Your search keyword '"Edith Lupu"' showing total 9 results

1. Development and Validation of a Plaque Assay to Determine the Titer of a Recombinant Live-Attenuated Viral Vaccine for SARS-CoV-2

Author

Einat Toister, Lilach Cherry, Edith Lupu, Arik Monash, Eyal Dor, Lilach Levin, Meni Girshengorn, Niva Natan, Shira Chapman, Shlomo Shmaya, Eyal Epstein, Yaakov Adar, Ran Zichel, Yakir Ophir, and Eran Diamant

Subjects

PFU, plaque assay, validation, SARS-CoV-2, COVID-19, vaccine, Medicine

Abstract

The COVID-19 pandemic, caused by severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), has resulted in more than seven million deaths worldwide. To reduce viral spread, the Israel Institute for Biological Research (IIBR) developed and produced a new rVSV-SARS-CoV-2-S vaccine candidate (BriLife®) based on a platform of a genetically engineered vesicular stomatitis virus (VSV) vector that expresses the spike protein of SARS-CoV-2 instead of the VSV-G protein on the virus surface. Quantifying the virus titer to evaluate vaccine potency requires a reliable validated assay that meets all the stringent pharmacopeial requirements of a bioanalytical method. Here, for the first time, we present the development and extensive validation of a quantitative plaque assay using Vero E6 cells for the determination of the concentration of the rVSV-SARS-CoV-2-S viral vector. Three different vaccine preparations with varying titers (DP_low, DP_high, and QC sample) were tested according to a strict validation protocol. The newly developed plaque assay was found to be highly specific, accurate, precise, and robust. The mean deviations from the predetermined titers for the DP_low, DP_high, and QC preparations were 0.01, 0.02, and 0.09 log10, respectively. Moreover, the mean %CV values for intra-assay precision were 18.7%, 12.0%, and 6.0%, respectively. The virus titers did not deviate from the established values between cell passages 5 and 19, and no correlation was found between titer and passage. The validation results presented herein indicate that the newly developed plaque assay can be used to determine the concentration of the BriLife® vaccine, suggesting that the current protocol is a reliable methodology for validating plaque assays for other viral vaccines.

Published

2024

2. Thermophilic Filamentous Fungus C1-Cell-Cloned SARS-CoV-2-Spike-RBD-Subunit-Vaccine Adjuvanted with Aldydrogel®85 Protects K18-hACE2 Mice against Lethal Virus Challenge

Author

Ram Nechooshtan, Sharon Ehrlich, Marika Vitikainen, Arik Makovitzki, Eyal Dor, Hadar Marcus, Idan Hefetz, Shani Pitel, Marilyn Wiebe, Anne Huuskonen, Lilach Cherry, Edith Lupu, Yehuda Sapir, Tzvi Holtzman, Moshe Aftalion, David Gur, Hadas Tamir, Yfat Yahalom-Ronen, Yuval Ramot, Noam Kronfeld, David Zarling, Anne Vallerga, Ronen Tchelet, Abraham Nyska, Markku Saloheimo, Mark Emalfarb, and Yakir Ophir

Subjects

COVID-19, antigen, pandemic, SARS-CoV-2, receptor binding domain, RBD, Medicine

Abstract

SARS-CoV-2 is evolving with increased transmission, host range, pathogenicity, and virulence. The original and mutant viruses escape host innate (Interferon) immunity and adaptive (Antibody) immunity, emphasizing unmet needs for high-yield, commercial-scale manufacturing to produce inexpensive vaccines/boosters for global/equitable distribution. We developed DYAI-100A85, a SARS-CoV-2 spike receptor binding domain (RBD) subunit antigen vaccine expressed in genetically modified thermophilic filamentous fungus, Thermothelomyces heterothallica C1, and secreted at high levels into fermentation medium. The RBD-C-tag antigen strongly binds ACE2 receptors in vitro. Alhydrogel®‘85’-adjuvanted RDB-C-tag-based vaccine candidate (DYAI-100A85) demonstrates strong immunogenicity, and antiviral efficacy, including in vivo protection against lethal intranasal SARS-CoV-2 (D614G) challenge in human ACE2-transgenic mice. No loss of body weight or adverse events occurred. DYAI-100A85 also demonstrates excellent safety profile in repeat-dose GLP toxicity study. In summary, subcutaneous prime/boost DYAI-100A85 inoculation induces high titers of RBD-specific neutralizing antibodies and protection of hACE2-transgenic mice against lethal challenge with SARS-CoV-2. Given its demonstrated safety, efficacy, and low production cost, vaccine candidate DYAI-100 received regulatory approval to initiate a Phase 1 clinical trial to demonstrate its safety and efficacy in humans.

Published

2022

3. Highly Efficient Purification of Recombinant VSV-∆G-Spike Vaccine against SARS-CoV-2 by Flow-Through Chromatography

Author

Elad Lerer, Ziv Oren, Yaron Kafri, Yaakov Adar, Einat Toister, Lilach Cherry, Edith Lupu, Arik Monash, Rona Levy, Eyal Dor, Eyal Epstein, Lilach Levin, Meni Girshengorn, Niva Natan, Ran Zichel, and Arik Makovitzki

Subjects

rVSV, SARS-CoV-2, downstream process, chromatography, membrane adsorbers, Biotechnology, TP248.13-248.65

Abstract

This study reports a highly efficient, rapid one-step purification process for the production of the recombinant vesicular stomatitis virus-based vaccine, rVSV-∆G-spike (rVSV-S), recently developed by the Israel Institute for Biological Research (IIBR) for the prevention of COVID-19. Several purification strategies are evaluated using a variety of chromatography methods, including membrane adsorbers and packed-bed ion-exchange chromatography. Cell harvest is initially treated with endonuclease, clarified, and further concentrated by ultrafiltration before chromatography purification. The use of anion-exchange chromatography in all forms results in strong binding of the virus to the media, necessitating a high salt concentration for elution. The large virus and spike protein binds very strongly to the high surface area of the membrane adsorbents, resulting in poor virus recovery (TM Core 700 resin, which does not require binding and the elution of the virus, is described. rVSV-S cannot enter the inner pores of the resin and is collected in the flow-through eluent. Purification of the rVSV-S virus with CaptoTM Core 700 resulted in viral infectivity above 85% for this step, with the efficient removal of host cell proteins, consistent with regulatory requirements. Similar results were obtained without an initial ultrafiltration step.

Published

2021

4. A Novel Quantitative Multi-Component Serological Assay for SARS-CoV-2 Vaccine Evaluation

Author

Morly Fisher, Alon Manor, Hagar Abramovitch, Ella Fatelevich, Yafa Afrimov, Gal Bilinsky, Edith Lupu, Amir Ben-Shmuel, Itai Glinert, Noa Madar-Balakirski, Hadar Marcus, and Adva Mechaly

Subjects

COVID-19 Vaccines, Immunoglobulin M, SARS-CoV-2, Immunoglobulin G, COVID-19, Humans, Antibodies, Viral, Sensitivity and Specificity, Analytical Chemistry

Abstract

A multi-component microarray, applying a novel analysis algorithm, was developed for quantitative evaluation of the SARS-CoV-2 vaccines' immunogenicity. The array enables simultaneous quantitation of IgG, IgM, and IgA, specific to the SARS-CoV-2 spike, receptor binding domain, and nucleocapsid proteins. The developed methodology is based on calculating an apparent immunoglobulin signal from the linear range of the fluorescent read-outs generated by scanning the microarray slides at different exposure times. A dedicated algorithm, employing a rigorous set of embedded conditions, then generates a normalized signal for each of the unique assays. Qualification of the multi-component array performance (evaluating linearity, extended dynamic-range, specificity, precision, and accuracy) was carried out with an in-house COVID-19, qRT-PCR positive serum, as well as pre-pandemic commercial negative sera. Results were compared to the WHO international standard for anti-SARS-CoV-2 immunoglobulins. Specific IgG, IgM, and IgA signals obtained by this array enabled successful discrimination between SARS-CoV-2 q-RT-PCR positive (seroconverted SARS-CoV-2 patients) and negative (naïve) samples. This array is currently used for evaluation of the humoral response to BriLife, the VSV-based Israeli vaccine during phase I/II clinical trials.

Published

2022

5. A single dose of recombinant VSV-∆G-spike vaccine provides protection against SARS-CoV-2 challenge

Author

Hila Gutman, Shirley Lazar, Itai Glinert, Anat Zvi, Shmuel Yitzhaki, Tomer Israely, Noam Erez, Reut Puni, Shmuel C. Shapira, Einat B. Vitner, Shay Weiss, Dana Stein, Sharon Melamed, Inbar Cohen-Gihon, Haim Levy, Assa Sittner, Adi Beth-Din, Shlomi Lazar, Ohad Mazor, Yaron Vagima, Roy Avraham, Hagit Achdout, Boaz Politi, Ofir Israeli, Yfat Yahalom-Ronen, Nir Paran, Ran Zichel, Hadas Tamir, Edith Lupu, Lilach Cherry, Elad Milrot, Emanuelle Mamroud, Ohad Shifman, Elad Bar-David, Orly Laskar, and Amir Ben-Shmuel

Subjects

0301 basic medicine, viruses, General Physics and Astronomy, Antibodies, Viral, law.invention, 0302 clinical medicine, law, Cricetinae, skin and connective tissue diseases, Antigens, Viral, Lung, Vaccines, Synthetic, Vaccines, Multidisciplinary, biology, Vaccination, Viral Load, 030220 oncology & carcinogenesis, Spike Glycoprotein, Coronavirus, Recombinant DNA, Antibody, Viral load, COVID-19 Vaccines, Science, Dose-Response Relationship, Immunologic, Hamster, Genome, Viral, Vesicular stomatitis Indiana virus, Article, General Biochemistry, Genetics and Molecular Biology, Cell Line, 03 medical and health sciences, Antigen, Animals, SARS-CoV-2, fungi, Body Weight, COVID-19, General Chemistry, Viral membrane, Virology, respiratory tract diseases, body regions, Mice, Inbred C57BL, Disease Models, Animal, 030104 developmental biology, Cell culture, Mutation, biology.protein

Abstract

The COVID-19 pandemic caused by SARS-CoV-2 imposes an urgent need for rapid development of an efficient and cost-effective vaccine, suitable for mass immunization. Here, we show the development of a replication competent recombinant VSV-∆G-spike vaccine, in which the glycoprotein of VSV is replaced by the spike protein of SARS-CoV-2. In-vitro characterization of this vaccine indicates the expression and presentation of the spike protein on the viral membrane with antigenic similarity to SARS-CoV-2. A golden Syrian hamster in-vivo model for COVID-19 is implemented. We show that a single-dose vaccination results in a rapid and potent induction of SARS-CoV-2 neutralizing antibodies. Importantly, vaccination protects hamsters against SARS-CoV-2 challenge, as demonstrated by the abrogation of body weight loss, and alleviation of the extensive tissue damage and viral loads in lungs and nasal turbinates. Taken together, we suggest the recombinant VSV-∆G-spike as a safe, efficacious and protective vaccine against SARS-CoV-2., Here, the authors generate a replication-competent VSV based vaccine expressing SARS-CoV-2 spike protein and show protection in the hamster model with one dose. Analysis of the antibody response in mice shows induction of neutralizing antibodies and suggests a desirable Th1-biased response to the vaccine.

Published

2020

6. Application of Ambr15 system for simulation of entire SARS-CoV-2 vaccine production process involving macrocarriers

Author

Avital Jayson, Michael Goldvaser, Eyal Dor, Arik Monash, Lilach Levin, Lilach Cherry, Edith Lupu, Niva Natan, Meni Girshengorn, Eyal Epstein, and Osnat Rosen

Subjects

Bioreactors, COVID-19 Vaccines, Virus Cultivation, SARS-CoV-2, Chlorocebus aethiops, Cell Culture Techniques, Animals, COVID-19, Humans, Vero Cells, Biotechnology

Abstract

The Ambr15 system is an automated, high-throughput bioreactor platform which comprises 24 individually controlled, single-use stirred-tank reactors. This system plays a critical role in process development by reducing reagent requirements and facilitating high-throughput screening of process parameters. However, until now, the system was used to simulate processes involving cells in suspension or growing on microcarriers and has never been tested for simulating cells growing on macrocarriers. Moreover, to our knowledge, a complete production process including cell growth and virus production has never been simulated. Here, we demonstrate, for the first time, the amenability of the automated Ambr15 cell culture reactor system to simulate the entire SARS-CoV-2 vaccine production process using macrocarriers. To simulate the production process, accessories were first developed to enable insertion of tens of Fibra-Cel macrocarries into the reactors. Vero cell adsorption to Fibra-Cels was then monitored and its adsorption curve was studied. After incorporating of all optimized factors, Vero cells were adsorbed to and grown on Fibra-Cels for several days. During the process, culture medium was exchanged, and the quantity and viability of the cells were followed, resulting in a typical growth curve. After successfully growing cells for 6 days, they were infected with the rVSV-ΔG-Spike vaccine virus. The present results indicate that the Ambr15 system is not only suitable for simulating a process using macrocarriers, but also to simulate an entire vaccine production process, from cell adsorption, cell growth, infection and vaccine virus production.

Published

2022

7. Optimization of VSV-ΔG-spike production process with the Ambr15 system for a SARS-COV-2 vaccine

Author

Osnat Rosen, Avital Jayson, Michael Goldvaser, Eyal Dor, Arik Monash, Lilach Levin, Lilach Cherry, Edith Lupu, Niva Natan, Meni Girshengorn, and Eyal Epstein

Subjects

COVID-19 Vaccines, SARS-CoV-2, Chlorocebus aethiops, Spike Glycoprotein, Coronavirus, Animals, COVID-19, Humans, Bioengineering, Applied Microbiology and Biotechnology, Vero Cells, Biotechnology

Abstract

To face the coronavirus disease 2019 pandemic caused by the severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) virus, our institute has developed the rVSV-ΔG-spike vaccine, in which the glycoprotein of vesicular stomatitis virus (VSV) was replaced by the spike protein of SARS-CoV-2. Many process parameters can influence production yield. To maximize virus vaccine yield, each parameter should be tested independently and in combination with others. Here, we report the optimization of the production of the VSV-ΔG-spike vaccine in Vero cells using the Ambr15 system. This system facilitates high-throughput screening of process parameters, as it contains 24 individually controlled, single-use stirred-tank minireactors. During optimization, critical parameters were tested. Those parameters included: cell densities; the multiplicity of infection; virus production temperature; medium addition and medium exchange; and supplementation of glucose in the virus production step. Virus production temperature, medium addition, and medium exchange were all found to significantly influence the yield. The optimized parameters were tested in the BioBLU 5p bioreactors production process and those that were found to contribute to the vaccine yield were integrated into the final process. The findings of this study demonstrate that an Ambr15 system is an effective tool for bioprocess optimization of vaccine production using macrocarriers and that the combination of production temperature, rate of medium addition, and medium exchange significantly improved virus yield.

Published

2022

8. Highly Efficient Purification of Recombinant VSV-∆G-Spike Vaccine against SARS-CoV-2 by Flow-Through Chromatography

Author

Rona Levy, Edith Lupu, Meni Girshengorn, Yaakov Adar, Ran Zichel, Eyal Dor, Eyal Epstein, Yaron Kafri, Arik Makovitzki, Ziv Oren, Niva Natan, Einat Toister, Elad Lerer, Arik Monash, Lilach Cherry, and Lilach Levin

Subjects

Infectivity, Chromatography, biology, Chemistry, Elution, SARS-CoV-2, Biomedical Engineering, Ultrafiltration, Bioengineering, biology.organism_classification, Applied Microbiology and Biotechnology, Biochemistry, Virus, downstream process, law.invention, Membrane, Column chromatography, law, Vesicular stomatitis virus, Recombinant DNA, rVSV, chromatography, TP248.13-248.65, membrane adsorbers, Biotechnology

Abstract

This study reports a highly efficient, rapid one-step purification process for the production of the recombinant vesicular stomatitis virus-based vaccine, rVSV-∆G-spike (rVSV-S), recently developed by the Israel Institute for Biological Research (IIBR) for the prevention of COVID-19. Several purification strategies are evaluated using a variety of chromatography methods, including membrane adsorbers and packed-bed ion-exchange chromatography. Cell harvest is initially treated with endonuclease, clarified, and further concentrated by ultrafiltration before chromatography purification. The use of anion-exchange chromatography in all forms results in strong binding of the virus to the media, necessitating a high salt concentration for elution. The large virus and spike protein binds very strongly to the high surface area of the membrane adsorbents, resulting in poor virus recovery (&lt, 15%), while the use of packed-bed chromatography, where the surface area is smaller, achieves better recovery (up to 33%). Finally, a highly efficient chromatography purification process with CaptoTM Core 700 resin, which does not require binding and the elution of the virus, is described. rVSV-S cannot enter the inner pores of the resin and is collected in the flow-through eluent. Purification of the rVSV-S virus with CaptoTM Core 700 resulted in viral infectivity above 85% for this step, with the efficient removal of host cell proteins, consistent with regulatory requirements. Similar results were obtained without an initial ultrafiltration step.

Published

2021

9. Evaluation of a downstream process for the recovery and concentration of a Cell-Culture-Derived rVSV-Spike COVID-19 vaccine candidate

Author

Meni Girshengorn, Ofir Israeli, Lilach Cherry, Edith Lupu, Arnon Tal, Rona Levy, Osnat Rosen, Arik Monash, Einat Toister, Yaron Kafri, Arik Makovitzki, Lilach Levin, Irit Simon, Eyal Dor, Ziv Oren, Elad Lerer, Idan Hefetz, Hanan Tzadok, Yaakov Adar, Eyal Epstein, and Ophir Hazan

Subjects

PES, polyethersulfone, rVSV-S, recombinant vesicular stomatitis virus-ΔG-spike, COVID-19 Vaccines, MWCO, molecular weight cutoff, Coronavirus disease 2019 (COVID-19), Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), PFU, plaque-forming units, TMP, transmembrane pressure, ACE2, angiotensin-converting enzyme 2, DSP, downstream process, Article, MEM, minimal essential medium, HF-TFF, hollow fiber-tangential flow filtration, Downstream (manufacturing), rVSV, SFM, serum-free medium, Animals, Humans, hc-DNA, host cell DNA, DO, dissolved oxygen, Pandemics, Infectivity, MOI, multiplicities of infection, Downstream process, General Veterinary, General Immunology and Microbiology, Chemistry, SARS-CoV-2, Public Health, Environmental and Occupational Health, Spike Protein, COVID-19, Endonuclease digestion, Antibodies, Neutralizing, Cell biology, Clarification, MT, multi-tray, Infectious Diseases, Recombinant viral vaccine, Cell culture, Spike Glycoprotein, Coronavirus, Nucleic acid, Molecular Medicine, Hollow fiber, HCP, host cell protein, NTU, nephelometric turbidity units, HR, horseradish peroxidase

Abstract

rVSV-Spike (rVSV-S) is a recombinant viral vaccine candidate under development to control the COVID-19 pandemic and is currently in phase II clinical trials. rVSV-S induces neutralizing antibodies and protects against SARS-CoV-2 infection in animal models. Bringing rVSV-S to clinical trials required the development of a scalable downstream process for the production of rVSV-S that can meet regulatory guidelines. The objective of this study was the development of the first downstream unit operations for cell-culture-derived rVSV-S, namely, the removal of nucleic acid contamination, the clarification and concentration of viral harvested supernatant, and buffer exchange. Retaining the infectivity of the rVSV-S during the downstream process was challenged by the shear sensitivity of the enveloped rVSV-S and its membrane protruding spike protein. Through a series of screening experiments, we evaluated and established the required endonuclease treatment conditions, filter train composition, and hollow fiber-tangential flow filtration parameters to remove large particles, reduce the load of impurities, and concentrate and exchange the buffer while retaining rVSV-S infectivity. The combined effect of the first unit operations on viral recovery and the removal of critical impurities was examined during scale-up experiments. Overall, approximately 40% of viral recovery was obtained and the regulatory requirements of less than 10 ng host cell DNA per dose were met. However, while 86–97% of the host cell proteins were removed, the regulatory acceptable HCP levels were not achieved, requiring subsequent purification and polishing steps. The results we obtained during the scale-up experiments were similar to those obtained during the screening experiments, indicating the scalability of the process. The findings of this study set the foundation for the development of a complete downstream manufacturing process, requiring subsequent purification and polishing unit operations for clinical preparations of rVSV-S.

Published

2021