2014
DOI: 10.1038/gt.2014.37
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Comparative analysis of enzymatically produced novel linear DNA constructs with plasmids for use as DNA vaccines

Abstract: The use of DNA to deliver vaccine antigens offers many advantages, including ease of manufacture and cost. However, most DNA vaccines are plasmids and must be grown in bacterial culture, necessitating elements which are either unnecessary for effective gene delivery (e.g. bacterial origins of replication) or undesirable (e.g. antibiotic resistance genes). Removing these elements may improve the safety profile of DNA for the delivery of vaccines. Here we describe a novel, double-stranded, linear DNA construct p… Show more

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Cited by 45 publications
(53 citation statements)
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“…Although not statistically significant, there was also a trend toward a lower proportion of T cells expressing CAR in CAR19 T cell cultures generated using only dbDNA. These findings are consistent with previous reports of a trend toward reduced expression from dbDNA compared to an equimolar amount of plasmid 30 and that piggyBac transposition occurs more efficiently from circular than linear donor vectors. 45 Transfection of an equal mass of dbDNA to plasmid leads to equivalent levels of expression, 30,31 and this approach might also improve CAR expression in this setting.…”
Section: Discussionsupporting
confidence: 93%
See 1 more Smart Citation
“…Although not statistically significant, there was also a trend toward a lower proportion of T cells expressing CAR in CAR19 T cell cultures generated using only dbDNA. These findings are consistent with previous reports of a trend toward reduced expression from dbDNA compared to an equimolar amount of plasmid 30 and that piggyBac transposition occurs more efficiently from circular than linear donor vectors. 45 Transfection of an equal mass of dbDNA to plasmid leads to equivalent levels of expression, 30,31 and this approach might also improve CAR expression in this setting.…”
Section: Discussionsupporting
confidence: 93%
“…Doggybones (dbDNA) are minimal DNA vectors that can be produced enzymatically in vitro at scale. [30][31][32] As production does not involve bacteria, the issues associated with plasmids are avoided. No origin of replication sequences or antibiotic-resistance genes is required, and the risk of recombination events within bacteria is eliminated.…”
Section: Introductionmentioning
confidence: 99%
“…Alternatively, one might create plasmids that do not contain the ORI and thus only a single corepromoter that one should be able to choose freely. A family of vectors designed to remove prokaryotic parts of the plasmid after amplification in bacteria (minicircles [10][11][12] or in vitro synthesis (doggybones 13 ) could be such alternatives, as might be different lower copy ORIs. Alternatively, one could screen linear DNA fragments that lack the ORI (e.g.…”
Section: Discussionmentioning
confidence: 99%
“…For infectious pathogens, two major types of RNA vaccine have been utilized: nonreplicating and self-amplifying. The recent development of scalable, cell-free, enzyme-driven DNA production technologies strengthens the case for the translatability of DNA vaccines [51]. Self-amplifying RNA systems can be based on sequences and principles borrowed from single-positive strand RNA viruses, such as alphaviruses (Alphavax).…”
Section: J Wallis Et Almentioning
confidence: 99%
“…Should the delivery barrier faced by DNA be overcome, a resurgence in the interest in its use may follow. The recent development of scalable, cell-free, enzyme-driven DNA production technologies strengthens the case for the translatability of DNA vaccines [51].…”
Section: Nucleic Acid Vaccinesmentioning
confidence: 99%