The Development of Methods for the Production of New Molecular Vaccines and Appropriate RNA Fragments to Counteract Unwanted Genes: A Pilot Study

Iskra Sainova; Vera Kolyovska; Iliana Ilieva; Tzvetanka Markova; Dimitrina Dimitrova-Dikanarova; Radka Hadjiolova

doi:10.3390/vaccines11071226

The Development of Methods for the Production of New Molecular Vaccines and Appropriate RNA Fragments to Counteract Unwanted Genes: A Pilot Study

Vaccines (Basel). 2023 Jul 11;11(7):1226. doi: 10.3390/vaccines11071226.

Authors

Iskra Sainova¹, Vera Kolyovska¹, Iliana Ilieva¹, Tzvetanka Markova², Dimitrina Dimitrova-Dikanarova³, Radka Hadjiolova⁴

Affiliations

¹ Institute of Experimental Morphology, Pathology and Anthropology with Museum (IEMPAM) to Bulgarian Academy of Sciences (BAS), 1113 Sofia, Bulgaria.
² Department of Pharmacology and Toxicology, Medical University of Sofia, 1431 Sofia, Bulgaria.
³ Department of Biology, Medical University of Sofia, 1431 Sofia, Bulgaria.
⁴ Department of Pathophysiology, Medical University of Sofia, 1431 Sofia, Bulgaria.

Abstract

The potential of viruses as appropriate vectors for the development of new therapeutic strategies, as well as for the design of molecular (DNA, RNA, and/or protein) vaccines via substitution of nucleotide sequences, has been proven. Among the most appropriate DNA and/or RNA fragments, members belonging to families Parvoviridae (particularly adeno-associated virus, AAV) and Poxviridae have frequently been suggested for this purpose. In previous studies, the vaccine avipoxvirus strains FK (fowl) and Dessau (pigeon) have been proven able to infect mammalian cells (as well as avian cells), and to replicate productively in a small number of them; thus, we may be able to adapt them using incubation, and in these conditions. Additionally, we have previously proved, based on AAV recombinant DNA vectors, that it is possible to transfer appropriate genes of interest via mouse embryonic stem cells (mESCs). In the current study, we develop methods for the application of the same vaccine avipoxviral strains, based on the AAV DNA genome recombinant constructs, to be used for gene transfer in cells, for the transfer of DNA and/or RNA fragments (for the suppression of unwanted viral and/or cellular genes), and for the production of molecular (DNA, RNA, and/or protein) anti-cancer and anti-viral vaccines. To this end, sub-populations of embryonic mammalian cells infected with the two forms of both vaccine avipoxviral strains were frozen in the presence of cryo-protector dimethylsulfoxide (DMSO), subsequently thawed, and re-incubated. In most cases, the titers of the intra-cellular forms of the two strains were higher than those of their extra-cellular forms. These data were explained by the probable existence of the intra-cellular forms as different sub-forms, including those integrated in the cellular genome proviruses at a given stage of the cellular infection, and suggest the possibility of transferring nucleotide (DNA and/or RNA) fragments between cellular and viral genomes; this is due to the influence of activated fusion processes on DMSO, as well as drastic temperature variations.

Keywords: adeno-associated virus DNA vectors; in vitro incubated cells; intra- and extracellular virus forms; vaccine avipoxviral strains.

Grants and funding

This research was funded by the project with number D-137/14.06.2022.