Characterization of a quail suspension cell line for production of a fusogenic oncolytic virus

Göbel, Sven; Jaén, Karim E; Fernandes, Rita P.; Reiter, Manfred; Altomonte, Jennifer; Reichl, Udo; Genzel, Yvonne

doi:10.1002/bit.28530

Cited by 6 publications

(2 citation statements)

References 51 publications

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“…Currently, the ambr15 system is predominantly used in CHO CLD and to a lesser extent in the field of cell and gene therapy. For vaccine manufacturing, we are only aware of a SARS‐CoV‐2 production process simulation involving adherent Vero cells on macrocarriers, a virus‐like particle vaccine against Chikungunya virus and a cancer vaccine [ 46 , 47 , 48 , 49 ]. With our study, we can add another example for virus production and showcase the usefulness of the system for screenings.…”

Section: Resultsmentioning

confidence: 99%

From single‐cell cloning to high‐yield influenza virus production – implementing advanced technologies in vaccine process development

Zinnecker,

Badri,

Araujo

et al. 2024

Engineering in Life Sciences

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Innovations in viral vaccine manufacturing are crucial for pandemic preparedness and to meet ever‐rising global demands. For influenza, however, production still mainly relies on technologies established decades ago. Although modern production shifts from egg‐based towards cell culture technologies, the full potential has not yet been fully exploited. Here, we evaluate whether implementation of state‐of‐the‐art technologies for cell culture‐based recombinant protein production are capable to challenge outdated approaches in viral vaccine process development. For this, a fully automated single‐cell cloning strategy was established to generate monoclonal suspension Madin‐Darby canine kidney (MDCK) cells. Among selected cell clones, we could observe distinct metabolic and growth characteristics, with C59 reaching a maximum viable cell concentration of 17.3 × 106 cells/mL and low doubling times in batch mode. Screening for virus production using a panel of human vaccine‐relevant influenza A and B viruses in an ambr15 system revealed high titers with yields competing or even outperforming available MDCK cell lines. With C113, we achieved cell‐specific virus yields of up to 25,000 virions/cell, making this cell clone highly attractive for vaccine production. Finally, we confirmed process performance at a 50‐fold higher working volume. In summary, we present a scalable and powerful approach for accelerated development of high‐yield influenza virus production in chemically defined medium starting from a single cell.

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Section: Resultsmentioning

confidence: 99%

From single‐cell cloning to high‐yield influenza virus production – implementing advanced technologies in vaccine process development

Zinnecker,

Badri,

Araujo

et al. 2024

Engineering in Life Sciences

Self Cite

View full text Add to dashboard Cite

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“…I.B. sVero monkey sus SFM4-sVero 4.6E+06 na nd nd nd nd nd STR, P 49, 119 CCX.E10 avian sus SFM 8.5E+06 5.0E+06 nd #, nd FFA 1.00E+08 nd 200 Spinner, B p.c.M.W., 120 DuckCelt-T17 avian sus Optipro SFM 1.1E+07 1.0E+06 1.8 log 2 (HAU/100 µL) nd 3.20E+08 nd 320 TubeSpin, B 37, 121 PBS-12SF avian adh Optipro SFM nd nd 36 HAU/50 µL #, 1.9 3.39E+09 nd nd 12 well, B 122 PER.C6 human sus Ex-Cell 525 medium 3.0E+06 3.0E+06 2100 HAU #, 3.3 1.00E+10 …”

Section: Cell Culture-based Influenza Virus Productionmentioning

confidence: 99%

Innovations in cell culture-based influenza vaccine manufacturing – from static cultures to high cell density cultivations

Zinnecker,

Reichl,

Genzel

2024

Human Vaccines & Immunotherapeutics

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Production of recombinant vesicular stomatitis virus-based vectors by tangential flow depth filtration

Göbel,

Pelz,

Silva

et al. 2024

Appl Microbiol Biotechnol

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Cell culture-based production of vector-based vaccines and virotherapeutics is of increasing interest. The vectors used not only retain their ability to infect cells but also induce robust immune responses. Using two recombinant vesicular stomatitis virus (rVSV)-based constructs, we performed a proof-of-concept study regarding an integrated closed single-use perfusion system that allows continuous virus harvesting and clarification. Using suspension BHK-21 cells and a fusogenic oncolytic hybrid of vesicular stomatitis virus and Newcastle disease virus (rVSV-NDV), a modified alternating tangential flow device (mATF) or tangential flow depth filtration (TFDF) systems were used for cell retention. As the hollow fibers of the former are characterized by a large internal lumen (0.75 mm; pore size 0.65 μm), membrane blocking by the multi-nucleated syncytia formed during infection could be prevented. However, virus particles were completely retained. In contrast, the TFDF filter unit (lumen 3.15 mm, pore size 2–5 μm) allowed not only to achieve high viable cell concentrations (VCC, 16.4–20.6×106 cells/mL) but also continuous vector harvesting and clarification. Compared to an optimized batch process, 11-fold higher infectious virus titers were obtained in the clarified permeate (maximum 7.5×109 TCID50/mL). Using HEK293-SF cells and a rVSV vector expressing a green fluorescent protein, perfusion cultivations resulted in a maximum VCC of 11.3×106 cells/mL and infectious virus titers up to 7.1×1010 TCID50/mL in the permeate. Not only continuous harvesting but also clarification was possible. Although the cell-specific virus yield decreased relative to a batch process established as a control, an increased space-time yield was obtained. Key points • Viral vector production using a TFDF perfusion system resulted in a 460% increase in space-time yield • Use of a TFDF system allowed continuous virus harvesting and clarification • TFDF perfusion system has great potential towards the establishment of an intensified vector production

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Characterization of a quail suspension cell line for production of a fusogenic oncolytic virus

Cited by 6 publications

References 51 publications

From single‐cell cloning to high‐yield influenza virus production – implementing advanced technologies in vaccine process development

From single‐cell cloning to high‐yield influenza virus production – implementing advanced technologies in vaccine process development

Innovations in cell culture-based influenza vaccine manufacturing – from static cultures to high cell density cultivations

Production of recombinant vesicular stomatitis virus-based vectors by tangential flow depth filtration

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