Time- and cost-effective production of untagged recombinant MVA by flow virometry and direct virus sorting

Daniela Boselli; Maddalena Panigada; Simona Di Terlizzi; Monica Romanò; Emanuele Canonico; Chiara Villa; Claudia Minici; Eelco van Anken; Elisa Soprana; Antonio G. Siccardi

doi:10.1186/s12967-023-04353-7

Journal of Translational Medicine (Jul 2023)

Time- and cost-effective production of untagged recombinant MVA by flow virometry and direct virus sorting

Daniela Boselli,
Maddalena Panigada,
Simona Di Terlizzi,
Monica Romanò,
Emanuele Canonico,
Chiara Villa,
Claudia Minici,
Eelco van Anken,
Elisa Soprana,
Antonio G. Siccardi

Affiliations

Daniela Boselli: FRACTAL - San Raffaele Scientific Institute
Maddalena Panigada: Division of Genetics and Cell Biology, San Raffaele Scientific Institute
Simona Di Terlizzi: FRACTAL - San Raffaele Scientific Institute
Monica Romanò: FRACTAL - San Raffaele Scientific Institute
Emanuele Canonico: FRACTAL - San Raffaele Scientific Institute
Chiara Villa: FRACTAL - San Raffaele Scientific Institute
Claudia Minici: Division of Genetics and Cell Biology, San Raffaele Scientific Institute
Eelco van Anken: Università Vita-Salute San Raffaele
Elisa Soprana: Division of Genetics and Cell Biology, San Raffaele Scientific Institute
Antonio G. Siccardi: Division of Genetics and Cell Biology, San Raffaele Scientific Institute

DOI: https://doi.org/10.1186/s12967-023-04353-7
Journal volume & issue: Vol. 21, no. 1
pp. 1 – 14

Abstract

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Abstract Background Recombinant MVAs (rMVAs) are widely used both in basic and clinical research. Our previously developed Red-to-Green Gene Swapping Method (RGGSM), a cytometry-based Cell-Sorting protocol, revolves around the transient expression of a green fluorescent cytoplasmic marker, to subsequently obtain purified untagged rMVA upon loss of that marker by site-specific recombination. The standard RGSSM is quite costly in terms of bench work, reagents, and Sorting Facility fees. Although faster than other methods to obtain recombinant MVAs, the standard RGSSM still is time-consuming, taking at least 25 days to yield the final product. Methods The direct sorting of fluorescent virions is made amenable by the marker HAG, a flu hemagglutinin/EGFP fusion protein, integrated into the external envelope of extracellular enveloped virions (EEVs). Fluorescent EEVs-containing supernatants of infected cultures are used instead of purified virus. Direct Virus-Sorting was performed on BD FACSAria Fusion cell sorter equipped with 4 lasers and a 100-mm nozzle, with 20 psi pressure and a minimal flow rate, validated using Megamix beads. Results Upon infection of cells with recombinant EEVs, at the first sorting step virions that contain HAG are harvested and cloned, while the second sorting step yields EEVs that have lost HAG, allowing to clone untagged rMVA. Because only virion-containing supernatants are used, no virus purification steps and fewer sortings are necessary. Therefore, the final untagged rMVA product can be obtained in a mere 8 days. Conclusions Altogether, we report that the original RGSSM has been markedly improved in terms of time- and cost efficiency by substituting Cell-Sorting with direct Virus-Sorting from the supernatants of infected cells. The improved virometry-based RGGSM may find wide applicability, considering that rMVAs hold great promise to serve as personalized vaccines for therapeutic intervention against cancer and various types of infectious diseases. Graphical Abstract

Published in Journal of Translational Medicine

ISSN: 1479-5876 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine
Website: https://translational-medicine.biomedcentral.com/

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