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dc.contributor.authorChan, L
dc.contributor.authorNesbeth, D
dc.contributor.authorMackey, t
dc.contributor.authorGalea-Lauri, J
dc.contributor.authorGaken, J
dc.contributor.authorMufti, F
dc.contributor.authorFarzaneh, F
dc.contributor.authorDarling, D
dc.contributor.authorCollins, Mary
dc.contributor.authorMartín Molina, Francisco 
dc.date.accessioned2025-01-31T08:33:37Z
dc.date.available2025-01-31T08:33:37Z
dc.date.issued2005
dc.identifier.citationJournal of Virology. Volumen: 79(20); Págs: 13190-13194. (2005):es_ES
dc.identifier.urihttps://hdl.handle.net/10481/101491
dc.description.abstractNonviral producer cell proteins incorporated into retroviral vector surfaces profoundly influence infectivity and in vivo half-life. We report the purification and concentration of lentiviral vectors using these surface proteins as an efficient gene transduction strategy. Biotinylation of these proteins and streptavidin paramagnetic particle concentration enhances titer 400- to 2,500-fold (to 10(9) CFU/ml for vesicular stomatitis virus G protein and 5 x 10(8) for amphotropic murine leukemia virus envelope). This method also uses newly introduced membrane proteins (B7.1 and DeltaLNGFR) directed to lentiviral surfaces, allowing up to 17,000-fold concentrations. Particle conjugation of lentivirus allows facile manipulation in vitro, resulting in the transduction of 48 to 94% of human acute myeloid leukemia blasts.es_ES
dc.language.isoenges_ES
dc.publisherAmerican Society of Microbiologyes_ES
dc.subjectgene therapy es_ES
dc.subjecttargetinges_ES
dc.subjectLentiviral vectorses_ES
dc.subjectMyeloid leukemia cellses_ES
dc.subjectconcentrationes_ES
dc.subjectConjugationes_ES
dc.titleConjugation of lentivirus to paramagnetic particles via non-viral proteins allows efficient concentration and infection of primary Acute Myeloid Leukaemia cellses_ES
dc.typejournal articlees_ES
dc.rights.accessRightsopen accesses_ES
dc.identifier.doi10.1128/JVI.79.20.13190-13194.2005
dc.type.hasVersionAOes_ES


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