Development of Orf virus as a vaccine vector : manipulation of structural proteins for surface display of immunogenic peptides

Tan, Joanne Li-Ching, n/a

January 2009

Orf virus (ORFV) has the potential to be developed as a vaccine vector. Its ability to stimulate non-specific as well as specific immune responses in permissive and non-permissive hosts stands it in good stead to be utilised as such a tool. The fusion of immunogenic peptides to vaccinia virus (VACV) structural proteins have been shown to improve their immunogenicity due to presentation of the foreign antigens in a particulate form that can stimulate both B and T cells. The aims of this study were to fuse foreign antigens to ORFV structural proteins to demonstrate proof-of-concept that such surface display could also render the foreign antigens more immunogenic. Little is known about ORFV structure and morphogenesis. When this study commenced, the ORFV genome had recently been sequenced and this revealed a large number of homologues in common with VACV. It was thus assumed that both viruses may share structural similarities and that ORFV also assumes the different morphological forms such as the mature virion (MV) and extracellular virion (EV) that are present in VACV. The MV and EV forms are both infectious, with the EV containing an additional membrane acquired from the trans-Golgi network during viral morphogenesis. Furthermore, specific viral proteins are associated with both the MV and EV membranes. Six ORFV structural proteins ORFV 089, 10 kDa, F1, that are homologues of structural membrane proteins A13, A27 and H3 of VACV MVs, together with ORFV 109, ORFV 110 and B2, that are homologues of structural membrane proteins A33, A34 and F13 of VACV EVs were selected as possible candidates for manipulation. At present, there is some information available only for 10 kDa, F1 and B2. The 10 kDa is required for virus assembly, F1 for mediating cell attachment while B2 has been shown to induce significant antibody responses in sheep. Indeed proteomic analyses predicted similarities in the topologies of all of these proteins with their VACV counterparts. Using this information, preliminary studies were conducted to generate recombinant ORFVs (rORFVs) which had FLAG fused to the terminus of the protein that was exposed on the surface of the virus particle. Three rORFVs 10 kDa, F1L and 110 were successfully generated. Immunogold labelling of FLAG proteins on virus particles isolated from lysed cells showed that FLAG-10 kDa and FLAG-F1 were displayed on the surface of MV particles whereas FLAG-ORFV 110 could not be detected. Western blot analyses of solubilised recombinant ORFV 110-FLAG particles revealed that FLAG-ORFV 110 was abundant and undergoes post-translational modification indicative of endoplasmic reticulum trafficking whereas FLAG-10 kDa and FLAG-F1 did not appear to be subjected to post-translational modifications. Fluorescent microscopy confirmed the prediction that ORFV 110-FLAG localised to the Golgi in virus-infected cells and immunogold labelling of EVs showed that ORFV110-FLAG became exposed on the surface of EV-like particles as a result of egress from the cell, suggesting that the membranes had been acquired from the Golgi. These modifications also appeared to have minimal effect on the infectivity of these rORFVs. The study was extended by replacing the small FLAG peptide with an immunogenic protein (EG95), derived from the oncosphere of the zoonotic parasite Echinococcus granulosus. This protein is known to confer protection in immunised animals. Three rORFVs were generated in which a truncated version of the protein, EG95[Delta]TM, was fused to 10 kDa in the absence (rORFV 699) or presence (rORFV 700) of a linker, and also to F1 (rORFV 701). Western blot analyses of these solubilised particles demonstrated that the fusion proteins appeared to be post-translationally modified while immunogold labelling using anti-EG95 monoclonal antibodies successfully demonstrated the surface labelling on these rORFVs. In order to test the immunogenicity of these rORFVs, prime-boost experiments in sheep were conducted using rORFVs 699, 700 and 701 and a glutathione-S-transferase (GST-EG95) based vaccine. The results showed the production of EG95-specific antibodies. In particular, antibody production by group rORFV 701 compared favourably with a control group that was primed and boosted by GST-EG95 vaccine. This was despite the slightly slower growth rates of rORFVs 700 and 701 and the decreased infectivity of all three rORFVs discovered in in vitro experiments. In conclusion, these studies indicated the feasibility of this strategy to manipulate ORFV structural proteins for use as an agent for vaccine delivery.

Orf virus

viral vaccines

peptides

immunology

proteins

Investigation of epoxide hydrolase activity in Saccharomyces cerevisiae ORF YNR064c protein

Ali Ahmed, Said

January 2013

No description available.

epoxide hydrolase

ORF YNR064c

2-phenyloxirane.

Avaliação dos lipídeos de membrana e das ORF s dos contratransportadores Na+/H+ e Na+/Ca2+ associados a mecanismos de adaptação à halofilia em Halococcus morrhuae

Assis, Priscila Anne Castro de

23 September 2011

Made available in DSpace on 2015-04-01T14:16:00Z (GMT). No. of bitstreams: 1 arquivototal.pdf: 3272893 bytes, checksum: 54fd73a37837f8d64e245874e3ff9a98 (MD5) Previous issue date: 2011-09-23 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPES / Soil saliniy is a major factor in reducing plant growth and, consequently, their agricultural productivity. Most of the studies in the literature presents a strategy for reducing the effects of improving salt tolerance in plants for the production of osmolytes and stress proteins, and there are few studies aimed at increasing salt tolerance by restoring ionic homeostasis. This work was proposed to understand the physiological mechanisms and structural related with adjustment in the halophyle Halococcus morrhuae. This showed significant growth in the medium to halobacterias, that are organized in the form of sarcina of different sizes. The results achieved in attempts to characterize the lipid membrane halobactéria according to the values of retention time corresponding to phosphatidic acid (PA) and phosphatidylglycerol (C20-C20) (PG), and glycolipid known as Diglicosilarqueol (DGA-1 ). Additionally, patterns of breaks fatty acids extracted from Halococcus morrhuae showed a significant similarity when compared with the fatty acids found in organisms of the domain Eucarya and Bacteria. The genes of the antiport Na + / Ca2+ and Na + / H+ proved functional after cloning in Escherichia coli DH5α in solid and liquid medium. The antiport Na+ / H+ activity showed a statistically more significant when compared to the growth of clones containing the antiport Na+/Ca2+, making it interesting for the construction of transgenic plants tolerant to salinity. These database contribute to understanding the physiology of Halococcus morrhuae for future biotechnological applications, among them the inclusion of these genes in plants to assess the functionality in eukaryotic models. / A salinização do solo é um dos principais fatores para redução do crescimento das plantas e, consequentemente, da sua produtividade agrícola. A maioria dos estudos presentes na literatura apresenta como estratégia para redução dos seus efeitos o melhoramento da tolerância a sal pelas plantas pela produção de osmólitos e proteínas de estresse, existindo poucos estudos visando o aumento da tolerância ao sal pelo restabelecimento da homeostase iônica. Neste trabalho foi proposto compreender mecanismos fisiológicos e estruturais relacionados com a adaptação à halofilia em Halococcus morrhuae. O crescimento de H. morrhuae foi significativo no meio para halobactérias, organiza-se na forma de sarcinas de diferentes tamanhos ao longo do tempo. Os resultados alcançados na tentativa de caracterização de lipídios da membrana da halobactéria, de acordo com os valores de tempo de retenção, correspondem ao ácido fosfatídico (PA) e fosfatidilglicerol (C20-C20)(PG), e ao glicolipídio conhecido como diglicosilarqueol (DGA-1). Adicionalmente, os padrões de quebras dos ácidos graxos extraídos de Halococcus morrhuae apresentaram uma similaridade significativa quando comparada com a dos ácidos graxos encontrados em organismos do domínio Eucarya e Bacteria. Os genes dos antiportes Na+/Ca+2 e Na+/H+ aumetaram a tolerância ao sal, mostrando-se funcionais após espressão em Escherichia coli DH5α em meio sólido e em meio líquido. O antiporte Na+/H+ apresentou uma atividade estatisticamente mais significativa (p<0,03) quando comparada ao crescimento dos clones contendo o antiporte Na+/Ca2 (p<0,05). Entretanto, ambos os antiportes são candidatos interessantes para a construção de plantas geneticamente modificadas tolerantes a salinidade. Estes dados também contribuem para o entendimento da fisiologia de H. morrhuae para futuras aplicações biotecnológicas, dentre elas a inserção desses genes em plantas para avaliar a funcionalidade em modelos eucarióticos.

Genética molecular

ORF s

Halococcus morrhuae

Molecular genetic

ORF s

Halococcus morrhuae

CIENCIAS BIOLOGICAS::BIOLOGIA GERAL

Infecção experimental de coelhos e camundongos com o vírus do ectima contagioso / Experimental infection of rabbits and mice with contagious ecthyma virus

Cargnelutti, Juliana Felipetto

25 February 2010

Conselho Nacional de Desenvolvimento Científico e Tecnológico / Contagious ecthyma (orf) is a cutaneous disease that affects sheep and goats, and may be occasionally transmitted to humans. The disease is caused by orf virus (ORFV). ORFV infection produces croustous and proliferative lesions, usually on the nostrils and labial commissures of lambs, and also in the udder, teat skin and coronary bands of adults animals. The pathogenesis of ORFV infection is poorly understood and a search for an adequate animal model is required, yet the disease has been already reproduced in sheep, goats and rabbits. This dissertation relates the clinical, virological and pathological aspects of ORFV infection in rabbits and mice experimental inoculated. Ten rabbits, ten mice and two lambs were inoculated intradermally after skin scarification with an hypodermic needle. A viral suspension of ORFV IA-82 strain (108.5TCID50/mL) was inoculated in the internal face of the ear, back skin and labial commissure of rabbits; internal face of the ear of mice. Lambs were inoculated in the labial commissures and in the internal face of hind limbs. All animals were monitored clinically, virologically, and pathologically for 21 days. All rabbits developed clinical signs in the inoculation sites, begining with mild hyperemia that evolved to macules, papules, vesicle, pustules and scabs. Lesions appeared at days 3 and 4 post-inoculation (pi) and lasted to 3 to 10 days. Viral shedding was detected from days 2 to 14pi. Histological examination of lesions revealed focal proliferative dermatitis with ballooning degeneration and eosinophilic intracytoplasmic inclusions in keratinocytes, histological hallmarks of contagious ecthyma in sheep. A similar, albeit much milder clinical course was observed in 5 out of 10 inoculated mice. All lambs presented characteristic contagious ecthyma clinical and histopathologycal lesions from days 3 to 18pi, and the virus was recovered from lesions between days 2 and 19pi. At day 28pi, seroneutralization test (SN) was unable to detect neutralizing antibodies in all inoculated animals. These findings show that ORFV replicates and produce local lesions in rabbits and mice. However, rabbits are more susceptible to infection and disease, and may be used as an animal model to study some aspects of ORFV pathogenesis. / O ectima contagioso (ou orf) é uma doença infecto-contagiosa de pele que afeta principalmente ovinos e caprinos, e que ocasionalmente pode acometer o homem. O seu agente etiológico é o vírus da orf (ORFV). O ORFV produz lesões proliferativas, geralmente na comissura labial e no plano naso-labial de cordeiros, e também na pele do úbere, nos tetos e no rodete coronário dos cascos de animais adultos. A patogenia da infecção pelo ORFV é pouco conhecida, embora a doença já tenha sido reproduzida em ovinos, caprinos e coelhos. Essa dissertação relata os achados clínicos, virológicos e histopatológicos da infecção experimental de coelhos e camundongos pelo ORFV. Para isso, coelhos, camundongos e cordeiros foram inoculados pela via intradérmica (ID), após escarificação da pele com agulha hipodérmica. A inoculação dos cordeiros serviu como controle positivo. Uma suspensão viral da cepa IA-82 do ORFV (108,5DICC50/mL) foi inoculada na face interna da orelha, na pele do dorso e na comissura labial dos coelhos; na face interna da orelha dos camundongos; e na comissura labial e face interna do membro pélvico dos cordeiros. Os animais foram monitorados por 21 dias nos aspectos clínicos, virológicos e patológicos. Todos os coelhos inoculados apresentaram lesões semelhantes nos locais de inoculação, iniciando com hiperemia, evoluindo para máculas, pápulas, vesículas, pústulas e crostas. Os sinais surgiram 3 a 4 dias pós inoculação (pi) e duraram por 3 a 10 dias. Excreção viral foi detectada entre os dias 2 e 14pi. A análise histológica das lesões revelou dermatite focal proliferativa, com degeneração balonosa e corpúsculos de inclusão intracitoplasmáticos eosinofílicos nos queratinócitos, semelhante às alterações histológicas observadas nos cordeiros. Lesões similares, mas de menor intensidade foram observadas em 5 de 10 camundongos. Os cordeiros, utilizados como controles positivos, apresentaram lesões clínicas e histopatológicas características de ectima contagioso entre os dias 3 e 18pi, sendo que o vírus foi recuperado das lesões entre os dias 2 e 19dpi. No dia 28pi, pelo teste de soroneutralização (SN), não foram detectados anticorpos neutralizantes no soro dos animais inoculados. Esses resultados demonstram que a inoculação de ORFV resulta em replicação viral e produção de lesões em coelhos e camundongos, porém a doença é reproduzida de forma mais consistente em coelhos. Portanto, sugere-se que coelhos possam ser utilizados como modelos para estudos in vivo com o ORFV.

ORFV

Vírus da orf

Patogenia

Modelos experimentais

ORFV

Orf virus

Pathogenesis

Experimental models

Régulation post-transcriptionnelle dans l'adaptation des plantes genes aux stress abiotiques / Post-transcriptional regulation of plant genes in adaptation to abiotic stresses : regulation of target of rapamycin (tor) gene

Mahgoub, Hany

05 May 2011

Les plantes sont ancrées au sol pendant la majorité de leur cycle de vie et doivent donc constamment adapter leur croissance et leur métabolisme aux stress abiotiques. Ainsi, la subsistance des plantes dépend de leur capacité à réguler rapidement l’expression des gènes afin d’adapter leur physiologie à l’environnement. L’expression d’un gène peut être contrôlé à plusieurs niveaux; transcriptionnel, post-transcriptionnel, traductionnel et post-traductionnel.De nombreux processus cellulaires vitaux tels que la réplication de l’ADN, la transcription, la synthèse protéique, et la dégradation des protéines, sont régulés par les signaux environnementaux. Des études chez la levure, la drosophile et les animaux ont montré que la protéine kinase TOR (Target Of Rapamycin) est impliquée dans le contrôle de la croissance cellulaire et de la prolifération en réponse à différents signaux tels que les nutriments, les acides aminés, les hormones et les facteurs de croissance. Chez Arabidopsis thaliana, TOR est nécessaire au développement de l’embryon et de l’endosperme. De plus, des modifications du niveau de protéine AtTOR affectent la croissance végétative et la reproduction.Le principal objectif de cette thèse est de caractériser les mécanismes qui contrôlent l’expression de AtTOR en déterminant les éléments de régulation situés sur le la région 5’ non traduite (5′UTR) de l’ARNm de AtTOR, puis de manipuler ces éléments de régulation afin d étudier leur rôle. Nous avons choisi de nous focaliser sur la région 5′UTR de AtTOR, et sur une microORF (uORF) située en amont de l’ORF principale de AtTOR. Il s’agit de la première tentative d’étude de la régulation de l’expression de TOR par ces éléments chez les eucaryotes.Trois constructions chimériques ont été réalisées pour cette étude et transformée transitoirement est de manière stable dans des plantes. La première construction (contrôle positif) incluse le promoteur de AtTOR, la région 5′UTR, le premier intron et le début du premier exon fusionné au gène rapporteur GUS. La seconde construction (microORF mutée) est présente une mutation du codon start de la microORF (ATG changé en TTG). Enfin, la troisième construction (5′UTR délétée) contient la même séquence que le contrôle positif mais sans la région 5′UTR. Ces constructions ont également été placée sous le contrôle du promoteur 35S au lieu du promoteur de AtTOR afin d’étudier un lien éventuel entre la 5′UTR et la microRF et le promoteur de AtTORNos résultats indiquent une régulation généralement négative exercée par la 5′UTR, et dans une moindre mesure par la microORF, sur l’expression de AtTOR. Cette régulation semble avoir lieu au niveau transcriptionnel ou au niveau de la stabilité de l’ARNm, mais pas au niveau de la traduction. En effet, les modifications du niveau de transcrit GUS sont suivie d’un changement équivalent de l’activité GUS. De plus, nous avons observé que l’auxine et le sucrose ont un effet positif sur l’expression de AtTOR. Dans le cas de l’auxine, cet effet semble lié à la présence de la région 5′UTR de AtTOR.D’autres études de la fonction de la région 5’UTR et de la microORF de AtTOR, ainsi que de leur relation avec d’autres éléments régulateurs localisée dans le promoteur de AtTOR, permettront de mieux comprendre comment ces éléments régulateurs contrôlent finement l’expression de AtTOR. / Land plants are anchored in one place for most of their life cycle and therefore must constantly adapt their growth and metabolism to abiotic stresses. Thus, plants’ subsistence depends on their ability to regulate rapidly gene expression in order to adapt their physiology to their environment. The expression of a gene can be controlled at many levels, including transcription, post-transcription, translation, and post-translation.Many vital cellular processes like DNA replication, transcription, protein synthesis, and protein degradation are regulated by environmental signals. Studies in yeast, Drosophila, and mammals showed that the target of rapamycin (TOR) protein is involved in control of cell growth and cell proliferation in response to different types of environmental signals such as nutrients, amino acids, hormones, and growth factors. In Arabidopsis thaliana, TOR is necessary for both embryo and endosperm development in, and changes of TOR protein level affect both vegetative and reproductive growth.The main purpose from this thesis is to highlight the mechanisms that control AtTOR expression at the post-transcriptional level through determination of the possible regulatory elements within the 5′ untranslated region (5′UTR) or the first intron of AtTOR mRNA itself, and through manipulation of these regulatory elements to study their precise role. We have chosen to focus on the small upstream open reading frame (uORF) as well as the 5′UTR region. This is the first attempt to study the regulation of TOR kinase expression in eukaryotes through these small uORF or the sequence of 5′ untranslated region (5′UTR).To achieve this purpose, three chimeric constructs have been established and transformed in Nicotiana benthamiana leaves and Arabidopsis thaliana plants. The first construct (the positive control) contains the AtTOR promoter, the 5′UTR, the first intron, and the beginning of the second exon fused to the GUS reporter gene. The second construct (mutated uORF) have the same sequence as the positive control construct except the start codon of uORF was changed from ATG to TTG. The third construct (deleted 5′UTR) have the same sequence as the positive control construct without the 5′UTR. These constructs have also been placed under the activity of CaMV 35S promoter instead of AtTOR promoter to investigate whether there is a link between the 5′UTR/or uORF and the promoter.Our work show an overall negative regulation exerted by the 5′UTR and, to a lesser extent, by the uORF on AtTOR gene regulation. This regulation is likely at the level of transcription or mRNA stability, since the changes in GUS transcript level was followed by the same changes in GUS activity. In addition we found that external inducers like auxin or sucrose exert a positive effect on AtTOR expression. This effect appears somehow linked to the presence of the 5′UTR of AtTOR mRNA.Greater insight into the molecular mechanisms of AtTOR 5′UTR/or uORF function and its relationship with other regulatory elements located in AtTOR promoter will be required to understand how these regulatory elements work either individually or in combination to achieve the fine and accurate regulation of their gene expression.

Arabidopsis thaliana

Target of Rapamicyne

Régulations post transcriptionnelles

5'utr

Micro ORF

Arabaidopsis thaliana

Target of Rapamicyn

Post transcriptional regulations

5'utr

Micro ORF

Inhibition des Interferon-Beta-Systems durch Tribec-Virus / Inhibition of the interferon-beta system by Tribec virus

Brandt, Nora Elena

30 January 2013

No description available.

610 Medizin, Gesundheit

MED 332

Medicine

Tribec-Virus (TRBV)

Interferon (IFN)

IRF-3

Orbivirus

ORF-X

Tribec virus (TRBV)

interferon (IFN)

IRF-3

Orbivirus

ORF-X

44.75

44.43

Efeitos do parapoxvirus ovis inativado sobre eventos da resposta imune inata em camundongos / Effects of inactivated parapoxvirus ovis in events of the innate immune response in mice

Anziliero, Deniz

08 November 2013

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / The immunostimulatory properties of inactivated parapoxvirus ovis (iPPVO) have been investigated in different animal species and experimental settings. This study investigated the effects of administration of iPPVO on selected events of the innate response in mice. Neutrophil activation, phagocytic activity of macrophages, serum bactericidal activity, induction and antiviral activity of interferon type I (IFN - I) and expression of several classes of cytokines were assayed following intraperitoneal inoculation of Mus musculus with iPPVO (107 TCID50). Serum from iPPVO-treated animals showed IFN-I activity against murine encephalomyocarditis virus (EMCV) between 6 and 12 hours post infection (hpi), as shown by plaque reduction. A significant activation of neutrophils at 6hpi was observed by NBT reduction test in animals treated with the iPPVO. Peritoneal macrophages from mice treated with iPPVO demonstrated a significant increase (p<0.01) in phagocytic activity against Candida albicans both in vivo (between 12 and 96 hpi) and in vitro (24 and 72 hpi). iPPVO treated mice showed increased serum bactericidal activity against Escherichia coli (p<0.05) at two periods (24 and 72 hpi). A second study evaluated the expression of cytokines in response to inoculation of iPPVO. For this, spleens and serum samples were collected from mice treated with iPPVO at different intervals after inoculation and subjected to quantification of messenger RNA (mRNA) by real time PCR (qRT-PCR) and detection/quantification of serum cytokines by ELISA. Quantification of mRNA identified a significant and transient increase in the expression of various cytokines, with variable magnitude and kinetics. mRNA expression of proinflammatory cytokines (IL-1β, TNF-α and IL-8) peaked at 24 hpi (5.4 times increase) and 48 hpi (3 and 10 times, respectively). A 15-fold increase in expression of INF-γ and 6-fold for IL-12 was observed at 48 and 24 hpi, respectively. An increase in the expression of self-regulatory cytokines (Th2) cells, especially IL-10 and IL-4 was detected at later periods (72 and 96 hpi) with peaks of 4.7 and 4.9 fold, respectively. The determination of the concentration of serum cytokines by ELISA showed an increase in IL-1β, TNF-α, IL- 12, IFN-γ and IL-10 with kinetics similar to that observed by qPCR, especially for IL-1 and INF-γ. In summary, these results demonstrate that inoculation with iPPVO stimulates transiently a number events associated with cellular and humoral innate immune responses. If taken together, these effects would likely contribute for the enhanced resistance to certain pathogens observed in animals treated with iPPVO. / As propriedades imunoestimulatórias do Parapoxvirus ovis inativado (iPPVO) têm sido verificadas em diferentes espécies animais e condições experimentais. No presente trabalho foram investigados os efeitos da administração do iPPVO sobre eventos da resposta inata de camundongos. Ativação de neutrófilos, atividade fagocítica de macrófagos, atividade bactericida do soro, indução e atividade antiviral do interferon tipo I (INF-I) e expressão de várias classes de citocinas foram investigados em diferentes intervalos após inoculação de Mus musculus pela via intraperitonial com iPPVO (dose 107 TCID50). O soro de animais tratados com iPPVO apresentou atividade de INF-I frente ao vírus da encefalomiocardite murina (EMCV) entre 6 e 12 horas pós inoculação (hpi), como demonstrado pela redução significativa de formação de placas virais. Uma significativa ativação dos neutrófilos circulantes foi observada pela técnica de redução do NBT em animais tratados com o iPPVO às 6 hpi. Macrófagos peritoneais de camundongos tratados com iPPVO demonstraram um aumento significativo (p<0,01) na atividade fagocítica frente a Candida albicans tanto in vivo (entre 12 e 96 hpi) quanto in vitro (24 e 72hpi). Camundongos tratados com iPPVO apresentaram aumento na atividade bactericida do soro frente à Escherichia coli (p<0,05) em dois períodos avaliados (24 e 72 hpi). Um segundo estudo avaliou a expressão de citocinas em resposta à inoculação do iPPVO. Para isso, amostras de baço e soro foram coletados de camundongos tratados com iPPVO em diferentes intervalos após a inoculação e submetidas a quantificação de RNA mensageiro (RNAm) por PCR em tempo real (qRT-PCR) e detecção/quantificação de citocinas no soro por ELISA. A quantificação de RNAm permitiu detectar um aumento significativo e transitório da expressão de várias citocinas, com magnitude e cinética variáveis. A expressão de RNAm das citocinas pró-inflamatórias (IL-1β, TNF-α e IL-8) atingiu o pico às 24 hpi (aumento de 5,4 vezes), 48 hpi (3 e 10 vezes, respectivamente). Um aumento de 15 vezes na expressão gênica do INF-γ, e de 6 vezes para a IL-12 foi observado às 48 e 24 hpi, respectivamente. Um incremento na expressão das citocinas auto-regulatórias (Th2), principalmente IL-10 e IL-4, foi detectado em períodos mais tardios (72 e 96 hpi) com picos de 4,7 e 4,9 vezes, respectivamente. A determinação da concentração das citocinas séricas por ELISA revelou um aumento nos níveis de IL-1β, TNF- α, IL-12, INF-γ e IL-10, com uma cinética similar à observada pela técnica de qPCR, especialmente para IL-1β e INF-γ. Em resumo, esses resultados demonstram que o tratamento com iPPVO estimula de forma significativa e transitória uma série de eventos celulares e humorais ligados à resposta imune inata. Esses efeitos, se considerados em conjunto, provavelmente contribuem para o aumento da magnitude da resposta imunológica a certos patógenos observada em animais tratados com o iPPVO.

Ectima contagioso

Vírus da orf

Imunoestimulante

Resposta imune inata

Contagious ecthyma virus

Orf virus

Immunostimulant

Innate immune response

SIRT7 and ATM are Barriers to a Productive Adenovirus E4 Mutant Infection

Stanley, Gabrielle

22 November 2021

No description available.

Virology

Molecular Biology

Microbiology

Adenovirus

E4 ORF 3

E4 11 kDa

E4 ORF 6

E4 34 kDa

ATM

DNA damage response

micrococcal nuclease

SIRT7

protein acetylation

Potentiating the Oncolytic Efficacy of Poxviruses

Komar, Monica

26 July 2012

Several wild-type poxviruses have emerged as potential oncolytic viruses (OVs), including orf virus (OrfV), and vaccinia virus (VV). Oncolytic VVs have been modified to include attenuating mutations that enhance their tumour selective nature, but these mutations also reduce overall viral fitness in cancer cells. Previous studies have shown that a VV (Western Reserve) with its E3L gene replaced with the E3L homologue from, OrfV (designated VV-E3LOrfV), maintained its ability to infect cells in vitro, but was attenuated compared to its parental VV in vivo. Our goal was to determine the safety and oncolytic potential VV-E3LOrfV, compared to wild type VV and other attenuated recombinants. VV-E3LOrfV, was unable to replicate to the same titers and was sensitive to IFN compared to its parental virus and other attenuated VVs in normal human fibroblast cells. The virus was also less pathogenic when administered in vivo. Viral replication, spread and cell killing, as measures of oncolytic potential in vitro, along with in vivo efficacy, were also observed.. The Parapoxvirus, OrfV has been shown to have a unique immune-stimulation profile, inducing a number of pro-inflammatory cytokines, as well as potently recruiting and activating a number of immune cells. Despite this unique profile, OrfV is limited in its ability to replicate and spread in human cancer cells. Various strategies were employed to enhance the oncolytic efficacy of wild-type OrfV. A transient transfection/infection screen was created to determine if any of the VV host-range genes (C7L, K1L, E3L or K3L) would augment OrfV oncolysis. Combination therapy, including the use of microtubule targeting agents, Viral Sensitizer (VSe) compounds and the addition of soluble VV B18R gene product were employed to see if they also enhance OrfV efficacy. Unfortunately, none of the strategies mentioned were able to enhance OrfV.

Poxvirus

Vaccinia virus

Orf Virus

Interferon

Host-range genes

Cancer

Oncolytic virus

Combination therapy

E3L

Caractérisation fonctionnelle de nouveaux gènes mitochondriaux chez les espèces à DUI : étude du gène f-orf chez la moule marine Mytilus edulis

Ouimet, Philip

08 1900

No description available.

mitochondrie

génome

bivalve

ORFans

f-orf

Mytilus edulis

Mitochondria