux comprendre les mécanismes par lesquels la protéine HBx participe au développement de CHC. / Hepatitis B virus (HBV) is a worldwide health issue, as it is estimated that 350 millions people are chronically infected. Among the viral proteins, HBx is thought to be involved in hepatocellular carcinoma (HCC) development. In this work, we were interested in biological differences between HBx sequence from non tumoral region (HBx-NT) compared to HBx from tumoral region (HBx-T) from a single patient. In particular, we studied liver regeneration after partial hepatectomy et hepatocarcinogenesis in a transgenic mice model. We demonstrated that HBx-T did not modulate liver regenereation. We also showed that HBx-NT induced IL-6 overexpression during priming phase of liver regeneration, and that IL-6 overexpression was involved in STAT3 hyperactivation, SOCS3 accumulation and inhibition of ERK. Overall, HBx-NT induced IL-6 overexpression was responsible for a delay in liver regeneration. Moreover, we showed that HBx-T induced a faster development of hepatic tumor after DEN initiation, compared to HBx-NT. Both HBx forms were involved in an apoptosis sensibilization during acute liver injury, that could be involved in co-carcinogenic effect of HBx-T and HBx-NT. Overall, my results participate to the comprehension of HBx impact on liver carcinogenesis
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Quantitative assessment of HLA-DQ gene polymorphisms with the development of hepatitis B virus infection, clearance, liver cirrhosis, and hepatocellular carcinomaXu, Tao, Zhu, Anyou, Sun, Meiqun, Lv, Jingzhu, Qian, Zhongqing, Wang, Xiaojing, Wang, Ting, Wang, Hongtao 06 December 2017 (has links)
Hepatitis B is one of the most common infectious diseases, which leads to public health problems in the world, especially in Asian counties. In recent years, extensive human genetic association studies have been carried out to identify susceptible genes and genetic polymorphisms to understand the genetic contributions to the disease progression of HBV infection. HLA-DQ gene variations have been reported to be associated with HBV infection/clearance, disease progression and the development of hepatitis B-related complications, including liver cirrhosis (LC) and hepatocellular carcinoma (HCC). However, the results are either inconclusive or controversial. Therefore, to derive a more precise estimation of the association, a meta-analysis was performed. Our data revealed that the HLA-DQ alleles rs2856718-G, rs7453920-A and rs9275319-G were significantly associated with decreased risk of HBV infection and HBV natural clearance. Logistic regression analyses showed that HLA-DQ alleles rs9275572-A significantly increased HBV infection clearance, and decreased HBV natural clearance. However, rs2856718-G and rs9275572-A were not associated with development of cirrhosis. The HLA-DQ polymorphisms (rs2856718 and rs9275572) were associated with a decreased HBV-related HCC risk in all genetic models, but rs9272105-A increased the risk of HBV-related HCC. In addition, no significant association was observed between HLA-DQ rs9275319-G polymorphism and HBVrelated HCC. These stratified analyses were limited due to relatively modest size of correlational studies. In future, further investigation on a large population and different ethnicities are warranted. Our findings contribute to the personalized care and prognosis in hepatitis B.
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