Inducible Overexpression of a Toxic Protein by an Adenovirus Vector with a Tetracycline-Regulatable Expression Cassette

Massie, Bernard; Lamoureux, Linda; Mosser, Dick D.; Guilbault, Claire; Jolicœur, Pierre; Bart, François; Langelier, Yves

doi:10.1128/jvi.72.3.2289-2296.1998

Cited by 110 publications

(71 citation statements)

References 38 publications

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“…While we have demonstrated that direct injection (9) or retrograde perfusion of the salivary gland resulted in the induction of a protective immune response using an attenuated (tcMCMV) viral system, to be generally applicable as a site for vaccination, it was necessary to demonstrate that direct protein expression in the salivary gland such as that delivered via a noninfectious, conventional subunit vaccine, could also elicit effective and functionally protective immunity. Recombinant adenoviruses are a versatile tool for gene delivery and expression, since they are able to infect a broad range of cell types, and infection is not dependent on active host cell division (31,32). The most commonly used adenoviral vectors are typically devoid of E1 and E3 genes, which not only render the virus incapable of replication but also make room for the insertion of up to 7.5 kb of foreign DNA (33,34).…”

Section: Discussionmentioning

confidence: 99%

Protective MCMV immunity by vaccination of the salivary glandviaWharton's duct: replication‐deficient recombinant adenovirus expressing individual MCMV genes elicits protection similar to that of MCMV

et al. 2014

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Salivary glands, a major component of the mucosal immune system, confer antigen-specific immunity to mucosally acquired pathogens. We investigated whether a physiological route of inoculation and a subunit vaccine approach elicited MCMV-specific and protective immunity. Mice were inoculated by retrograde perfusion of the submandibular salivary glands via Wharton's duct with tcMCMV or MCMV proteins focused to the salivary gland via replication-deficient adenovirus expressing individual MCMV genes (gB, gH, IE1; controls: saline and replication deficient adenovirus without MCMV inserts). Mice were evaluated for MCMV-specific antibodies, T-cell responses, germinal center formation, and protection against a lethal MCMV challenge. Retrograde perfusion with tcMCMV or adenovirus expressed MCMV proteins induced a 2- to 6-fold increase in systemic and mucosal MCMV-specific antibodies, a 3- to 6-fold increase in GC marker expression, and protection against a lethal systemic challenge, as evidenced by up to 80% increased survival, decreased splenic pathology, and decreased viral titers from 10(6) pfu to undetectable levels. Thus, a focused salivary gland immunization via a physiological route with a protein antigen induced systemic and mucosal protective immune responses. Therefore, salivary gland immunization can serve as an alternative mucosal route for administering vaccines, which is directly applicable for use in humans.

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Section: Discussionmentioning

confidence: 99%

Protective MCMV immunity by vaccination of the salivary glandviaWharton's duct: replication‐deficient recombinant adenovirus expressing individual MCMV genes elicits protection similar to that of MCMV

et al. 2014

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“…Several reports have previously described the use of a replication deficient adenovirus in combination with adenovirus production cells (HEK293) with the aim to produce recombinant protein (Andersen and Krummen, 2002;Cô té et al, 1998;Garnier et al, 1994;Lamarche et al, 1990;Massie et al, 1995Massie et al, , 1998. In these studies, the E1-deleted vector was allowed to replicate in HEK293 cells, in the process yielding high amounts (4-20% total cell protein) of the protein of interest.…”

Section: Discussionmentioning

confidence: 99%

Serum‐free transient protein production system based on adenoviral vector and PER.C6 technology: High yield and preserved bioactivity

Havenga

Holterman

Melis

et al. 2007

Biotech & Bioengineering

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Stable E1 transformed cells, like PER.C6, are able to grow at scale and to high cell densities. E1-deleted adenoviruses replicate to high titer in PER.C6 cells whereas subsequent deletion of E2A from the vector results in absence of replication in PER.C6 cells and drastically lowers the expression of adenovirus proteins in such cells. We therefore considered the use of an DeltaE1/DeltaE2 type 5 vector (Ad5) to deliver genes to PER.C6 cells growing in suspension with the aim to achieve high protein yield. To evaluate the utility of this system we constructed DeltaE1/DeltaE2 vector carrying different classes of protein, that is, the gene coding for spike protein derived from the Coronavirus causing severe acute respiratory syndrome (SARS-CoV), a gene coding for the SARS-CoV receptor or the genes coding for an antibody shown to bind and neutralize SARS-CoV (SARS-AB). The DeltaE1/DeltaE2A-vector backbones were rescued on a PER.C6 cell line engineered to constitutively over express the Ad5 E2A protein. Exposure of PER.C6 cells to low amounts (30 vp/cell) of DeltaE1/DeltaE2 vectors resulted in highly efficient (>80%) transduction of PER.C6 cells growing in suspension. The efficient cell transduction resulted in high protein yield (up to 60 picogram/cell/day) in a 4 day batch production protocol. FACS and ELISA assays demonstrated the biological activity of the transiently produced proteins. We therefore conclude that DeltaE1/DeltaE2 vectors in combination with the PER.C6 technology may provide a viable answer to the increasing demand for high quality, high yield recombinant protein.

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“…High-level recombinant protein production using AdVs was shown to be possible by using cells other than CHO cells (29,31,41,42). The cells used were either permissive for the replication of AdVs, such as 293 cells, or were non-permissive, such as HeLa, A549, or KB cells.…”

Section: Discussionmentioning

confidence: 99%

“…This plasmid contains also the 9.4-15.5 map unit segment of Ad5 genome for homologous recombination with Ad5-∆PS (see below). A plasmid (pMPG-BFP/CMV-cTA/tk-neo) expressing the cTA and the blue fluorescent protein (BFP) regulated by the CMV5 promoter (29,31) was constructed by replacing the IgG heavy and light chains of pMPG/chB43_TK/neo (32) with the cTA coding sequence excised from pAdCMV5-cTA (28) and the gene for BFP (29).…”

Section: Methodsmentioning

confidence: 99%

“…An E1/E3-deleted AdV encoding GFP (Qbiogene) regulated by the CR5 promoter (AdCR5-GFP) was generated by first replacing the Tet-regulated promoter (TR5) from pAdTR5-GFP (31) by the CR5 promoter isolated from pAdCR5-LacZ (28). The resulting plasmid (pAdCR5-GFP) was then used to produce AdCR5-GFP by homologous recombination after transfection of 293A cells with a mixture of linearized pAdCR5-GFP and E1/E3-deleted Ad5 DNA as described previously (31). AdCR5-GFP was then grown by sequential passages on BMAdE1 cells, except for the last passage, which was done on 293A cells, using standard procedure (35).…”

Section: Methodsmentioning

confidence: 99%

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High‐Level Recombinant Protein Production in CHO Cells Using an Adenoviral Vector and the Cumate Gene‐Switch

Gaillet

Gilbert

Amziani

et al. 2007

Biotechnology Progress

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To facilitate and accelerate the production of eukaryotic proteins with correct post-translational modifications, we have developed a protein production system based on the transduction of Chinese hamster ovary (CHO) cells using adenovirus vectors (AdVs). We have engineered a CHO cell line (CHO-cTA) that stably expresses the transactivator (cTA) of our newly developed cumate gene-switch transcription system. This cell line is adapted to suspension culture and can grow in serum-free and protein-free medium. To increase the transduction level of AdVs, we have also generated a cell line (CHO-cTA-CAR) that expresses additional amounts of the coxackievirus and adenovirus receptor (CAR) on its surface. Recombinant protein production was tested using an AdV carrying the secreted alkaline phosphatase (SEAP) under the control of the CR5 promoter, which is strongly and specifically activated by binding to cTA. The SEAP expression was linked to the expression of the green fluorescent protein (GFP) through an internal ribosome entry site (IRES) to facilitate titration of the AdV. We monitored SEAP expression on a daily basis for 9 days after transduction of CHO-cTA and CHO-cTA-CAR using different quantities of AdVs at 37 and 30 degrees C. Incubation at the latter temperature increased the production of SEAP at least 10-fold, and the presence of CAR increased the transduction level of the AdV. Maximum SEAP production (63 mg/L) was achieved at 6-7 days post-infection at 30 degrees C by transducing CHO-cTA-CAR with 500 infectious particles/cell. Because numerous AdVs can now be generated within a few weeks and large-scale production of AdVs is now a routine procedure, this system could be used to produce rapidly milligram quantities of a battery of recombinant proteins as well as for large-scale protein production.

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Inducible Overexpression of a Toxic Protein by an Adenovirus Vector with a Tetracycline-Regulatable Expression Cassette

Cited by 110 publications

References 38 publications

Protective MCMV immunity by vaccination of the salivary glandviaWharton's duct: replication‐deficient recombinant adenovirus expressing individual MCMV genes elicits protection similar to that of MCMV

Protective MCMV immunity by vaccination of the salivary glandviaWharton's duct: replication‐deficient recombinant adenovirus expressing individual MCMV genes elicits protection similar to that of MCMV

Serum‐free transient protein production system based on adenoviral vector and PER.C6 technology: High yield and preserved bioactivity

High‐Level Recombinant Protein Production in CHO Cells Using an Adenoviral Vector and the Cumate Gene‐Switch

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