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ISBN: 9781904455356 Year: 2008 Publisher: Norfolk Caister Academic Press
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ISBN: 063203436X 9780632034369 Year: 1996 Publisher: Oxford: Blackwell,
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ISBN: 0442307632 Year: 1981 Publisher: [S.l.] : Nelson,
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ISBN: 1555812651 9781555812652 Year: 2004 Publisher: Washington: ASM,
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Plasmids. --- Plasmides --- Plasmids --- Monograph --- PLASMIDS --- Genome, bacterial --- DNA, bacterial --- metabolism
ISBN: 9057024624 9789057024627 Year: 2000 Publisher: Amsterdam : Harwood academic publishers,
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Evolution, Molecular. --- Genes, Bacterial. --- Plasmids --- Plasmids. --- genetics.
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ISBN: 0444801618 Year: 1979 Volume: 1 Publisher: Amsterdam ; New York : New York : Elsevier/North Holland, Biomedical Press ; Sole distributors for the USA and Canada, Elsevier North Holland,
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Plasmids --- Congresses --- Congresses.
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ISBN: 0914826476 9780914826477 Year: 1984 Publisher: Washington (D.C.): American society of microbiology
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Plasmids. --- R factors.
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Year: 2015 Publisher: Bruxelles: UCL. Faculté de pharmacie et des sciences biomédicales,
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·L'utilisation de particules pseudo-virales (VLPs) pour l'administration de protéines antigéniques est une approche attractive. Le but de ce projet est de concevoir des VLPs fluorescentes à base de protéines structurelles gag virales couplées à la enhanced Green Fluorescent Protein (eGFP). La visualisation des VLPs permettra l'étude de leur comportement, l'évaluation de la capture cellulaire in vitro et de leur devenir in vivo.Dans ce contexte, les plasmides codant les protéines gag des virus de l'immunodéficience humaine (HIV) et de la leucémie murine (MLV) fusionnées à la eGFP, ont été clonés. Les VLPs fluorescentes, enveloppées avec la glycoprotéine G du virus de la stomatite vésiculaire (VSV-G) ou non ont ensuite été produites dans des cellules embryonnaires rénales humaines (293T) puis caractérisées qualitativement et quantitativement.La capture cellulaire des VLPs fluorescentes par des macrophages (J774) a été évaluée avec succès par cytométrie de flux . Cependant, l'évaluation in vivo des VLPs fluorescentes a été compromise par l'autofluorescence émise par la peau des souris.L'ensemble des résultats obtenus suggère que les VLPs fluorescentes produites in vitro sont captées efficacement par les cellules et pourront permettre des études in vivo après optimisation de leur visualisation. Using virus-like particles (VLPs) to deliver antigenics proteins is an attractive method. The aim of this project is to design fluorescent VLPs using a gag-enhanced Green Fluorescent Protein (eGFP) fusion constructs to study their caracteristics and to evaluate cellular uptake in vitro and in vivo outcome. In this context, plasmids fused eGFP, based on gag proteins from human immunodeficiency virus (HIV) and murine leukemia virus (MLV) were cloned. The, fluorescents VLPs with glycoprotein G from vesicular stomatitis virus (VSV-G) or naked fluorescents VLPs were produced in human embryonnary kidney cells (293T) and caracterized qualitatively and quantitatively. VLPs uptake in macrophages (J774) was evaluated with success by flow cytometry. Yet, aveluation of fluorescents VLPs uptake in vivo was compromised by emitted autofluoresence from skin mice. Taken together, these results suggest cellular uptake of fluorescents VLPs produced in vitro is effective and may allow in vivo studies after optimizing their visualization.
Plasmids --- Genetic Vectors --- Vaccination
Book
ISBN: 0306419017 Year: 1985 Publisher: New York (N.Y.): Plenum
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Bacteria --- Plasmids --- Congresses --- genetics
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