Immunogenicity and protection efficacy of a COVID-19 DNA vaccine encoding spike protein with D614G mutation and optimization of large-scale DNA vaccine production

Author:

Gül Aytül,Erkunt Alak Sedef,Can Hüseyin,Karakavuk Muhammet,Korukluoğlu Gülay,Altaş Ayşe Başak,Gül Ceren,Karakavuk Tuğba,Köseoğlu Ahmet Efe,Ülbeği Polat Hivda,Yazıcı Malkoçoğlu Hilal,Taş Ekiz Arzu,Abacı İrem,Aksoy Özge,Enül Hakan,Adıay Cumhur,Uzar Serdar,Saraç Fahriye,Ün Cemal,Gürüz Adnan Yüksel,Kantarcı Ayşe Gülten,Akbaba Hasan,Erel Akbaba Gülşah,Yılmaz Habibe,Değirmenci Döşkaya Aysu,Taşbakan Meltem,Pullukçu Hüsnü,Karasulu Ercüment,Tekin Şaban,Döşkaya Mert

Abstract

AbstractSevere acute respiratory syndrome coronavirus 2 had devastating consequences for human health. Despite the introduction of several vaccines, COVID-19 continues to pose a serious health risk due to emerging variants of concern. DNA vaccines gained importance during the pandemic due to their advantages such as induction of both arms of immune response, rapid development, stability, and safety profiles. Here, we report the immunogenicity and protective efficacy of a DNA vaccine encoding spike protein with D614G mutation (named pcoSpikeD614G) and define a large-scale production process. According to the in vitro studies, pcoSpikeD614G expressed abundant spike protein in HEK293T cells. After the administration of pcoSpikeD614G to BALB/c mice through intramuscular (IM) route and intradermal route using an electroporation device (ID + EP), it induced high level of anti-S1 IgG and neutralizing antibodies (P < 0.0001), strong Th1-biased immune response as shown by IgG2a polarization (P < 0.01), increase in IFN-γ levels (P < 0.01), and increment in the ratio of IFN-γ secreting CD4+ (3.78–10.19%) and CD8+ (5.24–12.51%) T cells. Challenging K18-hACE2 transgenic mice showed that pcoSpikeD614G administered through IM and ID + EP routes conferred 90–100% protection and there was no sign of pneumonia. Subsequently, pcoSpikeD614G was evaluated as a promising DNA vaccine candidate and scale-up studies were performed. Accordingly, a large-scale production process was described, including a 36 h fermentation process of E. coli DH5α cells containing pcoSpikeD614G resulting in a wet cell weight of 242 g/L and a three-step chromatography for purification of the pcoSpikeD614G DNA vaccine.

Publisher

Springer Science and Business Media LLC

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