A New Generation of Retroviral Producer Cells: Predictable and Stable Virus Production by Flp-Mediated Site-Specific Integration of Retroviral Vectors

Schucht, Roland; Coroadinha, Ana S.; Zanta-Boussif, Maria Antonietta; Verhoeyen, Els; Carrondo, Manuel J.T.; Hauser, Hansjörg; Wirth, Dagmar

doi:10.1016/j.ymthe.2005.12.003

Cited by 63 publications

(92 citation statements)

References 42 publications

(45 reference statements)

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“…It contains Flp recombination targets F-WT and F-5 flanking the viral genome. EMCV-IRES elements and an ATG start codon are positioned upstream to the F-5 site to complement the ATG-deficient neomycin-phosphotransferase expression upon targeting (for details consult Verhoeyen et al, 2001;Schucht et al, 2006).…”

Section: Lentiviral Vectorsmentioning

confidence: 99%

“…It is well known that a critical parameter is the nature of the vector integration site, which defines the expression and thus the titer. This has been studied for single copy vector integration events (Coroadinha et al, 2006;Schucht et al, 2006). Conceptually, safe (i.e., defined and genetically stable) production systems for c-retroviral and lentiviral vectors require a low copy number or, most beneficially, a single vector copy integrated into the producer cell genome.…”

Section: Introductionmentioning

confidence: 99%

“…c-Retroviral modular producer cell lines have been established that allow production of high titer vectors from single, defined chromosomal sites (Gama-Norton et al, 2010;Coroadinha et al, 2006;Schucht et al, 2006;Loew et al, 2010). This permits production of c-retroviral vectors in a predictable and controlled manner (Coroadinha et al, 2006;Schucht et al, 2006;Loew et al, 2010;Gama-Norton et al, 2010).…”

Section: Introductionmentioning

confidence: 99%

“…This permits production of c-retroviral vectors in a predictable and controlled manner (Coroadinha et al, 2006;Schucht et al, 2006;Loew et al, 2010;Gama-Norton et al, 2010). However, the development of cellular systems that exploit single chromosomal loci for the production of lentiviral vectors in a predictable and controlled manner has not been achieved so far.…”

Section: Introductionmentioning

confidence: 99%

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Lentivirus Production Is Influenced by SV40 Large T-Antigen and Chromosomal Integration of the Vector in HEK293 Cells

et al. 2011

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Currently, lentiviral vectors for research and gene therapy are produced from 293-T cells that are transiently transfected with plasmids encoding the vector and helper functions. However, transiently transfected vectors as well as the presence of SV40 virus large T-antigen (T-Ag) cause serious technical and safety considerations. We aimed to exploit single copy integration sites in the HEK293 genome supporting lentiviral vector production. We found that lentiviral vectors result in minimal infectious particle production from single copy integrants in HEK293. Moreover, once this cell line harbors single copy integrations of lentiviral vectors, its ability to transiently produce lentiviral vectors becomes strongly impaired. T-Ag has a dramatic effect on virus production. Low levels of constitutive T-Ag expression can overcome the production restriction imposed by integrated lentiviral vectors copies. Interestingly, T-Ag does not exert its role at the level of transcriptional activity of the vector; rather, it seems to impose an indirect effect on the cell thereby enabling lentiviral vector production. Altogether, our study highlights the restrictions for integrated lentiviral vectors that are relevant for the establishment of stable and safe producer cell lines.

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Section: Lentiviral Vectorsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Lentivirus Production Is Influenced by SV40 Large T-Antigen and Chromosomal Integration of the Vector in HEK293 Cells

et al. 2011

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“…89071904) harboring a MFGSnlsLacZ transgene [18]; HEK 293 derived 1B28F cell line producing amphotropic RVs harboring a pEMCeGFPROL coding for GFP protein [19]. Amphotropic lentiviral vectors were produced by the 293T-derived STAR-A cell line (ECCAC no.…”

Section: Cell Lines and Culture Conditionsmentioning

confidence: 99%

Removal of envelope protein‐free retroviral vectors by anion‐exchange chromatography to improve product quality

Rodrigues

Alves

Lopes

et al. 2008

J of Separation Science

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Original PaperRemoval of envelope protein-free retroviral vectors by anion-exchange chromatography to improve product qualityWe have investigated the role of the retroviral lipid bilayer and envelope proteins in the adsorption of retroviral vectors (RVs) to a Fractogel TM DEAE matrix. Intact RVs and their degradation components (envelope protein-free vectors and solubilized vector components) were adsorbed to this matrix and eluted using a linear gradient. Envelope protein-free RVs (Env -) and soluble envelope proteins (gp70) eluted in a significantly lower range of conductivities than intact RVs (Env + ) (13.7 -30 mS/cm for Env -and gp70 proteins vs. 47 -80 mS/cm for Env + ). The zeta (f)-potential of Env + and Env -vectors was evaluated showing that envelope proteins define the pI of the viral particles (pI (Env + ) a 2 versus 3 a pI (Env -) a 4) and that Env + and Env -vectors have similar f-potentials within pH 5 and 8. The results presented herein indicate that the adsorption of retroviral particles occurs through multi-point interaction of the envelope proteins with the cationic groups on the chromatographic matrix. The strength of this adsorption is thus dependent on the amount of envelope protein present in the viral lipid bilayer. In conclusion, AEXc enables the separation of gp70 proteins as well as envelope protein-free vectors constituting a significant improvement to the quality of retroviral preparations for gene therapy applications.

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Retroviral vector production under serum deprivation: The role of lipids

Rodrigues

Carmo

Alves

et al. 2009

Biotech & Bioengineering

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The use of retroviral vectors for gene therapy applications demands high titer preparations and stringent quality standards. However, the manufacturing of these vectors still represents a highly challenging task due to the low productivity of the cell lines and reduced stability of the vector infectivity, particularly under serum-free conditions. With the objective of understanding the major limitations of retroviral vector production under serum deprivation, a thorough study of viral production kinetics, vector characterization and cell growth and metabolic behavior was conducted, for 293 FLEX 18 and Te Fly Ga 18 producer cell lines using different serum concentrations. The reduction of serum supplementation in the culture medium resulted in pronounced decreases in cell productivity of infectious vector, up to ninefold in 293 FLEX 18 cells and sevenfold in Te Fly Ga 18 cells. Total particles productivity was maintained, as assessed by measuring viral RNA; therefore, the decrease in infectious vector production could be attributed to higher defective particles output. The absence of the serum lipid fraction was found to be the major cause for this decrease in cell viral productivity. The use of delipidated serum confirmed the requirement of serum lipids, particularly cholesterol, as its supplementation not only allowed the total recovery of viral titers as well as additional production increments in both cell lines when comparing with the standard 10% (v/v) FBS supplementation. This work identified lower production ratios of infectious particles/total particles as the main restraint of retroviral vector production under serum deprivation; this is of the utmost importance concerning the clinical efficacy of the viral preparations. Lipids were confirmed as the key serum component correlated with the production of infective retroviral vectors and this knowledge can be used to efficiently design medium supplementation strategies for serum-free production. Biotechnol. Bioeng. 2009; 104: 1171-1181. (c) 2009 Wiley Periodicals, Inc.

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A New Generation of Retroviral Producer Cells: Predictable and Stable Virus Production by Flp-Mediated Site-Specific Integration of Retroviral Vectors

Cited by 63 publications

References 42 publications

Lentivirus Production Is Influenced by SV40 Large T-Antigen and Chromosomal Integration of the Vector in HEK293 Cells

Lentivirus Production Is Influenced by SV40 Large T-Antigen and Chromosomal Integration of the Vector in HEK293 Cells

Removal of envelope protein‐free retroviral vectors by anion‐exchange chromatography to improve product quality

Retroviral vector production under serum deprivation: The role of lipids

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